Abstract
Dopamine (DA) neurons of the ventrolateral periaqueductal gray (vlPAG) and dorsal raphe nucleus (DRN) fire spontaneous action potentials (APs) at slow, regular patterns in vitro but a detailed account of their intrinsic membrane properties responsible for spontaneous firing is currently lacking. To resolve this, we performed a voltage-clamp electrophysiological study in brain slices to describe their major ionic currents and then constructed a computer model and used simulations to understand the mechanisms behind autorhythmicity in silico. We found that vlPAG/DRN DA neurons exhibit a number of voltage-dependent currents activating in the subthreshold range including, a hyperpolarization-activated cation current (IH), a transient, A-type, potassium current (IA), a background, ‘persistent’ (INaP) sodium current and a transient, low voltage activated (LVA) calcium current (ICaLVA). Brain slice pharmacology, in good agreement with computer simulations, showed that spontaneous firing occurred independently of IH, IA or calcium currents. In contrast, when blocking sodium currents, spontaneous firing ceased and a stable, non-oscillating membrane potential below AP threshold was attained. Using the DA neuron model we further show that calcium currents exhibit little activation (compared to sodium) during the interspike interval (ISI) repolarization while, any individual potassium current alone, whose blockade positively modulated AP firing frequency, is not required for spontaneous firing. Instead, blockade of a number of potassium currents simultaneously is necessary to eliminate autorhythmicity. Repolarization during ISI is mediated initially via the deactivation of the delayed rectifier potassium current, while a sodium background ‘persistent’ current is essentially indispensable for autorhythmicity by driving repolarization towards AP threshold.
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1 Introduction
Studies of physiological characteristics of dopamine (DA) neurons have been largely concentrated around the midbrain areas of substantia nigra pars compacta (SNc) and ventral tegmental area (VTA) due to their well-known importance in motor control and reward processing (Schultz 1998; Pollack 2001). Midbrain DA neurons fire spontaneous action potentials (APs) at 3–8 Hz in a tonic or bursting manner in vivo (Grace and Bunney 1983a, 1983b; Grace and Bunney 1984a, 1984b) and maintain spontaneous tonic (but not bursting) firing at 1–10 Hz even in the absence of synaptic transmission in vitro (Grace and Onn 1989; Lacey et al. 1989; Puopolo et al. 2007; Lammel et al. 2008; Khaliq and Bean 2010). Through intensive research using the in vitro brain slice preparation and/or dissociated cell preparations a number of intrinsic ionic currents have been described to modulate firing frequency of midbrain DA neurons including, a hyperpolarization-activated cation current [IH] (Seutin et al. 2001; Neuhoff et al. 2002), an A-type potassium current [IA] (Liss et al. 2001; Koyama and Appel 2006a; Khaliq and Bean 2008; Kimm and Bean 2014; Subramaniam et al. 2014), an M-type potassium current [IM] (Hansen et al. 2006; Koyama and Appel 2006b; Koyama et al. 2007; Drion et al. 2010), an apamin-sensitive, calcium-activated potassium current [ISK] (Wolfart et al. 2001; Koyama et al. 2005; Bishop et al. 2010; Deignan et al. 2012), an iberiotoxin-sensitive calcium-activated potassium current [IBK] (Kimm et al. 2015), a delayed rectifier potassium current [IKdr] (Silva et al. 1990; Kimm et al. 2015), transient (low voltage activated, LVA) and persistent (high voltage activated, HVA) calcium currents [ICaLVA and ICaHVA] (Kang and Kitai 1993a, 1993b; Wolfart and Roeper 2002; Branch et al. 2014; Poetschke et al. 2015; Philippart et al. 2016) and background ‘persistent’ and transient sodium currents [INaP and INaT] (Puopolo et al. 2007; Khaliq and Bean 2010; Ding et al. 2011).
The tonic-firing pacemaking mechanism of SNc and VTA midbrain DA neurons seem to differ in at least two important ways. First, IH current inhibition decreases pacemaker firing frequency in some SNc neurons but not in VTA neurons (Neuhoff et al. 2002; Khaliq and Bean 2010) arguing that IH current may have a role in pacemaking in SNc neurons but it is not essential for autorhythmicity in either group. It is noteworthy that VTA neurons, especially those projecting to the prefrontal cortex, lack a prominent expression of an IH current (Margolis et al. 2006; Lammel et al. 2008). Second, during the interspike interval (ISI), SNc neurons rely substantially on subthreshold calcium conductances to repolarise to AP threshold (Wilson and Callaway 2000; Chan et al. 2007; Puopolo et al. 2007; Putzier et al. 2009) and to a far lesser degree on sodium conductances (Puopolo et al. 2007; Khaliq and Bean 2010). Interestingly, the opposite is true for VTA neurons that, rely heavily on both voltage-dependent, TTX-sensitive and voltage-independent, TTX-resistant, background ‘persistent’ sodium currents to repolarise to AP threshold during ISI (Khaliq and Bean 2010). SNc pacemaker firing frequency can be often greatly reduced or even halted by L-type calcium channel blockers (Nedergaard et al. 1993; Mercuri et al. 1994; Puopolo et al. 2007; Putzier et al. 2009, but see also Chan et al. 2007, Guzman et al. 2009, Poetschke et al. 2015) or abolished by cadmium (Puopolo et al. 2007) suggesting that calcium currents are indispensable for SNc autorhythmicity although the impact of L-type blockers on firing rate of SNc DA neurons is often hard to reproduce for reasons that are not clear (see Chan et al. 2007; Guzman et al. 2009; see also explanations provided in modeling study by Drion et al. 2011). In contrast, in VTA neurons, the absence of external calcium speeds rather than abolishes the pacemaker firing frequency (Khaliq and Bean 2010), whereas blockade of a TTX-sensitive sodium current resulted in a stable resting membrane potential (negative to AP threshold) with no evidence of background oscillations, a situation unlike to what has been reported for SNc neurons that exhibit calcium-mediated small oscillating potentials (SOP) in the presence of sodium channel blockers (Nedergaard et al. 1993; Mercuri et al. 1994; Chan et al. 2007; Puopolo et al. 2007; Guzman et al. 2009). The presumed qualitative difference in the mechanism of pacemaking in VTA neurons and SNc neurons, in that there is little role of subthreshold calcium current in driving pacemaking in VTA neurons, also supports the hypothesis that the selective vulnerability of SNc DA neurons in Parkinson’s disease (as opposed to the selective sparring of VTA neurons, see Mosharov et al. 2009; Surmeier and Schumacker 2013) may depend on this prominent calcium entry during pacemaking cycles and its link to mitochondrial potential flickering and oxidative stress (Guzman et al. 2010; Surmeier et al. 2011; Philippart et al. 2016). Given the diversity of the functional phenotypes of midbrain DA neurons based on their neuroanatomical positioning and projection targets (Lammel et al. 2008, 2011; Poulin et al. 2014; Beier et al. 2015; Lerner et al. 2015), it is likely that the VTA and SNc DA neuronal subgroups may utilise a multitude of mechanisms under different circumstances to maintain tonic firing (e.g. see results in Chan et al. 2007; Puopolo et al. 2007; Guzman et al. 2009; Poetschke et al. 2015) which in turn could influence to a different degree the neuron’s propensity for degeneration.
The ventrolateral periaqueductal grey (vlPAG) and dorsal raphe nucleus (DRN) regions contain a population of DA neurons, often considered to be a dorsocaudal extension of the VTA area towards the brainstem, termed collectively the A10dc system (Hokfelt et al. 1984). These DA neurons may play a role in wakefulness (Lu et al. 2006), opiate antinociception (Flores et al. 2004; Li et al. 2016), drug reward (Flores et al. 2006; Li et al. 2013) while they have been recently shown to encode the experience of social isolation (Matthews et al. 2016). Using the pitx3-GFP and TH-GFP transgenic mouse models as an aid to identification of DA neuron phenotype, we have previously reported the physiological characteristics of DA vlPAG/DRN neurons in vitro under current-clamp (regular firing with broad APs at a range 1-10 Hz and spike-frequency adaptation in response to prolonged depolarization, Dougalis et al. 2012). Interestingly during our studies we have also noted that spontaneous tonic firing of DA vlPAG/DRN neurons in vitro can persist in the absence of glutamatergic and GABAergic synaptic transmission but the mechanism behind this property is not known despite the availability of such data for SNc and VTA, midbrain DA neuronal groups (see Grace and Onn 1989; Silva et al. 1990; Puopolo et al. 2007; Khaliq and Bean 2010). To resolve this, we have conducted a voltage-clamp study to provide a kinetic description of major sodium, potassium and calcium ionic currents operant on DA vlPAG/DRN neurons in brain slices. Based on experimentally derived voltage-clamp data, we then constructed a simplified, conductance-based, Hodgkin and Huxley-type, computer model and validated its behaviour against in vitro neurophysiological data. Using simulations in the computational DA model, we explored the contribution of individual ionic currents in vlPAG/DRN DA neuron’s spontaneous firing, pacemaker frequency and threshold for spike frequency adaptation in silico.
2 Methods
2.1 Brain slice preparation
Three to six months old, male, GFP-pitx3 heterozygous mice (transgenic line generated as described previously, see Zhao et al. 2004) were sacrificed by isoflurane anaesthesia followed by decapitation. All breeding and experimental procedures were conducted in accordance with the Animals (Scientific Procedures) Act of 1986 (United Kingdom) or were approved by the German Regierungspräsidium Tübingen (AZ 35/9185.81–3. TV1043, Reg. Nr. 0.147). The brain was rapidly removed out of the cranial cavity and bathed with ice-cold (0–2 °C), fully equilibrated (with carbogen gas, 95% carbon dioxide and 5% oxygen) artificial celebrospinal fluid (aCSF, composition in mM, NaCl 120, KCl 3.5, NaH2PO4 1.25, NaHCO3 26, Glucose 10, MgCl2 1, CaCl2 2). Two or three thin coronal brain slices (220 μm thickness) encompassing the dorsal raphe nucleus (DRN) were obtained using a vibratome (Leica VT1000S, Germany) and were maintained into a standard in-house-made maintenance chamber (Edwards et al. 1989) gently and continuously aerated with carbogen gas for at least one and a half hours at room temperature (20–22 °C) before use for electrophysiology.
2.2 Neuron identification
Slices were transferred to a submersion recording chamber and were continuously perfused at a rate of 2–4 ml/min with fully oxygenated aCSF (composition as above) at 35.5 °C (± 0.5 °C) for at least 30 min before attempting recordings. Whole-cell current and voltage-clamp recordings were obtained from DA neurons using infra-red differential interference contract (IR-DIC) videomicroscopy as described previously (Stuart et al. 1993). In short, neurons were visualized under an upright microscope equipped with ×40 or ×60 objectives, an IR filter, DIC optics and a charged cooled diode (CCD) video camera. GFP-pitx3 DA neurons were firstly identified in the slice by using fluorescence illumination coupled to a GFP excitation filter and then further visualized under IR-DIC conditions prior to electrophysiology. For comparative purposes, in some experiments, we also obtained targeted recordings from SNc and VTA DA neurons as described previously (Bishop et al. 2010).
2.3 Electrophysiology
Tight seal (>10 GΩ) whole-cell, current-clamp recordings were performed with a Multiclamp 700B amplifier (Molecular Devices), while voltage-clamp recordings were performed with an Axopatch 200A (Molecular Devices) or an EPC-10 (HEKA Electronics, Germany) using glass microelectrodes (3–6 MΩ in resistance) filled with a standard internal solution containing (in mM) 140 potassium gluconate (KGlu), 5 NaCl, 1 MgCl2, 10 HEPES, 1 EGTA, 2 MgATP and 0.5 LiGTP, pH 7.25–7.35, osmolality 280–290 mosmol/l. For voltage-clamp recordings aiming to isolate specific ionic currents, internal and external solutions were modified accordingly depending on the current under investigation (see descriptive text below in solutions and voltage-clamp protocols for ionic currents). Series resistance (Rs) and input resistance (Rin) were frequently monitored throughout the experiments via at 10 mV, 250 ms hyperpolarizing step under voltage-clamp. Rs value was <13 MΩ (average 8.3 ± 1.1 MΩ, n = 40) for all recordings and was compensated by approximately 60–90% leaving on average an uncompensated Rs of 3.2 MΩ (range, 2.5–7 MΩ) and an estimated error in voltage-clamp command potentials when recording an one nanoampere current under most circumstances of <5 mV. Whole-cell capacitive transients were evaluated under voltage-clamp through a 10 mV step (−50 to −60 mV) and were negated using the amplifier’s circuitry. The recorded neurons had an average CW of 7.8 ± 0.4 pF (n = 40, range, 4.5 to 12.0 pF). Currents were filtered at 1 KHz (low-pass), collected at 3–5 KHz through an A/D converter (PC-5230, National Instruments, USA) on WINWCP (University of Strathclyde, courtesy of Dr. John Dempster) or via an onboard card from EPC-10 to PatchMaster software (HEKA Electronics, Germany) and stored for offline analysis. The combination of our intracellular and extracellular recording solutions lead to an estimated liquid junction potential (LJP) of +7 and +12 mV for the cesium methanesulphonate (CsMe) and KGlu filled electrodes respectively (measured in pClamp10 calculator). Holding voltages reported herein for electrophysiological experiments have been corrected by this amount.
2.4 Solutions and pharmacology
The standard KGlu internal solution (detailed above) was used in voltage-clamp experiments isolating sustained (IKdr and IM) and transient (IA) potassium currents as well as the hyperpolarization-activated cation current (IH). In these experiments the aCSF was supplemented with tetrodotoxin (TTX, 1 μM). For experiments involving calcium, barium and sodium current isolation, KGlu was substituted for CsMe (120 mM) and tetraethylammonium (TEA, 20 mM) in internal solutions. External aCSF solution’s NaCl concentration was reduced to 100 mM and was supplemented with 20 mM TEA, 2 mM 4-aminopyridine (4-AP) and 1 μM TTX for calcium/barium current recordings. Barium chloride (BaCl2) substituted calcium chloride in the external solution for barium current recordings (1 mM BaCl2 for 2 mM CaCl2). For isolation of sodium currents we included 1 mM BaCl2 in external aCSF and replaced TTX with cadmium chloride (200 μM). Osmolality in all above aCSF solutions was kept constant at 300 mosmol/l by equivalent reductions in NaCl when more than 2 mM additions were made. All drugs used in this study for formulating external and internal solutions were bought from Sigma-Aldrich (UK) apart from 2,3-dihydroxy-6-nitro-7-sulfamoyl-benzo[f]quinoxaline-2,3-dione (NBQX), tetrodotoxin (TTX), 10,10-bis(4-Pyridinylmethyl)-9(10H)-anthracenone dihydrochloride (XE991) and 4-Ethylphenylamino-1,2-dimethyl-6-ethylaminopyrimidinine (ZD7288) which were bought from Tocris (UK). For pharmacological investigations, drugs were made fresh from appropriately concentrated aliquots stored according to the manufacturer’s recommendations. All drugs were dissolved on the day in freshly prepared oxygenated aCSF and superfused on the tissue for 10 min to achieve steady-state concentration in the intima of the brain slices before any measurements were taken.
2.5 Voltage-clamp protocols for ionic currents
2.5.1 Hyperpolarization-activated cation current (IH)
Neurons were voltage-clamped at −47 mV and hyperpolarizing steps of 1 s in duration were delivered in 10 mV decrements from −62 to −152 mV in the presence of TTX (1 μM) using a standard KGlu based-internal solution. Determination of IH current amplitude at potentials more negative than −152 mV was not routinely attempted as this lead to loss of recording. IH currents were measured as slowly activating inward currents calculated from the difference of the instantaneous currents and the steady-state currents, in the first 5–20 ms after the beginning and 25 ms before the end of the hyperpolarizing voltage step respectively, at each test holding potential.
2.5.2 A-type (IA) and delayed rectifier (IKdr) potassium currents
IA currents were isolated by digital subtraction of currents between two specific voltage-clamp protocols using a standard KGlu based-internal solution in the presence of TTX (1 μM) as reported previously (Koyama and Appel 2006a). IA current amplitude was measured from peak till 25 ms before the end of the inactivating current during the 1 s long pulses used in our study. To study IA current steady-state activation, neurons were held at −72 mV and a 250 ms hyperpolarizing prepulse to −112 mV was used to facilitate the recovery from inactivation of the IA current. Subsequently the neurons were stepped to the test voltage from −92 to +18 mV in 10 mV increments for 1 s to activate and record the resultant IA current transient and its inactivation (protocol 1). In the second protocol, neurons were held at −72 mV and a 250 ms prepulse to −52 mV was given to facilitate the inactivation of the IA transient current before stepping the neurons from −92 to +18 mV in 10 mV increments for 1 s (protocol 2). Currents obtained from the second protocol were slowly activating sustained outward currents reminiscent of a delayed rectifier (IKdr) and were subtracted from the currents obtained from protocol 1 to obtain the IA current. To study IA current steady-state inactivation, neurons were held at −47 mV and a 250 ms prepulse was given from -152 mV to −52 mV (in 10 mV increments) before stepping the neuron to the test voltage of −47 mV for 1 s to record the extend of IA current inactivation as a function of the prepulse holding voltage. Current subtraction was not necessary for steady-state inactivation experiments because the fast peak of IA current was not contaminated by the slowly activating sustained currents at the test voltage of −47 mV. We also obtained IA currents via a single activation voltage protocol (protocol 1 described above) in the presence of 10 mM TEA (to block IKdr potassium currents) as described previously (Silva et al. 1990) to compare the results obtained via the two protocol subtraction method. Finally, IA currents were also isolated via a third method using protocol 1 above in the presence of TEA (10 mM) by current subtraction after the addition of 2 mM 4-AP to reveal the 4-AP sensitive component. IKdr currents were isolated using a KGlu based-internal solution in the presence of TTX (1 μM) as reported previously (Silva et al. 1990) using a modified protocol 2 detailed above. To study IKdr current steady-state activation neurons were held at −72 mV and a 250 ms hyperpolarizing prepulse to −52 mV was used to facilitate the inactivation of the IA transient current. Subsequently the neurons were stepped to the test voltage from −92 to +18 mV in 10 mV increments for 1 s to activate and record the resultant slowly-activating sustained IKdr current. Current amplitude was measured 25 ms before the end of the depolarizing step.
2.5.3 M-type (IM) potassium currents
IMcurrents were isolated using a standard deactivation protocol in KGlu-based internal solution in the presence of TTX (1 μM) as reported previously (Koyama and Appel 2006b). The neurons were held at −72 mV and were given a depolarizing prepulse to −32 mV for 1 s before stepped down to the test voltage from −42 to −72 mV in 10 mV decrements for 1 s to record the resultant IM current deactivation tail.
2.5.4 Calcium and Barium currents (ICa and IBa)
Low and high threshold voltage-activated (LVA and HVA) inward calcium/barium currents (LVA and HVA) were isolated using a combination of blockers in both internal and external solutions in an attempt to block potassium and sodium conductances as described previously (Brevi et al. 2001). Neurons were bathed in TTX (1 μM), 4-AP (2 mM) and TEA (20 mM) and recorded with CsMe (120 mM) and TEA (20 mM) based internal solutions. For ICa experiments, neurons were held at −67 mV and were depolarized to the test voltage from −57 to +3 mV in 10 mV increments for 250 ms. Calcium currents recorded through this protocol would inactivate with different time constants during our steps at nearly all potentials. This inactivation could theoretically result from calcium-mediated intracellular calcium release (that can induce calcium channel inactivation) or it could be directly related to the kinetic, voltage-dependent properties of the calcium channels (Giannattasio et al. 1991; Haack and Rosenberg 1994; Catterall 2000; Budde et al. 2002). To reduce the amount of inactivation seen with calcium and discriminate better between these two possibilities we have used barium ions (1 mM) instead of calcium (2 mM) as the charge carrier, since barium currents undergo significantly less inactivation during long steps than calcium currents (see Hille 2001). Furthermore, to ascertain the presence of LVA currents we recorded barium currents from a more hyperpolarized potential (−87 mV). IBa were recorded via two different protocols essentially used to isolate LVA/HVA or HVA currents alone (Brevi et al. 2001). Neurons were held at either −87 mV (LVA/HVA protocol) or −67 mV (HVA protocol) and were depolarized in 10 mV increments for 250 ms to +3 mV. Current subtraction was used to isolate the LVA component from LVA/HVA protocol by subtracting the HVA protocol currents. As an alternative method to study calcium and barium currents, we employed fast voltage-ramps (200–500 mV/s, from −107 to +13 mV) to measure the background flowing currents at different potentials after leak current subtraction.
2.5.5 Sodium currents (INa)
Fast transient (INaT) and persistent (INaP) sodium currents were recorded from neurons bathed in TEA (20 mM), barium chloride (1 mM) and cadmium chloride (200 μM) using CsMe/TEA (120/20 mM)-based internal solutions as reported previously (Pignatelli et al. 2005; Magistretti et al. 2006). Neurons were held at −107 mV and a depolarizing prepulse of 5 ms in duration was delivered to −47 mV to activate unclamped axonal sodium currents, before hyperpolarizing the neuron to −77 mV for 4 ms and then step wise depolarizing it (in 5 mV increments from −77 to +13 mV for 110 ms) to sample somatic INa current activation devoid of axonal contamination as described previously (Milescu et al. 2010). To study steady-state inactivation of transient somatic sodium currents, neurons were subjected to the above protocol with a prepulse to −47 to activate and inactivate axonal sodium currents but then were given a 4 ms variable hyperpolarizing step from −77 to −42 mV (in 5 mV steps) before measuring the somatic sodium current at the test potential of −37 mV (held for 20 ms). The amplitude of the background ‘persistent’ sodium current was measured 10 ms before the end of the depolarizing steps and of the transient sodium current at the peak of the response during the steady state activation/inactivation protocol. We also sampled persistent non-inactivating sodium currents via an alternative method by subjecting neurons to slow voltage ramps (16 mV/s, from −107 to +53 mV) and leak current substraction in the presence of the above blocking solutions.
2.6 Current-clamp experiments
The standard KGlu internal solution and standard external aCSF (as detailed above) were used in all current-clamp experiments unless otherwise indicated in text. Experiments were conducted in the presence of NBQX (5 μM) and picrotoxin (25 μM) to block excitatory and inhibitory synaptic activity respectively.
2.7 Voltage-clamp data analysis
Voltage-clamped currents were averaged in three to five trials at each test holding voltage. We employed capacitive transient artifact and leak subtraction for sodium and calcium inward conductance using a modified P/4 protocol off-line. Averaged currents from different protocols were exported as text files (.txt) for subtraction in Excel spreadsheets and were then imported into Spike2 (Cambridge electronic design, CED, UK) for measurements and exponential function fitting. Data transformations, statistical analysis and fitting of single order Boltzmann function to the data set were performed in Prism software (version 7, GraphPad, USA).
Measured current amplitude at peak (or steady-state) was converted into conductance at any given holding potential by using eq. (1) below
where, G represents the current conductance at a given test holding voltage V, while I is the current amplitude at the given holding voltage and Erev is the equilibrium potential (calculated using the Nernst equation) of the current under investigation. The Nernst equation yielded for our conditions (35 °C) an estimated equilibrium potential of −105, +135, +75 mV for the major ions (EK+, ECa++, ENa+, respectively).
To construct steady-state activation (or inactivation) curves we normalized conductance to its maximal value and plotted it against holding voltage (G/Gmax against holding voltage). The data were then fitted with a single first order Boltzmann function using eq. (2) below
where, G is the conductance at the holding test voltage of V, Gmax is the maximal conductance set to be 1 and Gmin is the minimum conductance set to be 0, V50 is the membrane potential for half-maximal activation and s is the slope factor of the activation/inactivation curve.
To measure the activation and inactivation time constants currents were fitted from start to peak (activation time constant) or from peak to end (inactivation time constant) with a single exponential function according to the eq. (3) below
where, I is the current amplitude at time t and Imax is the maximal current amplitude, while τ is the time constant. In some currents (e.g. sodium currents and A-type potassium currents), inactivation was best described by two exponential function fitting at most holding voltages. These currents were fitted accordingly with following eq. (4) for bi-exponential inactivation
where, I is the total current amplitude at time t, Imax(f) is the maximal current amplitude of the first (fast) inactivating component of the current and Imax(s) is the maximal current amplitude of the second (slow) inactivating component of the current, while τf and τs are the fast and the slow component inactivation time constants respectively. Decision on using mono versus bi-exponential fitting was guided by inspection of the residual value table and compared by using the R value and the standard deviation for the fit. Calculated time constants were plotted against holding voltage and were fitted a single order modified first order Boltzmann function [eq. (5)] to calculate the voltage to attain half-maximal activation/inactivation time constant (V50 value) and its corresponding slope factor.
where, τ is the activation/inactivation time constant at the holding test voltage of V, τmax is the maximal value of the time constant, τmin is the minimum value of the time constant, V50 is the membrane potential where time constant is half maximal and s is the slope factor of the time constant curve.
2.8 Current-clamp data analysis
All neurons were monitored frequently for stability of series resistance (Rs) and input resistance through the recording and during pharmacological investigations. Rs did not exceed 25 MΩ in our recordings. Action potentials (APs) and accompanying afterhyperpolarization (AHP) were averaged during epochs of interest (100–200 APs) in Spike2 software (CED, UK) and their characteristics were calculated (AP amplitude, AP width, AHP amplitude, AHP repolarization) with respect to the AP threshold (defined as the point where the rate of voltage change exceeded 10 mV/ms, calculated through the first differential of the voltage trace). Average firing rate for each cell was calculated from the inverse of the average interspike interval (ISI) from ISI histograms while the coefficient of variation of the ISI was calculated as the ratio of the standard deviation (SD) of the ISI to the mean ISI. Hyperpolarizing current injections (−10 to −120 pA, 1000 ms in duration) were used to ascertain the extent of IH current activation (referred to as the IH current-mediated voltage-sag) and of the extent of IA current activation (referred to as delayed repolarization). The voltage-sag was measured during the hyperpolarizing step as the voltage difference from the peak of the voltage response at the beginning of the step (occurring in the first 50–100 ms from step initiation) till 20 ms before the end of the hyperpolarizing step. Delayed repolarization was measured at the termination of the hyperpolarizing step as the time from step termination till the firing of the first AP. Depolarizing current injections (+10 to +120 pA, 1000 ms in duration) were used to elicit APs and measure the gain (input-output relationship) of vlPAG/DRN DA neurons. We measured instantaneous firing frequency by using the first two APs elicited by the depolarizing step. Sustained firing frequency was measured as the mean AP firing frequency during the last 100 ms of the depolarizing step as described previously (Dougalis et al. 2012).
2.9 Statistical data analysis
All values reported represent mean ± standard error of the mean (s.e.m). The n number reported for each experiment represents replicated observations in different neurons from slices obtained from a minimum of three different animals (range of 3–5 per experiment as indicated in results section for each experiment). A P value of less than 0.05 was taken to indicate significance using a paired or unpaired t-test as appropriate for pair-wise comparisons or one-way analysis of variance (ANOVA) followed by Tukey’s multiple comparison test.
2.10 Modelling and computer simulations
The DA neuron was modelled using NEURON software (Hines and Carnevale 1997, available freely at https://www.neuron.yale.edu/neuron/) as a single compartment, spherical neuron of 15 μm in diameter. General model assumptions and specific model equations used in the construction of the model are detailed in the appendix. The model code will be deposited and will be freely available through the modelDB database (https://senselab.med.yale.edu/modeldb/) following article publication (also available through direct request to the authors). Electrophysiological data were collected at 35 °C and thus the model replicates behaviour at this temperature. The model DA neuron was constructed to operate through eight Hodgkin and Huxley-type conductances (INaT, INaP, IKdr, IA, IM, IH, ICaHVA, ICaLVA) and a leak conductance. Since it is not possible to examine electrophysiologically a single neuron for all conductances, the values derived for any conductance represent mean values over a population of different neurons examined and these were used in the model unless otherwise stated. All values used in the model (Table 1) were mean values taken from experimental data. In some cases, values were optimized by allowing use of mean ± one standard deviation of the reported experimental values where necessary to improve model functionality. For the operation of the model and in line with Hodgkin and Huxley (1952) we have used three activation gates for sodium currents and four activation gates for the delayed rectifier potassium current. Only one activation gate was used for calcium currents, IA current, IM and IH current as described previously (Xiao et al. 2004) and in line with our experimental fitting. Barium currents were shifted 10 mV more positive to mirror the V50 values for calcium currents. The leak current in the DA model was given a constant conductance of 0.04 mS/cm2 and an Erev of −55 mV based on experimental data of DA neurons mean input resistance (7 GΩ) and reversal potential in the presence of calcium, sodium and potassium channel blockers. Simulated responses (numerical integration in steps of 25 μs corresponding to a reconstruction frequency of 40 KHz) for the model DA neuron were exported programmatically from NEURON as text files (.txt) and imported in Spike2 (CED, UK) for measurements of membrane potential, firing frequency and action potential characteristics under basal and various test conditions.
3 Results
We used Pitx3-GFP mice that express GFP selectively in midbrain dopamine neurons (Zhao et al. 2004), to conduct targeted whole-cell recordings from vlPAG/DRN DA neurons in acute brain slices, an approach that we have previously described (Dougalis et al. 2012). Under these conditions, most DA neurons in the vlPAG/DRN fire action potentials spontaneously (Dougalis et al. 2012).
3.1 Hyperpolarization-activated cation current (IH)
Midbrain DA neurons express a hyperpolarization-activated inward current (IH) whose blockade can decrease pacemaker frequency of some, but not all, SNc DA neurons (see Neuhoff et al. 2002; Seutin et al. 2001; Khaliq and Bean 2010). The IH current recorded in vlPAG/DRN DA neurons was sensitive to the specific IH current blocker ZD7288 (30 μM) which completely ablated the inward currents recorded under a hyperpolarizing pulse from −62 to −132 mV in voltage-clamp (87 ± 4% current block, n = 6, from three mice, Fig. 1a). A series of hyperpolarizing pulses from −52 mV to −152 mV for 1 s in the presence of TTX (n = 6, three mice, Fig. 1b) resulted in IH current steady-state activation values for V50 and slope of −114.7 ± 1.7 mV and −12.7 ± 1.6 respectively (Fig. 1c). IH current activation time constant was voltage-dependent becoming faster at more positive potentials (2118 ± 664 ms at −102 mV and 151.0 ± 24 ms at −152 mV, n = 6, P < 0.001, paired t-test) with V50 and slope values of −112.7 ± 7.8 mV and 6.1 ± 5.1 respectively (Fig. 1d). Maximal IH conductance was calculated to be 0.56 ± 0.01 nS at −152 mV (n = 6). Results quantifying IH current steady-state activation and activation kinetics via a current subtraction protocol (before and after addition of ZD7288) did not differ from results obtained using the simplified activation voltage-clamp protocol used above and thus the subtraction protocol was not routinely used for measurements of IH current kinetics of vlPAG/DRN DA neurons (data not shown). To evaluate the impact of IH current blockade on autorhythmicity and pacemaker frequency of DA neurons, ZD7288 (30 μM) was perfused under current-clamp conditions while monitoring spontaneous firing in the presence of synaptic blockers for glutamatergic and GABAergic transmission (see methods). The IH current blocker, did not affect firing frequency of DA neurons (firing frequency in control, 3.1 ± 0.5 Hz; in ZD 7288, 3.5 ± 0.8 Hz, n = 7 from four mice, P > 0.05, paired t-test, Fig. 1e, g) or firing regularity (CV-ISI in control, 0.46 ± 0.07; in ZD7228, 0.44 ± 0.07, n = 7 from four mice, P > 0.05, paired t-test, Fig. 1h) despite eliminating the IH mediated voltage-sag under current-clamp induced by hyperpolarizing current injections (−60 pA for 1 s, Fig. 1f). For comparative purposes we also recorded IH current in SNc and VTA DA neurons (three mice). As expected, both midbrain nuclei responded with an inward current upon a series of hyperpolarizing voltage steps (from −62 to −132 mV in 10 mV increments, online resource 1A) albeit with evidently differential current steady-state activation midpoint (online resource 1B) and kinetics (online resource 1C). SNc neurons had more positive V50 values (SNc, −92 ± 2.3 mV, n = 6–7 for each set, P < 0.01 to both VTA and vlPAG/DRN, ANOVA with Tukey’s post-hoc test) for IH current activation and a significantly faster activation time constant (at −132 mV, SNc, 114 ± 14 ms, n = 6–7 for each set, P < 0.05 to both VTA and vlPAG/DRN, ANOVA with Tukey’s post-hoc test) than either VTA (−121 ± 5.6 mV and 397 ± 84 ms respectively) or vlPAG/DRN (−121 ± 3.5 mV and 260 ± 34 ms respectively) that exhibited comparable profiles without any significant differences between them in either parameter (VTA vs vlPAG/DRN, P > 0.05 for both comparisons, unpaired t-test). Also no differences were detected in the slope of the activation curve (slope, SNc, −11.8 ± 2.6; VTA, −12.0 ± 2.8; vlPAG/DRN, −13.0 ± 1.8, n = 6–7 for each set, P > 0.05, ANOVA with Tukey’s post-hoc test).
3.2 A-type (IA) transient potassium currents
One of the hallmarks of the electrophysiological behavior of DA neurons in the vlPAG/DRN brain slice is the pronounced outward tail current recorded at subthreshold potential (−60 to −50 mV) following a hyperpolarizing pulse (beyond −85 mV) under voltage-clamp (Fig. 2a). The amplitude of the outward transient tail conductance after a hyperpolarizing step was suppressed (90.1 ± 2.4% at −62 mV, n = 6 from three mice) by 2–3 mM 4-aminopyridine (4-AP) indicating that it represents an A-type transient outward potassium conductance (IA current, Fig. 2a, b). Subtraction of the 4-AP sensitive current lead to the typical ‘current crossing’ (Fig. 2c) as reported previously by others (Khaliq and Bean 2008) suggesting that 4-AP also increases some background conductance while blocking the IA current (and potentially blocking a fast delayed rectifier conductance in some neurons, see Itri et al. 2005) making its kinetic description difficult. An alternative method to examine IA current steady-state activation is using digital current subtraction between two different activation protocols in the presence of TTX (1 μM) as reported previously (Koyama and Appel 2006a). Responses to protocol one (Fig. 2d) activated transient and sustained outward currents while responses to protocol two activated slowly-activating sustained outward currents only (reminiscent of delayed rectifier potassium currents, Fig. 2d). Subtraction of the responses (protocol 1 minus protocol 2) resulted in isolation of the IA current (Fig. 2e). Steady-state inactivation was studied using a single standard inactivation protocol without digital current subtraction since the peak of the IA current at the test voltage studied (−47 mV) was not contaminated by slowly activating outward currents (Fig. 2f). Maximal IA conductance was calculated to be 10.0 ± 1.1 nS at +8 mV (n = 6, from four mice). The V50 value for steady-state activation was −57.5 ± 0.5 mV with a slope of 7.7 ± 0.4, while the corresponding values of V50 for steady-state inactivation and its slope were −87.4 ± 0.8 mV and −6.1 ± 0.8 respectively (n = 6, Fig. 2g). Activation time constant for IA current was voltage-dependent becoming faster at more positive potentials (5.45 ± 0.27 ms at −62 mV and 0.95 ± 0.06 ms at +8 mV, n = 6, P < 0.001, paired t-test) with a V50 and slope values of −68.8 ± 0.7 mV and −5.0 ± 0.7 respectively (Fig. 2h). Inactivation kinetics were also voltage-dependent with faster inactivation at more positive potentials (128.3 ± 9.5 ms at −62 mV and 50.8 ± 10.0 ms at +8 mV, n = 6, P < 0.01, paired t-test) with V50 and slope values of −24.6 ± 5.7 mV and −8.6 ± 5.3 respectively (Fig. 2i). A second, voltage-independent, slow inactivation time constant (τslow) could be fitted to IA currents recorded more positively than −30 mV and contributed to approximately 35% and 50% of the maximal IA current amplitude recorded at −22 and +8 mV respectively (357 ± 53 ms at −22 mV and 562 ± 106 ms at +8 mV, n = 6, P > 0.05, paired t-test, online resource 2A). We did not further investigate the origin of this slow conductance but we noted interestingly that 4-AP subtracted currents (as shown in Fig. 2c) not only exhibited a similar average activation steady-state curve (V50 of −61.4 ± 0.9 and slope of 7.1 ± 0.8, n = 3, online resource 2B) to currents recorded here with the two protocol current subtraction method, but more importantly, 4-AP sensitive currents also exhibited consistently a bi-exponential decay with commensurate, voltage-dependent, fast and slow inactivation time constants that differentially contributed to current amplitude at a range of holding voltages (online resource 2C, D). To examine further the properties of IA currents and to compare our results obtained with the methods described above we recruited IA currents via a single activation protocol (protocol 1) in the presence of 10 mM TEA (as described previously by Silva et al. 1990) a method that does not rely on digital current subtraction. This resulted in recording IA currents (Fig. 2j) with analogous average activation steady-state V50 of −55.6 ± 1.0 mV, but shallower activation slope of 15.1 ± 1.1 (n = 5, from three mice, online resource 2E), to the two protocol subtraction method and the 4-AP-sensitive IA currents. Interestingly, the single protocol IA current isolation in TEA also resulted in a bi-exponential inactivation of recorded IA currents with differential contributions to current amplitude at different voltages (online resource 2F, G). However, unlike the previous methods, inactivation kinetics under these circumstances did not exhibit strong voltage dependence at positive potentials (online resource 2F). Both 4-AP-sensitive IA currents and IA currents isolated in TEA exhibited commensurate voltage-dependent activation kinetics (faster at more positive potentials) in good agreement with the two protocol current subtraction method (data not shown).
3.3 Delayed rectifier (IKdr) sustained potassium currents
Sustained, non-inactivating/slowly inactivating, outward currents reminiscent of the delayed rectifier IKdr were isolated using KGlu based-internal solution in the presence of TTX (1 μM) via a standard voltage-clamp activation protocol as reported previously (Silva et al. 1990). Currents recruited were slowly activating, largely non-inactivating during the depolarizing 1 s step, exhibiting a fast deactivation upon return to negative holding potentials and sensitivity to tetraethylammonium (TEA, 10 mM) suggesting the presence of a delayed rectifier current IKdr in vlPAG/DRN DA neurons (Fig. 3a). Maximal IKdr conductance was calculated to be 7.0 ± 0.6 nS at +8 mV (n = 6, from four mice). The V50 value for steady-state activation was −26.9 ± 1.7 mV with a slope of 13.4 ± 1.8 (n = 6, Fig. 3b). Activation time constant for IKdr current was voltage-dependent becoming faster at more positive potentials (98.1 ± 7.7 ms at −52 mV and 2.8 ± 0.2 ms at +8 mV, n = 6, P < 0.001, paired t-test) with V50 and slope of values of −38.4 ± 1.0 mV and −6.8 ± 0.9 respectively (Fig. 3c). The IKdr current did not exhibit any appreciable inactivation even on long 10 s pulses at potentials up to −20 mV. We also monitored the deactivation of the IKdr tail current upon return to a single potential of −72 mV following the series of test potentials used to recruit the IKdr current as described above (Fig. 2d). Deactivation of the IKdr tail currents at −72 mV was sensitive to the test voltage potential prior to return to −72 mV and became faster at more positive test holding voltages (32.3 ± 2.0 ms following return from −52 mV and 17.2 ± 1.7 ms following return from +8 mV, n = 6, P < 0.001, paired t-test) with V50 and slope of values of −38.9 ± 12 mV and −11.5 ± 6.7 respectively (Fig. 3e). Activation of delayed rectifier-type currents is usually associated with Kv2.1 and/or Kv2.2 families of voltage-gated potassium channels in sympathetic neurons (Malin and Nerbonne 2002) and SNc DA dissociated neurons (Kimm et al. 2015). A KV7 (KCNQ)-mediated current (also known as the M-type current, IM) has been has been described in VTA neurons (Koyama and Appel 2006b). The IM potassium current is a slowly activating, non-inactivating current with sensitivity to TEA (through Kv7.2 subunits, Hadley et al. 2000) and activation that partially overlaps with that of delayed rectifier currents (Brown and Adams 1980; see also review, Brown and Passmore 2009). To examine the possibility of the presence of an IM current in vlPAG/DRN DA neurons we used a modified deactivation tail protocol (Koyama and Appel 2006b) where neurons were held at −72 mV and given an 1 s prepulse to −32 mV to activate the IM current before stepped to −42 to −72 mV 1 s to record the resultant IM current deactivation tail in the presence of TTX (1 μM) (online resource 2A, B). We recorded IM current relaxations (online resource 3C) with similar properties to that reported previously for VTA neurons (Koyama and Appel 2006b). These were sensitive to the KCNQ blocker XE991 (30 μM, online resource 3A, B, D). Moreover, XE991 partially inhibited the depolarization-induced sustained outward currents at −32 mV (67 ± 7% of control, n = 4, online resource 3D) suggesting that depolarizing pulses recruit effectively a large component of sustained outward current that is carried forward by the KCNQ family of voltage-gated potassium channels. Finally, perfusion with XE991 (30 μM) induced a depolarizing current in voltage clamp at −70 mV (control holding current at −70 mV, −18.2 ± 2.1 pA, in XE991, 27.2 ± 1.5 pA, n = 4, P < 0.05, paired t-test, data not shown).
3.4 Low and high-voltage activated (LVA and HVA) calcium currents (ICaLVA and ICaHVA)
Calcium currents play an important role in neuronal autorhythmicity and pacemaking in DA midbrain neurons (Wolfart and Roeper 2002; Puopolo et al. 2007; Khaliq and Bean 2010). We have isolated and recorded calcium currents on vlPAG/DRN DA neurons using standard activation protocols in the presence of blockers of potassium and sodium conductances (Brevi et al. 2001; Pignatelli et al. 2005). Calcium currents exhibited a characteristic inward current-voltage relationship with the maximal amplitude (Imax) occurring around −15 to −10 mV (Fig. 4a) and were fully sensitive to cadmium (200 μM, n = 4, from three mice, data not shown). They exhibited a fast, voltage-dependent, activation time constant (τact, 1.27 ± 0.28 ms at −47 mV and 0.62 ± 0.06 ms at −17 mV, n = 4, P < 0.05, paired t-test, Fig. 4b) and inactivated in a voltage-dependent manner during the 250 ms long steps used (inactivation time constant τina, 114 ± 28 ms at −47 mV and 16.7 ± 1.7 ms at −17 mV, n = 4, P < 0.05, paired t-test, Fig. 4b). The corresponding mean V50 values for the voltage dependency of the activation and inactivation time constants were −23.9 ± 4.3 mV and −39.0 ± 2.1 mV with a slope of −6.9 ± 3.8 and −2.6 ± 2.1 respectively (n = 4). Mean steady-state activation V50 for the recorded calcium currents using a series of voltage steps was −26.1 ± 0.7 mV with a slope value of 5.0 ± 0.6 (n = 4, Fig. 4c). Using fast voltage-ramps (500 mV/s, from −107 mV to +53 mV) as an alternative way of describing background calcium currents we found that we could successfully discriminate in a subset of vlPAG/DRN DA neurons (n = 3 of 7 neurons tested) two peaks of different amplitude (fully sensitive to cadmium), a small one peaking at around −60 to −50 mV and a larger one peaking at around −20 to −10 mV (Fig. 4d, e). Analysis of the voltage ramps suggested that LVA calcium currents had a mean steady-state activation V50 of −61.2 ± 2.1 mV with a slope value of 3.9 ± 0.9 (n = 3) while HVA calcium currents exhibited a mean steady-state activation V50 of −22.4 ± 1.7 mV with a slope value of 7.1 ± 1.0 (n = 3). To test the effects of calcium current abolition on spontaneous firing we replaced calcium ions with magnesium and recorded in current-clamp mode using KGlu-filled electrodes in standard aCSF in the presence of synaptic blockers (n = 6 from three mice, Fig. 4f). We found that this replacement did not prevent expression of spontaneous firing and that it significantly accelerated pacemaking frequency (control firing frequency, 3.7 ± 0.6; firing frequency in zero calcium, 5.6 ± 0.8, n = 6, P < 0.01, paired t-test, Fig. 4g) without affecting firing regularity (mean CV-ISI and median in 2 mM calcium, 0.66 ± 0.29 and 0.42; mean CV-ISI and median in zero mM calcium, 0.44 ± 0.06 and 0.35, n = 6, P > 0.05, paired t-test, Fig. 4h) suggesting that calcium (and calcium-dependent) currents modulate basal firing frequency but are not responsible in driving spontaneous firing of vlPAG/DRN DA neurons.
3.5 Low and high-voltage activated (LVA and HVA) barium currents (IBaLVA and IBaHVA)
Calcium currents are known to undergo two types of inactivation (voltage-dependent and calcium-dependent) in a number of preparations (Giannattasio et al. 1991; Haack and Rosenberg 1994; Catterall 2000; Budde et al. 2002). It is unlikely that the inactivation observed here in calcium during the series of depolarizing voltage steps (starting at −67 mV) is due to a transient low voltage activated (LVA) calcium current as this voltage protocol should not have recruited such currents to any significant degree while the inactivation kinetics of LVA transient currents are reported to be different from the inactivation seen here for calcium currents (Kang and Kitai 1993a; Pignatelli et al. 2005, see also below the inactivation of barium LVA currents). The inactivation of calcium currents recorded here during long steps could be explained by intracellular calcium release inducing calcium current inactivation or could be attributed to the specific properties of a high voltage activated (HVA) calcium conductance (e.g. see Keja et al. 1992; Kang and Kitai 1993a, 1993b). To distinguish between these possibilities, we replaced calcium (2 mM) with barium (1 mM) in the extracellular solution to reduce calcium release-induced calcium current inactivation (Hille 2001). We used two protocols to record barium currents, commencing from a different potential that can recruit selectively HVA or a composite of LVA/HVA currents (see Brevi et al. 2001; Hille 2001). Barium replacement resulted in robust non-inactivating HVA currents during long steps (250 ms) used in our study (Fig. 5a) suggesting that calcium release-induced calcium current inactivation is the most likely explanation for the observed inactivation of calcium currents (compare Figs. 4a and 5a). During LVA/HVA composite current protocol recording we noticed the appearance of transient fast activating, fast inactivating barium current (Fig. 5a). These currents were subtracted from HVA currents to reveal the LVA component (Fig. 5b) and both components were individually subjected to kinetic analysis. Maximal conductance (Gmax) for the LVA and HVA calcium component was calculated at 0.65 ± 0.14 nS and 1.06 ± 0.18 nS respectively (n = 6, from three mice). Mean steady-state activation V50 for LVA and HVA barium currents were −58.9 ± 1.5 mV and −34.6 ± 0.9 mV with slope values of 6.3 ± 1.2 and 5.1 ± 0.8 respectively (n = 6, Fig. 5c). Activation time constants were voltage-dependent for both LVA and HVA barium currents, being faster at more positive potentials (τact at −57 mV and +3 mV, LVA, 1.11 ± 0.18 ms and 0.53 ± 0.09 ms; HVA, 2.77 ± 0.76 ms and 0.78 ± 0.12 ms respectively, n = 6, P < 0.05 for both comparisons, Fig. 5d). There was also significant difference between LVA and HVA activation at all holding potentials more negative than −7 mV but not at more positive potentials (n = 6, P < 0.05, paired t-test). Mean activation time constant V50 for LVA and HVA barium currents was −49.2 ± 3.4 mV and −39.7 ± 5.1 mV with slope values of −5.8 ± 3.0 and −13.4 ± 5.1 respectively (n = 6, Fig. 5d). LVA inactivation time constant exhibited voltage-dependency, being slower at more positive potentials (at −67 mV, 8.5 ± 0.8 ms; at +3 mV, 16.8 ± 1.4 ms, n = 6, P < 0.05, paired t-test, Fig. 5e), while when fitted with a Boltzmann function in the voltage range it exhibited V50 value of −34.5 ± 11.1 mV with slope of 0.37 ± 4.3 (n = 6). Fast voltage-ramps (200–500 mV/s, from −107 mV to +13 mV) recruited a barium current peaking at −20 to −30 mV but were less successful in isolating a distinct peak reflecting an LVA component as seen in a some neurons recorded in calcium (e.g. Figure 4d). Despite this we found evidence of activation of an inward conductance at potentials more negative than −60 mV (Fig. 5f) of different slope than the activation of the HVA component that is expected to begin at much more positive potentials (starting at around −35 mV). Steady-state activation V50 for the background voltage-ramp barium current was −38.9 ± 2.5 mV with slope value of 6.3 ± 1.5 (n = 4). Interestingly, leak current reversal during these voltage ramps appeared 30 mV more positive than ramps conducted in calcium (compare ramps in Fig. 4d and 5f) indicating that the leak conductance is probably at least partially carried forward to a degree by potassium ions through barium-sensitive ion channels. Nimodipine (10 μM), a L-type calcium channel blocker, blocked partially the HVA component (30–40% block) evoked by depolarizing steps (from −87 mV in 10 mV increments) without affecting the transient LVA component signifying that at least in part HVA barium currents are carried forward via the L-type calcium channel (online resource 4A, B).
3.6 Sodium (INa) currents
Transient and background ‘persistent’ sodium currents are operant on VTA and SNc neurons contributing differentially on their autorhythmicity (Puopolo et al. 2007; Khaliq and Bean 2010). We have recorded fast activating/inactivating (INaT) and persistent/non-inactivating inward sodium currents (INaP) through a standard activation depolarization step protocol and voltage-ramps in the presence of cadmium, cesium and TEA to block calcium and potassium currents respectively as reported previously (Pignatelli et al. 2005; Magistretti et al. 2006). Most voltage-clamped vlPAG/DRN DA neurons showed typical signs of problematic space-clamp control upon recordings of the fast transient sodium conductance as reported previously for neurons in brain slices (e.g. see Magistretti et al. 2006). Typical signs included distortion of sodium current waveform, clear long latencies to spike (> 4 ms from step onset to peak) and non-graded responses in activation implying activation of unclamped axonic sodium channels. To overcome this problem we have used a modified protocol exploiting a prepulse to selectively inactivate axonal currents and resolve somatic sodium currents as described previously (Milescu et al. 2010). Cells were held at −107 mV and a 4 ms depolarizing pulse to −47 mV was delivered to activate unclamped sodium channels (somatic and axonic, Milescu et al. 2010). Then, a 5 ms hyperpolarizing pulse was delivered to −77 mV to facilitate the fast deactivation of somatic (but not axonal, see Milescu et al. 2010) sodium currents before delivering 110 ms long, incremental 5 mV step depolarizations (up to +13 mV) to record somatic sodium currents. We routinely recorded good quality somatic sodium currents in one every 3–4 neurons at room temperature (20–22 °C) but at a much lower yield of one every 8–10 neurons at higher temperature in line with the problems that occur in electrophysiological recordings of very fast activating currents (Hille 2001; Milescu et al. 2010). At our target temperature of 35 °C, a few vlPAG/DRN DA neurons (n = 6, from three mice) exhibited a smooth graded response of somatic sodium current activation in the subthreshold range of −65 to −40 mV were accepted for kinetic analysis (Fig. 6a). Steady-state inactivation was studied by a series of prepulses (−77 to −42 mV for 5 ms, test pulse at −37 mV for 20 ms) delivered after a depolarizing step (−107 to −47 mV for 4 ms) to induce the inactivation of the axonal sodium current as detailed above for the construction of the steady-state activation curve (Fig. 6b). Following the fast transient sodium response, a “persistent”, background, sodium current appeared as an inward non-inactivating/slowly inactivating current upon 110 ms long step depolarizations (Fig. 6c). Both fast and persistent currents were fully sensitive to TTX while we did not detect any consistent residual inward current in the presence of TTX that would imply the activation of a TTX-resistant sodium conductance (n = 8, from four mice, data not shown). Slow voltage-ramps (16 mV/s, −107 to +53 mV) confirmed the presence of a background sodium conductance (Fig. 6d) that was 100–150 times smaller in magnitude than the transient sodium conductance. The average Gmax for the transient sodium component was 16.1 ± 1.2 nS with Gmax of persistent sodium currents reaching a much smaller value of 0.19 ± 0.04 nS (n = 6). Step depolarization and slow voltage-ramp activation protocols resulted in a GNaP that activated 5–10 mV more negative than GNaT (Fig. 6e). Steady-state activation V50 values were −45.2 ± 1.4 mV and −56.6 ± 1.3 mV with slope of 5.3 ± 1.3 and 3.3 ± 1.0 for GNaT and GNaP respectively (n = 6) whereas the corresponding values for ramp voltage determination of GNaP for V50 and slope was −60.7 ± 3.0 mV and 2.3 ± 0.7 (n = 3, Fig. 6e). INaT steady-state inactivation had a V50 of −62.8 ± 2.5 and a slope of −6.4 ± 1.7 (n = 4, Fig. 6e). INaT activation time constant (τact) was voltage-dependent becoming faster at more positive potentials (τact at −47 mV, 704. 5 ± 152.4 μs; at −2 mV, 147.2 ± 17.8 μs, n = 6, P < 0.05, paired t-test, Fig. 6f). The V50 and slope for the τact was −34.4 ± 4.1 mV and −5.6 ± 3.8 respectively (n = 6). The inactivation phase of the sodium current was consistently fitted with two (fast and slow, τinaF and τinaS) rather than one exponential function. The contribution of the τinaS exponential component in the inactivation phase of INaT would account only for <5% of the amplitude of the current for the voltage range studied (up to −2 mV, n = 6, data not shown). INaT inactivation time constants showed similar voltage-dependence (Fig. 6f) with both τinaF and τinaS becoming faster at more positive potentials (τinaF and τinaS at −47 mV, 888.8 ± 83 μs and 17.4 ± 2.0 ms; at −2 mV, 410.2 ± 80.5 μs and 4.2 ± 0.6 ms respectively, n = 6, P < 0.05 for both paired comparisons, paired t-test). The corresponding V50 values for τinaF and τinaS extracted with a first order Boltzmann in the voltage range tested, returned values of -46.4 ± 1.5 mV and −50.5 ± 1.4 mV and slopes of −11.3 ± 1.5 and −7.7 ± 1.4 respectively (n = 6). To investigate the impact of sodium channel blockade on spontaneous firing and pacemaker frequency we recorded in current-clamp in control conditions using standard KGlu filled electrodes and superfused the slice with 1 μM TTX (Fig. 6g, h) as reported previously (Khaliq and Bean 2010). We found that after perfusion of TTX the neurons stopped firing and had a stable, non-oscillating, resting membrane potential that was on average − 6.4 ± 0.8 mV more negative than the average action potential threshold (−43.1 ± 1.3 mV) (n = 8, from three mice, data not shown). These data suggest that TTX-sensitive sodium currents are important in membrane repolarization to AP threshold and neuron’s spontaneous firing.
3.7 Model DA neuron
3.7.1 Validation of in silico model DA neuron
Based on our experimental data, we constructed a single compartment, simplified, Hodgkin and Huxley- type DA neuron to compare model and in vitro neurophysiological behavior and explore the origin of autorhythmicity and pacemaking in silico. A summary of the mean values used for constructing the model DA neuron are given in Table 1. General equations used for the model DA neuron are given in the appendix. The model DA neuron exhibited autorhythmicity and fired APs at a pacemaker frequency of 4.6 Hz (Fig. 7a). AP characteristics (Fig. 7b) were measured and were compared with the corresponding mean values measured in the in vitro DA neuron in brain slices (Table 2, Fig. 7b). We found that the model DA neuron had similar AP characteristics and internal ratios to the native DA neurons (see also Dougalis et al. 2012) but notably had a faster action potential in width (at base) than in vitro vlPAG/DRN DA neurons. Model DA neuron exhibited an input resistance of 1.3 GΩ when subjected to small (−10 pA, 1000 ms) hyperpolarizing current injection in range with in vitro data (Dougalis et al. 2012). We injected a series of hyperpolarizing and depolarizing currents to the model DA neuron to validate its electrophysiological behavior (Fig. 7c, d) and to compare and contrast it with that of the in vitro DA neuron (Fig. 7e-h). Hyperpolarizing current injections were used to monitor the hyperpolarization-activated, cation current (IH current-mediated voltage-sag) and IA current-mediated delayed repolarization (quantified as the delay to firing a spike after the end of a hyperpolarizing current injection, Fig. 7c) which are the hallmarks of DA neuron electrophysiological behavior in vlPAG/DRN. Both responses were qualitatively and quantitatively similar to these obtained from in vitro brain slice preparation (Fig. 7g, h). Notably, the responses to the voltage-sag amplitude appeared fairly linear to those in vitro but the responses of the delayed depolarization produced an abruptly graded response at low current injections with no further increases detectable in delay to spiking thereafter. Upon injection of depolarizing pulses (Fig. 7d), the model DA neuron exhibited responses with similar gain (slope) in firing output to in vitro DA neurons only when given small magnitude current injection (10–40 pA, Fig. 7e-f). However, upon increasing the magnitude of the current injection (60–120 pA), the model DA neuron exhibited higher gain in output and fired at higher frequencies than that of the in vitro DA neurons while, it exhibited depolarization block (DB) at current magnitude within a similar range with in vitro data (Fig. 7e, f). Such behavior could be improved dramatically when needed by using a range of values reflecting the mean ± one standard deviation of the experimentally derived parameter during optimization without changing qualitatively the behavior and the origins of pacemaker (see later Figs. 8- 10). These data indicate that despite its apparent reductionist approach in the modelling of ion channel properties imposed herein, the model DA neuron captured and replicated well essential elements of vlPAG/DRN DA neuronal behavior as seen in vitro. Using this basal state of the model without further adjustments we then proceeded into further experiments attempting to understand the contribution of individual ion currents to firing frequency, autorhythmicity and threshold for depolarization block (Figs. 8- 10).
3.7.2 Contribution of ionic conductances in pacemaker firing frequency and expression of autorhythmicity
To evaluate the contribution of each ionic current to pacemaker firing frequency and neuronal autorhythmicity we used the model DA neuron to generate predictions by reducing the maximal conductance levels (Gmax from 100% to zero) of each one individual conductance in turn (Fig. 8). We found that complete elimination of the IA current caused a two-fold increase of model DA neuron basal pacemaker frequency (Fig. 8b). In contrast, eliminating the IH current lead to a very small change (decrease) in firing frequency (Fig. 8c). Eliminating ICaLVA and ICaHVA calcium conductances decreased the model’s pacemaking frequency to different levels (Fig. 8d, e). The former, but not the latter, appeared as a strong regulator of firing frequency (causing an approximate 25% reduction in basal firing frequency) but complete and concomitant elimination of both calcium conductances did not stop spontaneous firing suggesting that calcium currents are not indispensable for vlPAG/DRN neuron’s spontaneous firing (Fig. 8f). Complete elimination of IM current did not affect autorhythmicity either but instead it caused a two-fold increase in firing frequency (Fig. 8g). In contrast, small reductions of IKdr initially increased firing frequency (data not shown) but when the Gmax value was reduced below 25% of its basal level, a stable non-oscillating depolarized potential above AP threshold (−35 mV) was attained accompanied by complete elimination of spontaneous firing even upon depolarizing current injections (Fig. 8h). Under these circumstances, even a small increase in the magnitude of the sustained outward IM current (to 125% of the basal values, see online resource 3, also Wladyka and Kunze 2006; Shah et al. 2011) could rescue firing even when IKdr was set to zero (Fig. 8i) suggesting that although the Ikdr current modulates strongly autorhythmicity, its effect could be rescued by the small increase of another sustained potassium conductance in line with what would be expected from a Hodgkin and Huxley formalism, where the operation of sustained potassium conductances is a prerequisite for spontaneous firing. Elimination of INaP obliterated spontaneous firing but APs could still be observed under injection of depolarizing current (Fig. 8j). Eliminating the INaT current alone halted spontaneous firing (and depolarizing current injection- induced firing) but caused the appearance of a 6 mV oscillating background (at a frequency of 5.1 Hz) below AP threshold. Interestingly, concomitant elimination of both transient and persistent sodium currents stopped firing and produced a stable resting membrane potential nearly 10–20 mV more negative from the AP threshold (−55 to-64 mV, depending on the simulation conditions, Fig. 8k). The origin of the background oscillating potential seen in the absence of a INaT current was explored by inducing small reductions (to 75% of the value of Gmax) in either the INaP current (Fig. 8m) or the IM current (Fig. 8n). Both treatments completely obliterated the background oscillation observed in the absence of the INaT current suggesting an interaction of the IM and INaP persistent and opposing currents could give rise to a background oscillation under certain values/conditions in the subthreshold range when the INaT current is completely eliminated. These simulation data suggest that sodium, but not calcium, currents are primarily the mediators of autorhythmicity in the model DA neuron, while any individual potassium current alone (IA,IKdr,IM), although strongly modulated pacemaker firing frequency, did not endow DA neurons with autorhythmicity. In contrast, it is a prerequisite that all individual sustained potassium currents are blocked simultaneously or reduced to less than 10% of their basal Gmax value that causes spontaneous firing to cease due to the attainment of a depolarized steady state (e.g. Figure 8h).
3.7.3 Contribution of ionic conductances in repolarization during ISI
To understand in more detail the interplay of ionic currents in pacemaking and their contribution to the repolarization during the ISI we examined the trajectories of the each ionic current during this period in the model DA neuron (Fig. 9). We found that Ikdr potassium currents deactivated with an outward relaxation during ISI facilitating repolarization while the IA and IM currents activated during ISI thus opposing repolarization (Fig. 9b). Interestingly, the IM current did not fully inactivate exhibiting a persistent outward current even at the peak of the AHP. We detected a rather small contribution (compared to IKdr and IA type currents) from a inward current relaxation from the IH current giving rise to a net outward current during ISI repolarisation. Importantly, ICaHVA current did not contribute with any inward current during the ISI repolarization but ICaLVA current gave rise to a small inward persistent current even at the peak of the AHP with growing contribution during the early phase of the ISI repolarisation. INaP remained inwardly active at the peak of the AHP and activated therafter strongly and quickly compared to ICaLVA. It displayed similar magnitude to the ICaLVA current after 50–75 ms post AHP peak but INaP grew rapidly in inward contribution in the latter part of the ISI repolarisation, unlike the ICaLVA that maintained a steady (not growing) non-inactivating inward contribution during late ISI repolarization. Collectively, these results highlight the importance of the persistent sodium current activation in driving autorhythmicity in vlPAG/DRN DA neurons and the opposing and facilitating roles of other inward and outward currents in setting the trajectory of voltage during ISI.
3.7.4 Contribution of individual ionic conductances in depolarization block (DB)
DA neurons of the vlPAG/DRN, unlike serotonin neurons in the vicinity, exhibit depolarization block (DB), a gradual adaptation and ultimately cessation of firing following challenge with an increasing magnitude depolarizing current pulse (Dougalis et al. 2012). Attainment of a DB state in DA neurons has been postulated to be important in the mode of action of antipsychotics in schizophrenia (Grace et al. 1997). Our model DA neuron also exhibited DB upon depolarizing current injections at a similar range of depolarizing current injections as native vlPAG/DRN DA neurons (see Fig. 7d, also Fig. 10a). We thus used the model DA neuron to understand how individual ionic conductances affect the magnitude of the current required (threshold) to achieved DB by focusing first on sodium and calcium currents. Reducing the Gmax value (to 50%) of the INaT resulted in a reduction in the magnitude of the depolarized current required to produce DB (Fig. 10b) while increasing the Gmax (to 150%) lead to exactly the opposite effect. In contrast, decreasing Gmax value of the INaP (to 50%) resulted in no or a small increase in the DB threshold (Fig. 10c) while increasing Gmax (1.5 times the Gmax) produced a lower threshold for DB. Similar reductions or increases in either ICaHVA or ICaLVA conductances did not affect the threshold for DB to the extent that sodium conductance modulation revealed in the model DA neuron (Fig. 10d-e) Similarly, moderate changes (reduction/increase) in the Gmax of the IH current as imposed previously for the sodium and calcium currents did not produce any significant effects on the threshold of depolarization block (online resource 5A). Changes in the Gmax value for the IA potassium current did not have an apparent effect on the DB threshold either (online resource 5B) although further changes beyond 50% modulated the threshold for DB in a manner similar to the effect of INaT (data not shown). Changes in the Gmax values of the IM current caused an effect similar but at much lower magnitude to the IKdr current (online resource 5C and D). The effects of small changes in the Gmax value of the IKdr were more pronounced than the other potassium conductances where 50% increase or decrease in the Gmax value strongly increased and decreased the DB threshold respectively (online resource 5D). The data suggest that the maximal somatic conductance of transient and persistent sodium currents distinctly modulates, in an opposing manner, the threshold for DB. Similarly, potassium currents reduce the threshold for DB to different degrees but calcium currents do not, indicating the operating complexity between sodium and potassium currents in setting the DB threshold for vlPAG/DRN DA neurons. Imposing larger reductions/increases than 50% of the maximum conductance of each individual current (e.g. reductions set to less than 20%) lead to identical changes to those reported above, but also revealed some modulating effects of the IA and calcium currents (not seen before at 50 to 150% level changes imposed), suggesting that under more extreme challenges to the test conditions (longer steps, larger reductions/increases in the maximal conductance) other ionic currents may have a role in setting the DB threshold (data not shown).
4 Discussion
DA neurons of the vlPAG and DRN fire action potentials at a frequency of 1–10 Hz but exhibit a much higher coefficient of variation in their firing patterns than SNc DA neurons (Dougalis et al. 2012). Their firing rate and pattern were found to be most similar to those of the VTA DA neurons (Dougalis et al. 2012). However, details of their intrinsic mechanism of operation including, the characteristics of ionic currents and their contribution to spontaneous firing are not known although such mechanisms have been long described for other midbrain DA neuronal groups (see Grace and Onn 1989; Silva et al. 1990; Puopolo et al. 2007; Khaliq and Bean 2010). To address this gap in knowledge we used voltage-clamp electrophysiology and pharmacology to isolate and describe a number of ionic currents operant on adult vlPAG/DRN DA neurons. We then analysed the data using a Hodgkin and Huxley formalism (Hodgkin and Huxley 1952) to construct a conductance-based computer model of a vlPAG/DRN DA neuron. We used this model to perform simulations and examine the involvement of individual ionic currents in DA neuron’s excitability by exploring their contribution in spontaneous firing, pacemaker frequency and threshold for spike frequency adaptation.
DA neurons of the midbrain express a hyperpolarization-activated cation current (IH current) that has been long thought to be the hallmark of DA neuron electrophysiology. Recent evidence contest the absolute correlation of an IH current with the DA phenotype as some non-DAergic neurons in the VTA also express IH currents (see Margolis et al. 2006) while a subset of VTA DA neurons projecting to the prefrontal cortex (mesocortical projection pathway) do not express an IH current (Lammel et al. 2008). In IH-expressing midbrain DA neurons, blockade of IH conductance does not halt autorhythmicity, but instead leads to a reduction in pacemaker firing frequency only in a subtype of SNc, but not in VTA, DA neurons (Neuhoff et al. 2002; Puopolo et al. 2007; Khaliq and Bean 2010). DA vlPAG/DRN neurons expressed an IH current of similar magnitude and kinetics with that of VTA, but not of that of the SNc, DA neurons (online resource 1). Blockade of IH current in DA vlPAG/DRN neurons resulted, as expected, in ablation of the hyperpolarization-induced, slowly activating, inward current (under voltage-clamp) or the depolarizing voltage-sag (under current-clamp) but did not significantly affect basal firing frequency or pacemaker variability in vitro. The DA model and in vitro brain slice data were in good agreement regarding the magnitude and kinetics of the IH current-mediated voltage-sag. In our DA model, reduction or complete removal of the IH current did not halt autorhythmicity and did not have large effects on firing of the model DA neuron, although it resulted in a reduction in basal firing frequency (about 10%). This is largely because the V50 for activation of the IH current (−115 mV) is more negative than the subthreshold potential that the neuron usually attains in vitro (normally up to −70 mV) and thus the IH current does not get efficiently activated during AHP following an AP (estimated availability at −70 mV of less than 5%). The more positive V50 for IH current activation of the SNc DA neurons (25 mV more positive than vlPAG/DRN or VTA DA neurons, see online resource 1) could potentially explain the effects of IH current blockade on SNc DA neuron’s firing rate and the lack of effects in VTA DA neurons firing rate reported previously (Neuhoff et al. 2002; Puopolo et al. 2007¸ Khaliq and Bean 2010) or the lack of effects seen here for vlPAG/DRN DA neurons. Examination of the trajectory of activation of IH current in the model DA neuron during the ISI suggests that a small IH inward current declines steadily from the peak of AHP to AP threshold giving rise to a net outward current during ISI repolarization. The IH current did not modulate the threshold for DB (online resource 5) further arguing that this current plays no significant role in vlPAG/DRN DA neuron excitability. These data taken together suggest that, similar to VTA DA neurons (Khaliq and Bean 2010), autorhythmicity of adult vlPAG/DRN DA neurons is largely independent of the IH current which contributes little in setting their basal firing frequency or influencing neuronal excitability.
Repolarization of DA neurons during the ISI and tuning of pacemaker frequency in individual SNc and VTA neurons is dependent on expression of an A-type transient potassium current (IA current, Silva et al. 1990; Liss et al. 2001; Koyama and Appel 2006a). The diversity of IA current behavior is dependent on the different number of potassium transcripts that can contribute to the assembly of these channels. Kv4.1, Kv4.2, Kv4.3, Kv3.4 and Kv1.4 subunits have been reputed to give rise to transient IA-like currents but only the Kv4.3 transcripts were found expressed in SNc DA neurons (Liss et al. 2001). SNc DA neuron’s IA currents are mediated by the Kv4.3 (long) transcript (heteropoda toxin 3-sensitive) where it seems to form functional IA channels in combination with accessory protein KChip3 (but not KChip 1,2 or 4, see Liss et al. 2001). Using a two protocol subtraction method (as reported before, Koyama and Appel 2006a), we recorded outward transient currents sensitive to 4-AP blockade which possessed a voltage-dependent activation time constant consistent with previous reports (Liss et al. 2001; Koyama and Appel 2006a). However, in our study the activation V50 for the IA current was found to be 30 and 20 mV more negative to what has been reported previously for SNc and VTA DA neurons respectively (Liss et al. 2001; Koyama and Appel 2006a), while the inactivation V50 was similar to the study of VTA DA neurons (approximately −90 mV, Koyama and Appel 2006a) and about 30 mV more negative to what has been reported in SNc DA neurons recorded under whole-cell conditions (Liss et al. 2001). Additionally, inactivation of the IA currents in vlPAG/DRN DA neurons studied here was described better with the sum of two exponentials at potentials more positive than −30 mV, a fast (about 100 ms, voltage-dependent) and a slow (about 550 ms, voltage-independent), which differs kinetically from the reported monoexponential and voltage-independent fast decay (around 30–50 ms) of IA currents in both SNc and VTA neurons in vitro (Silva et al. 1990; Liss et al. 2001; Koyama and Appel 2006a). The differences in the activation /inactivation range and kinetics of the inactivation of IA currents described here with previous reports of IA currents in VTA and SNc DA neurons can be attributed to differences in the preparations (e.g. physiological versus room temperature, brain slices versus dissociated neurons, whole-cell recordings versus outside-out patches) or inherently differential calcium influx kinetics (that may affect the properties of IA currents recorded, see Koyama and Appel 2006a)and residual recruited currents. By exclusion of the above possibilities, the discrepancies can also represent a real difference in the gating properties of IA currents in vlPAG/DRN DA neurons given that SNc and VTA DA neurons exhibit projection-specific differential physiological characteristics and greater diversity in their properties than previously envisaged (e.g see results from Lammel et al. 2008, 2011). The methodological differences between our study and the available studies (Liss et al. 2001; Koyama and Appel 2006a) could explain some of the differences observed in IA current gating in vlPAG/DRN DA neurons. For example, IA channels may be distributed both in somatic and dendritic domains but the latter are severed in dissociated neurons while often a mixture of somatic/extrasomatic channels is sampled in outside-out patch recordings leading to potential difference in the kinetics recorded (as acknowledged by Liss and colleagues, a 15 mV difference in inactivation V50 value was seen between whole-cell and outside-out patch recordings in SNc DA neurons). Also, in both the studies of Liss and colleagues and Koyama and Appel, only a single exponential was fitted and reported for IA currents despite the fact that the currents could have had more complex inactivation properties (referred to as dominant fast time constant for SNc DA neurons in Liss et al. 2001; see also clear evidence of biexponential decay in IA current recordings from dissociated VTA DA neurons in Koyama and Appel 2006a, figure 1A2). In our hands, VTA and vlPAG/DRN DA neurons exhibited similar IA current behavior with slow (100–150 ms inactivation time constant), initially monoexponential decay (at more negative potentials than −40 mV) with biexponential inactivation apparent at more positive potentials than −30 mV on long steps (see tail currents in online resource 1). The available data derived from the interpretation of the three main studies of IA current kinetics (Silva et al. 1990; Liss et al. 2001 and Koyama and Appel 2006a) and the evidence from projection specific studies of DAergic populations (see Lammel et al. 2008, 2011) suggest that IA current properties in SNc and VTA DA neurons are not similar but a systematic study of the IA current properties of projection-specific DA groups is still lacking making further interpretation and comparison to our data difficult. Interestingly, in our hands, 4-AP sensitive currents also exhibited a bi-exponential inactivation (online resource 2) in a similar manner to those recorded with the two protocol subtraction method. In our experiments, 4-AP increased a background conductance leading to typical current ‘crossing’ upon current subtraction in good agreement to what has been reported before by others in DA neurons (see Liss et al. 2001; Khaliq and Bean 2008) indicating some of the potential inherent difficulties in using 4-AP as a tool to kinetically describe IA currents. Despite this, a third method of isolating the IA conductance (recordings in the presence of TEA as in Silva et al. 1990) also showed that the IA currents in vlPAG/DRN DA neurons exhibit a strong biexponential decay with the fast exponential decay being twice as long (approximately 70 ms, albeit voltage-independent) compared to the reports of Liss and colleagues or Koyama and Appel suggesting that the biexponential properties seen here should most likely reflect IA current physiological operation in adult vlPAG/DRN DA neurons in brain slices. Also, all three methods of IA current isolation used here resulted in commensurate V50 values for the activation of the current (around −55 to −60 mV) suggesting further that the kinetics of activation described here are likely to reflect IA current gating in situ in brain slices rather than an artefact of the isolation method. The contribution of other background residual currents that could potentially contaminate our IA recording (e.g. a calcium-activated potassium conductance, IH current) cannot be excluded, although such a proposal could not directly explain the biexponential decay of the 4-AP-sensitive currents seen here or the biexponential slow decay seen in TEA recordings. Using our voltage-clamp data, we modelled a reduced version of IA current with a single, voltage-dependent exponential decay according to the two protocol subtraction method. Our model DA neuron exhibited well-defined delayed repolarization upon hyperpolarizing current steps to > −80 mV under current-clamp that was carried forward by the IA conductance and was quantitatively similar to delayed repolarization to firing recorded in brain slices in vitro. The model DA neuron predicted that a reduction in IA currents will lead to an increase in pacemaker firing frequency an effect seen previously in SNc DA neurons using blockade with heteropoda toxin-3 (Liss et al. 2001). IA currents develop a strong outward current during ISI repolarization from the peak of the AHP to AP threshold. Although abolition of the IA current lead to a two-fold increase in firing frequency, it did not stop spontaneous firing, suggesting that IA current is not essential for autorhythmicity. Interestingly, blocking the IA current in the DA neuron model did not strongly reduce the threshold for DB (online resource 5) suggesting that IA currents are major determinants of neuronal excitability in DA vlPAG/DRN neurons but do not exhibit high propensity in modulating BD threshold at least when exposed to the sequences and range of depolarizing pulses studied herein. Indeed, longer pulses (> 1000 ms) or greater changes in Gmax rendered the DA model neuron more susceptible to the effects of the IA current (data not shown) suggesting that under certain, more robust, conditions DB threshold is also modulated by IA currents. In a similar manner to IA potassium currents, blockade of IKdr positively modulated firing frequency in the DA neuron model but also modulated strongly the threshold for DB (online resource 5). The deactivation of IKdr following the AHP had a dramatic effect in membrane repolarization during ISI repolarization to AP threshold. We also show here that outward potassium currents recorded in vlPAG/DRN DA neurons are a composite of different non-inactivating/slowly-inactivating currents including a non-inactivating potassium conductance activating at more negative potentials than typical IKdr currents and mediated through XE991-sensitive KCNQ (Kv7) channels suggesting that an M-current (IM) is also expressed in DA vlPAG/DRN neurons with similar properties to that expressed in VTA DA neurons (online resource 3, see also Koyama and Appel 2006b, see also Hansen et al. 2006; Drion et al. 2010). The complete abolition of IKdr current renders the neuron highly depolarized and stops autorhythmicity. This is largely because IKdr current is the only persistent outward current in this neuron that can help facilitate effective repolarization after an AP by virtue of its deactivation. Despite the three-fold lower maximal conductance of the IM current compared to the IKdr current used in our model, increasing the IM current contribution by just minute amounts (10–25%) rescues the spontaneous firing of the DA neuron in the complete absence of an IKdr current, leading to the establishment of low frequency rhythmic APs and plateaus in the DA model neuron. The model suggests that IM current does not inactivate completely following AHP, thus providing a steady background outward current even at the peak of the AHP. This explains the fact that increase of IM current rescues neuron’s spontaneous firing in the absence of IKdr while abolition of the IM current dramatically increased firing frequency (and induced a depolarising current in vitro) but did not halt spontaneous firing of the DA model neuron (as partially seen in Koyama and Appel 2006b also see opposite effects of IM current opener retigabine in Hansen et al. 2006). The IM current also had an effect on the threshold for DB in a manner similar, but far less stronger to the IKdr current (see online resource 5). Our model suggests that the IM current is efficiently activated during ISI repolarization and in tandem with the IA current provides a strong outward current delaying the repolarization to AP threshold. These results collectively suggest that potassium currents strongly modulate neuronal excitability of vlPAG/DRN neurons but are not necessary individually per se for the expression of autorhythmicity. It is rather that, the complete negation of sustained outward currents like IKdr and IM simultaneously, is the prerequisite to render the neuron inactive and unable to generate rhythmically APs in line with a Hodgkin and Huxley formalism (Hodgkin and Huxley 1952).
Calcium currents play an important role in the pacemaking process in a number of diverse neuronal preparations, from midbrain SNc DA neurons to hypothalamic GABAergic suprachiasmatic nucleus neurons (e.g. Jackson et al. 2004; Khaliq and Bean 2010). Unlike SNc DA neurons, VTA DA neurons express a sodium ‘persistent’ background current that dominates over the rather small calcium current in the subthreshold range during ISI (Puopolo et al. 2007; Khaliq and Bean 2010). In our study, similar to the results obtained by Khaliq and Bean (2010) in VTA DA neurons, blockade of voltage-gated calcium currents by low calcium/high magnesium solutions lead to an increase in the pacemaker frequency in vlPAG/DRN DA neurons. Although such a treatment could have also reduced calcium-dependent potassium conductances leading to an increase in firing rate (but see also studies of Wolfart and Roeper 2002; Deignan et al. 2012), it demonstrates that pacemaking can persist in the absence of calcium indicating that calcium is not critical in driving spontaneous firing of vlPAG/DRN DA neurons. Interestingly, removal of calcium from the extracellular solution lead to small, albeit statistically insignificant reduction in the pacemaker variability unlike what would be expected from blockade of calcium-dependent potassium currents (see Wolfart et al. 2001), implying that this change represents potentially the algebraic sum of negating all calcium-driven and calcium-dependent currents (with potentially opposing roles in pacemaker variability, see Poetschke et al. 2015) in vlPAG/DRN DA neurons. Our experiments indicate that both transient LVA and slowly-inactivating HVA (through a calcium release-mediated calcium inactivation) calcium currents are expressed in vlPAG/DRN DA neurons with properties similar to those described previously in other systems (Brevi et al. 2001; Jackson et al. 2004) but also in DA neurons (Kang and Kitai 1993a, 1993b). The slowly inactivating HVA component was sensitive to nimodipine, indicating that an L-type calcium current is partly responsible for the inward conductance recorded (online resource 4). The LVA component had characteristics reminiscent of a T-type current (see Kang and Kitai 1993a), was resistant to nimodipine (online resource 4) but sensitive to cadmium. Our model suggests that full blockade of the ICaLVA currents, did not halt DA model neuron autorhythmicity or affect its threshold for DB but reduced basal pacemaker firing frequency by nearly 30%. ICaLVA currents contributed with a small (compared to potassium currents) but constant inward current (that did not fully inactivate during or shortly after AP) during ISI repolarization to AP threshold. In contrast, to the ICaLVA currents, ICaHVA currents failed to contribute with any inward current during ISI repolarization to AP threshold, remaining essentially inactive during ISI and activating only during the AP. Blocking ICaHVA current did not halt autorhythmicity of DA model neuron (alone or in combination with blockade of the ICaLVA currents) and did not affect pacemaker firing frequency or contribute to any degree in setting the threshold for DB (even on longer steps as described for the IA current). This is perhaps expected by ICaHVA current that has on average nearly 30 mV more positive activation midpoint in comparison to the ICaLVA current, explaining why the latter can affect neuronal operation in the subthreshold range. Our data collectively suggest that calcium currents are not required for spontaneous firing on the model DA neuron but ICaLVA currents may have a role in modulating neuronal excitability in the opposite direction and less strongly than potassium conductances.
Sodium currents play an important role in the pacemaking activity of VTA DA neurons driving repolarization during ISI through a voltage-dependent, TTX-sensitive and a voltage-independent, TTX-resistant component (see Khaliq and Bean 2010). They are less important in the pacemaking of SNc DA neurons where calcium currents dominate and drive repolarization during the ISI (Puopolo et al. 2007). Blocking TTX-sensitive sodium channels in the brain slice lead to a stable, non-oscillating, resting membrane potential in vlPAG/DRN DA neurons, in a similar manner to what has been reported previously for VTA DA neurons (Khaliq and Bean 2010) and in contrast to the reported behavior of SNc DA neurons (see Nedergaard et al. 1993; Mercuri et al. 1994; Chan et al. 2007; Puopolo et al. 2007; Guzman et al. 2009). In the model DA neuron, blockade of both fast and persistent sodium conductances lead to the establishment of a hyperpolarized stable non-oscillating membrane potential in the same manner as in the in vitro brain slice. INaT and INaP currents start activating at different time points and rates following AHP during ISI repolarization and are adominant force driving DA neurons towards AP threshold. INaP current does not fully inactivate following an AP and rapidly activate during ISI repolarization relatively fast when compared to INaT current that is engaged significantly only in the last 50 ms before the occurrence of a AP under normal conditions. Blockade of INaP current alone halted spontaneous firing but depolarizing current injections restored the firing capacity of the DA model neuron suggesting that the expression of spontaneous firing is affected by the INaP current but not the capacity to generate APs in response to external inputs. Blockade of INaT currents alone stopped all spiking behavior on model DA neuron, inclusive of depolarization-induced spiking, and lead to a relatively hyperpolarized (compared to AP threshold) membrane potential with evidence of background oscillations (at 5 Hz) that were dependent on an interaction of the INaP current and the IM current. Indeed, small reductions (i.e. 10–25%) in either IM current or INaP current during the absence of a INaT current obliterated the oscillatory background behavior and resulted in a steady-state non-oscillating hyperpolarizing potential without affecting the overall working of the model. Such a behavior was not seen in the brain slice preparation suggesting that it could be related to the direct interaction of the activation kinetics of outward and inward persistent conductances in the model but its physiological significance (if any) is not currently known. Perhaps, studies utilizing dynamic voltage-clamp techniques to selectively negate INaP or INaT conductance in conjunction with pharmacology could help enormously in clarifying the distinct roles of transient and persistent sodium currents (or any interactions of the latter with the IM seen in the model DA neuron) in setting the properties of in vitro adult vlPAG/DRN DA neurons. Finally, using the DA model neuron we found that both transient and persistent sodium currents affected strongly DB threshold albeit exhibiting opposing effects. In good agreement with our study, Tucker et al. (2012) also found that reduction in somatic transient sodium currents reduces the DB threshold in a both in vitro and model SNc DA neuron (Tucker et al. 2012). During our voltage-clamp analysis, we could not reliably detect any discernable sodium current that persisted in the presence of TTX and thus we infer that TTX-resistant currents are not operant on vlPAG/DRN DA neurons, although it is also possible that we may have missed this small component. Our data collectively suggest that sodium currents endow DA vlPAG/DRN neurons with autorhythmicity by slowly activating during ISI repolarization and effectively bringing the neuron towards the AP threshold for firing.
In conclusion, the data presented here extend our previous physiological characterization (Dougalis et al. 2012) and argue that DA neurons of the vlPAG/DRN express autorhythmicity in the absence of synaptic transmission via the interplay of potassium and sodium currents without the absolute need of calcium currents. The properties of the ionic currents recorded here (IH current, IA current), the lack of small oscillating potentials in the presence of sodium channel blockers taken together with the mechanisms for autorhythmicity (reliance more on sodium rather than calcium currents) also support further the idea that vlPAG/DRN DA neurons are operationally similar to VTA, rather than SNc, DA neurons. In particular, the properties of a slowly inactivating IA current in conjunction with the small and slowly activating IH current described herein pinpoint that vlPAG/DRN DA neurons are most similar to prefrontal cortex or medial shell of nucleus accumbens projecting DA neurons (see Lammel et al. 2008, 2011). Given the importance of vlPAG/DRN DA neurons in arousal, reward and nociception, it would be interesting in the future to understand how the electrical properties and the synaptic activity arriving at these neurons may be modulated by sleep-wake cycles, drugs of abuse (e.g cocaine, heroin), or how it may change in models of nociception (e.g. following spinal cord injury or in neuropathic pain).
References
Beier, K. T., Steinberg, E. E., DeLoach, K. E., Xie, S., Miyamichi, K., Schwarz, L., Gao, X. J., Kremer, E. J., Malenka, R. C., & Luo, L. (2015). Circuit architecture of VTA dopamine neurons revealed by systematic input-output mapping. Cell, 162, 622–634.
Bishop, M. W., Chakraborty, S., Matthews, G. A., Dougalis, A., Wood, N. W., Festenstein, R., & Ungless, M. A. (2010). Hyperexcitable substantia nigra dopamine neurons in PINK1- and HtrA2/Omi-deficient mice. Journal of Neurophysiology, 104, 3009–3020.
Branch, S. Y., Sharma, R., & Beckstead, M. J. (2014) Aging decreases L-type calcium channel currents and pacemaker firing fidelity in substantia nigra dopamine neurons. The Journal of neuroscience: the official journal of the Society for Neuroscience, 34, 9310–9318
Brevi, S., de Curtis, M., & Magistretti, J. (2001). Pharmacological and biophysical characterization of voltage-gated calcium currents in the endopiriform nucleus of the guinea pig. Journal of Neurophysiology, 85, 2076–2087.
Brown, D. A., & Adams, P. R. (1980) Muscarinic suppression of a novel voltage-sensitive K+ current in a vertebrate neurone. Nature, 283, 673–676.
Brown, D. A., & Passmore, G. M. (2009) Neural KCNQ (Kv7) channels. British Journal of Pharmacology, 156, 1185–1195.
Budde, T., Meuth, S., & Pape, H. C. (2002). Calcium-dependent inactivation of neuronal calcium channels. Nature Reviews. Neuroscience, 3, 873–883.
Catterall, W. A. (2000). Structure and regulation of voltage-gated Ca2+ channels. Annual Review of Cell and Developmental Biology, 16, 521–555.
Chan, C. S., Guzman, J. N., Ilijic, E., Mercer, J. N., Rick, C., Tkatch, T., Meredith, G. E., & Surmeier, D. J. (2007). Rejuvenation' protects neurons in mouse models of Parkinson's disease. Nature, 447, 1081–1086.
Deignan, J., Lujan, R., Bond, C., Riegel, A., Watanabe, M., Williams, J. T., Maylie, J., & Adelman, J. P. (2012). SK2 and SK3 expression differentially affect firing frequency and precision in dopamine neurons. Neuroscience, 217, 67–76.
Ding, S., Wei, W., & Zhou, F. M. (2011). Molecular and functional differences in voltage-activated sodium currents between GABA projection neurons and dopamine neurons in the substantia nigra. Journal of Neurophysiology, 106, 3019–3034.
Dougalis, A. G., Matthews, G. A., Bishop, M. W., Brischoux, F., Kobayashi, K., & Ungless, M. A. (2012). Functional properties of dopamine neurons and co-expression of vasoactive intestinal polypeptide in the dorsal raphe nucleus and ventro-lateral periaqueductal grey. The European Journal of Neuroscience, 36, 3322–3332.
Drion, G., Bonjean, M., Waroux, O., Scuvée-Moreau, J., Liégeois, J. F., Sejnowski, T. J., Sepulchre, R., & Seutin, V. (2010). M-type channels selectively control bursting in rat dopaminergic neurons. The European Journal of Neuroscience, 31, 827–835.
Drion, G., Massotte, L., Sepulchre, R., & Seutin, V. (2011). How modeling can reconcile apparently discrepant experimental results: The case of pacemaking in dopaminergic neurons. PLoS Computational Biology, 7, e1002050.
Edwards, F. A., Konnerth, A., Sakmann, B., & Takahashi, T. (1989). A thin slice preparation for patch clamp recordings from neurones of the mammalian central nervous system. Pflügers Archiv - European Journal of Physiology, 414, 600–612.
Flores, J. A., El Banoua, F., Galan-Rodriguez, B., & Fernandez-Espejo, E. (2004). Opiate anti-nociception is attenuated following lesion of large dopamine neurons of the periaqueductal grey: Critical role for D1 (not D2) dopamine receptors. Pain, 110, 205–214.
Flores, J. A., Galan-Rodriguez, B., Ramiro-Fuentes, S., & Fernandez-Espejo, E. (2006). Role for dopamine neurons of the rostral linear nucleus and periaqueductal gray in the rewarding and sensitizing properties of heroin. Neuropsychopharmacology : Official Publication of the American College of Neuropsychopharmacology, 31, 1475–1488.
Giannattasio, B., Jones, S. W., & Scarpa, A. (1991). Calcium currents in the A7r5 smooth muscle-derived cell line. Calcium-Dependent and Voltage-Dependent Inactivation. The Journal of General Physiology, 98, 987–1003.
Grace, A. A., & Bunney, B. S. (1983a). Intracellular and extracellular electrophysiology of nigral dopaminergic neurons--1. Identification and Characterization. Neuroscience, 10, 301–315.
Grace, A. A., & Bunney, B. S. (1983b). Intracellular and extracellular electrophysiology of nigral dopaminergic neurons--2. Action Potential Generating Mechanisms and Morphological Correlates. Neuroscience, 10, 317–331.
Grace, A. A., & Bunney, B. S. (1984a). The control of firing pattern in nigral dopamine neurons: Burst firing. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 4, 2877–2890.
Grace, A. A., & Bunney, B. S. (1984b). The control of firing pattern in nigral dopamine neurons: Single spike firing. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 4, 2866–2876.
Grace, A. A., & Onn, S. P. (1989). Morphology and electrophysiological properties of immunocytochemically identified rat dopamine neurons recorded in vitro. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 9, 3463–3481.
Grace, A. A., Bunney, B. S., Moore, H., & Todd, C. L. (1997). Dopamine-cell depolarization block as a model for the therapeutic actions of antipsychotic drugs. Trends in Neurosciences, 20, 31–37.
Guzman, J. N., Sanchez-Padilla, J., Chan, C. S., & Surmeier, D. J. (2009). Robust pacemaking in substantia nigra dopaminergic neurons. The Journal of neuroscience : the Official Journal of the Society for Neuroscience, 29, 11011–11019.
Guzman, J. N., Sanchez-Padilla, J., Wokosin, D., Kondapalli, J., Ilijic, E., Schumacker, P. T., & Surmeier, D. J. (2010). Oxidant stress evoked by pacemaking in dopaminergic neurons is attenuated by DJ-1. Nature, 468, 696–700.
Haack, J. A., & Rosenberg, R. L. (1994). Calcium-dependent inactivation of L-type calcium channels in planar lipid bilayers. Biophysical Journal, 66, 1051–1060.
Hadley, J. K., Noda, M., Selyanko, A. A., Wood, I. C., Abogadie, F. C., & Brown, D. A. (2000). Differential tetraethylammonium sensitivity of KCNQ1-4 potassium channels. British Journal of Pharmacology, 129, 413–415.
Hansen, H. H., Ebbesen, C., Mathiesen, C., Weikop, P., Rønn, L. C., Waroux, O., Scuvée-Moreau, J., Seutin, V., & Mikkelsen, J. D. (2006). The KCNQ channel opener retigabine inhibits the activity of mesencephalic dopaminergic systems of the rat. The Journal of Pharmacology and Experimental Therapeutics, 318, 1006–1019.
Hille, B. (2001). Ion channels of excitable membranes, pp. 95–131. Sunderland: Sinauer Associates Inc..
Hines, M. L., & Carnevale, N. T. (1997). The NEURON simulation environment. Neural Computation, 9, 1179–1209.
Hodgkin, A. L., & Huxley, A. F. (1952). A quantitative description of membrane current and its application to conduction and excitation in nerve. The Journal of Physiology, 117, 500–544.
Hokfelt, T., Martensson, R., Bjorklund, A., Kleinau, S., & Goldstein, M. (1984). Distribution of tyrosine-hydroxylase-immunoreactive neurons in the rat brain. In A. Bjorklund & T. Hokfelt (Eds.), Handbook of chemical neuroanatomy (pp. 277–379). Amsterdam: Elsevier Science.
Itri, J. N., Michel, S., Vansteensel, M. J., Meijer, J. H., & Colwell, C. S. (2005) Fast delayed rectifier potassium current is required for circadian neural activity. Nature Neuroscience, 8, 650–656.
Jackson, A. C., Yao, G. L., & Bean, B. P. (2004). Mechanism of spontaneous firing in dorsomedial suprachiasmatic nucleus neurons. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 24, 7985–7998.
Kang, Y., & Kitai, S. T. (1993a). Calcium spike underlying rhythmic firing in dopaminergic neurons of the rat substantia nigra. Neuroscience Research, 18, 195–207.
Kang, Y., & Kitai, S. T. (1993b). A whole cell patch-clamp study on the pacemaker potential in dopaminergic neurons of rat substantia nigra compacta. Neuroscience Research, 18, 209–221.
Keja, J. A., Stoof, J. C., & Kits, K. S. (1992). Dopamine D2 receptor stimulation differentially affects voltage-activated calcium channels in rat pituitary melanotropic cells. The Journal of Physiology, 450, 409–435.
Khaliq, Z. M., & Bean, B. P. (2008). Dynamic, nonlinear feedback regulation of slow pacemaking by A-type potassium current in ventral tegmental area neurons. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 28, 10905–10917.
Khaliq, Z. M., & Bean, B. P. (2010). Pacemaking in dopaminergic ventral tegmental area neurons: Depolarizing drive from background and voltage-dependent sodium conductances. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 30, 7401–7413.
Kimm, T., & Bean, B. P. (2014). Inhibition of A-type potassium current by the peptide toxin SNX-482. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 34, 9182–9189.
Kimm, T., Khaliq, Z. M., & Bean, B. P. (2015). Differential regulation of action potential shape and burst-frequency firing by BK and Kv2 channels in substantia Nigra dopaminergic neurons. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 35, 16404–16417.
Koyama, S., & Appel, S. B. (2006a). A-type K+ current of dopamine and GABA neurons in the ventral tegmental area. Journal of Neurophysiology, 96, 544–554.
Koyama, S., & Appel, S. B. (2006b). Characterization of M-current in ventral tegmental area dopamine neurons. Journal of Neurophysiology, 96, 535–543.
Koyama, S., Kanemitsu, Y., & Weight, F. F. (2005). Spontaneous activity and properties of two types of principal neurons from the ventral tegmental area of rat. Journal of Neurophysiology, 93, 3282–3293.
Koyama, S., Brodie, M. S., & Appel, S. B. (2007). Ethanol inhibition of m-current and ethanol-induced direct excitation of ventral tegmental area dopamine neurons. Journal of Neurophysiology, 97, 1977–1985.
Lacey, M. G., Mercuri, N. B., & North, R. A. (1989). Two cell types in rat substantia nigra zona compacta distinguished by membrane properties and the actions of dopamine and opioids. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 9, 1233–1241.
Lammel, S., Hetzel, A., Hackel, O., Jones, I., Liss, B., & Roeper, J. (2008). Unique properties of mesoprefrontal neurons within a dual mesocorticolimbic dopamine system. Neuron, 57, 760–773.
Lammel, S., Ion, D. I., Roeper, J., & Malenka, R. C. (2011). Projection-specific modulation of dopamine neuron synapses by aversive and rewarding stimuli. Neuron, 70, 855–862.
Lerner, T. N., Shilyansky, C., Davidson, T. J., Evans, K. E., Beier, K. T., Zalocusky, K. A., Crow, A. K., Malenka, R. C., Luo, L., Tomer, R., & Deisseroth, K. (2015). Intact-Brain analyses reveal distinct information carried by SNc dopamine Subcircuits. Cell, 162, 635–647.
Li, C., McCall, N. M., Lopez, A. J., & Kash, T. L. (2013). Alcohol effects on synaptic transmission in periaqueductal gray dopamine neurons. Alcohol, 47, 279–287.
Li, C., Sugam, J. A., Lowery-Gionta, E. G., McElligott, Z. A., McCall, N. M., Lopez, A. J., McKlveen, J. M., Pleil, K. E., & Kash, T. L. (2016). Mu opioid receptor modulation of dopamine neurons in the periaqueductal gray/dorsal raphe: A role in regulation of pain. Neuropsychopharmacology : Official Publication of the American College of Neuropsychopharmacology, 41, 2122–2132.
Liss, B., Franz, O., Sewing, S., Bruns, R., Neuhoff, H., & Roeper, J. (2001). Tuning pacemaker frequency of individual dopaminergic neurons by Kv4.3L and KChip3.1 transcription. The EMBO Journal, 20, 5715–5724.
Lu, J., Jhou, T. C., & Saper, C. B. (2006). Identification of wake-active dopaminergic neurons in the ventral periaqueductal gray matter. The Journal of neuroscience : the Official Journal of the Society for Neuroscience, 26, 193–202.
Magistretti, J., Castelli, L., Forti, L., & D'Angelo, E. (2006). Kinetic and functional analysis of transient, persistent and resurgent sodium currents in rat cerebellar granule cells in situ: An electrophysiological and modelling study. The Journal of Physiology, 573, 83–106.
Malin, S. A., & Nerbonne, J. M. (2002). Delayed rectifier K+ currents, IK, are encoded by Kv2 alpha-subunits and regulate tonic firing in mammalian sympathetic neurons. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 22, 10094–10105.
Margolis, E. B., Lock, H., Hjelmstad, G. O., & Fields, H. L. (2006). The ventral tegmental area revisited: Is there an electrophysiological marker for dopaminergic neurons? The Journal of Physiology, 577, 907–924.
Matthews, G. A., Nieh, E. H., Vander Weele, C. M., Halbert, S. A., Pradhan, R. V., Yosafat, A. S., Glober, G. F., Izadmehr, E. M., Thomas, R. E., Lacy, G. D., Wildes, C. P., Ungless, M. A., & Tye, K. M. (2016). Dorsal raphe dopamine neurons represent the experience of social isolation. Cell, 164, 617–631.
Mercuri, N. B., Bonci, A., Calabresi, P., Stratta, F., Stefani, A., & Bernardi, G. (1994). Effects of dihydropyridine calcium antagonists on rat midbrain dopaminergic neurones. British Journal of Pharmacology, 113, 831–838.
Milescu, L. S., Bean, B. P., & Smith, J. C. (2010). Isolation of somatic Na+ currents by selective inactivation of axonal channels with a voltage prepulse. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 30, 7740–7748.
Mosharov, E. V., Larsen, K. E., Kanter, E., Phillips, K. A., Wilson, K., Schmitz, Y., Krantz, D. E., Kobayashi, K., Edwards, R. H., & Sulzer, D. (2009). Interplay between cytosolic dopamine, calcium, and alpha-synuclein causes selective death of substantia nigra neurons. Neuron, 62, 218–229.
Nedergaard, S., Flatman, J. A., & Engberg, I. (1993). Nifedipine- and omega-conotoxin-sensitive Ca2+ conductances in guinea-pig substantia nigra pars compacta neurones. The Journal of Physiology, 466, 727–747.
Neuhoff, H., Neu, A., Liss, B., & Roeper, J. (2002). I(h) channels contribute to the different functional properties of identified dopaminergic subpopulations in the midbrain. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 22, 1290–1302.
Philippart, F., Destreel, G., Merino-Sepúlveda, P., Henny, P., Engel, D., & Seutin, V. (2016). Differential somatic Ca2+ channel profile in midbrain dopaminergic neurons. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 36, 7234–7245.
Pignatelli, A., Kobayashi, K., Okano, H., & Belluzzi, O. (2005). Functional properties of dopaminergic neurones in the mouse olfactory bulb. The Journal of Physiology, 564, 501–514.
Poetschke, C., Dragicevic, E., Duda, J., Benkert, J., Dougalis, A., DeZio, R., Snutch, T.P., Striessnig, J. & Liss, B. (2015) Compensatory T-type Ca2+ channel activity alters D2-autoreceptor responses of substantia nigra dopamine neurons from Cav1.3 L-type Ca2+ channel KO mice. Scientific reports, 5, 13688.
Pollack, A. E. (2001). Anatomy, physiology, and pharmacology of the basal ganglia. Neurologic Clinics, 19, 523–534.
Poulin, J. F., Zou, J., Drouin-Ouellet, J., Kim, K. Y., Cicchetti, F., & Awatramani, R. B. (2014). Defining midbrain dopaminergic neuron diversity by single-cell gene expression profiling. Cell Reports, 9, 930–943.
Puopolo, M., Raviola, E., & Bean, B. P. (2007). Roles of subthreshold calcium current and sodium current in spontaneous firing of mouse midbrain dopamine neurons. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 27, 645–656.
Putzier, I., Kullmann, P. H., Horn, J. P., & Levitan, E. S. (2009). Cav1.3 channel voltage dependence, not Ca2+ selectivity, drives pacemaker activity and amplifies bursts in nigral dopamine neurons. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 29, 15414–15419.
Schultz, W. (1998). Predictive reward signal of dopamine neurons. Journal of Neurophysiology, 80, 1–27.
Seutin, V., Massotte, L., Renette, M. F., & Dresse, A. (2001). Evidence for a modulatory role of Ih on the firing of a subgroup of midbrain dopamine neurons. Neuroreport, 12, 255–258.
Shah, M. M., Migliore, M., & Brown, D. A. (2011). Differential effects of Kv7 (M-) channels on synaptic integration in distinct subcellular compartments of rat hippocampal pyramidal neurons. The Journal of Physiology, 589, 6029–6038.
Silva, N. L., Pechura, C. M., & Barker, J. L. (1990). Postnatal rat nigrostriatal dopaminergic neurons exhibit five types of potassium conductances. Journal of Neurophysiology, 64, 262–272.
Stuart, G. J., Dodt, H. U., & Sakmann, B. (1993). Patch-clamp recordings from the soma and dendrites of neurons in brain slices using infrared video microscopy. Pflügers Archiv - European Journal of Physiology, 423, 511–518.
Subramaniam, M., Althof, D., Gispert, S., Schwenk, J., Auburger, G., Kulik, A., Fakler, B.& Roeper, J. (2014) Mutant α-synuclein enhances firing frequencies in dopamine substantia nigra neurons by oxidative impairment of A-type potassium channels. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 34, 13586–13599.
Surmeier, D. J., & Schumacker, P. T. (2013). Calcium, bioenergetics, and neuronal vulnerability in Parkinson's disease. The Journal of Biological Chemistry, 288, 10736–10741.
Surmeier, D. J., Guzman, J. N., Sanchez-Padilla, J., & Schumacker, P. T. (2011). The role of calcium and mitochondrial oxidant stress in the loss of substantia nigra pars compacta dopaminergic neurons in Parkinson's disease. Neuroscience, 198, 221–231.
Tucker, K. R., Huertas, M. A., Horn, J. P., Canavier, C. C., & Levitan, E. S. (2012). Pacemaker rate and depolarization block in nigral dopamine neurons: A somatic sodium channel balancing act. The Journal of Neuroscience : The Official Journal of the Society for Neuroscience, 32, 14519–14531.
Wilson, C. J., & Callaway, J. C. (2000). Coupled oscillator model of the dopaminergic neuron of the substantia nigra. Journal of Neurophysiology, 83, 3084–3100.
Wladyka, C. L., & Kunze, D. L. (2006). KCNQ/M-currents contribute to the resting membrane potential in rat visceral sensory neurons. The Journal of Physiology, 575, 175–189.
Wolfart, J., & Roeper, J. (2002). Selective coupling of T-type calcium channels to SK potassium channels prevents intrinsic bursting in dopaminergic midbrain neurons. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 22, 3404–3413.
Wolfart, J., Neuhoff, H., Franz, O., & Roeper, J. (2001). Differential expression of the small-conductance, calcium-activated potassium channel SK3 is critical for pacemaker control in dopaminergic midbrain neurons. The Journal of Neuroscience : the Official Journal of the Society for Neuroscience, 21, 3443–3456.
Xiao, J., Cai, Y., Yen, J., Steffen, M., Baxter, D. A., Feigenspan, A., & Marshak, D. (2004). Voltage-clamp analysis and computational model of dopaminergic neurons from mouse retina. Visual Neuroscience, 21, 835–849.
Zhao, S., Maxwell, S., Jimenez-Beristain, A., Vives, J., Kuehner, E., Zhao, J., O'Brien, C., de Felipe, C., Semina, E., & Li, M. (2004). Generation of embryonic stem cells and transgenic mice expressing green fluorescence protein in midbrain dopaminergic neurons. The European Journal of Neuroscience, 19, 1133–1140.
Acknowledgements
This research was supported by grant U120085816 from the U.K. Medical Research Council (MRC) and a University Research Fellowship from The Royal Society to M.A.U. and, by the German DFG project LI1745/1 to B.L.
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All animal breeding and experimental procedures were conducted in accordance with the Animals (Scientific Procedures) Act of 1986 (United Kingdom) or as approved by the German Regierungspräsidium Tübingen. The manuscript does not contain clinical studies or patient data.
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The model and simulation experiments described herein have been conducted using free access software (NEURON, https://www.neuron.yale.edu/neuron/). Model parameters have been described extensively in the manuscript and model files are freely available from the authors upon request. Upon publication, the files will be made freely available to the modelDB database (https://senselab.med.yale.edu/modeldb/).
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Electronic supplementary material
Online resource 1
Comparative properties of IH current activation in SNc, VTA and vlPAG/DRN DA neurons. a. Representative electrophysiological traces recorded in voltage-clamp mode (holding voltage −62 mV, 10 mV incremental hyperpolarizing steps to −132 mV) depicting the activation of the IH current in SNc, VTA and vlPAG/DRN DA neurons. b. Comparison of the voltage-dependence of the activation of the IH current (% I/Imax) for SNc, VTA and vlPAG/DRN DA neurons. Note the more positive mean activation V50 for SNc neurons (−92 mV, n = 7) as opposed to VTA and vlPAG/DRN neurons (VTA,-121 mV; vlPAG/DRN,-121 mV, n = 7 and 6 respectively). c. Comparison of the voltage-dependence of the activation time constant of the IH current for SNc, VTA and vlPAG/DRN DA neurons. Note the similarity of the mean activation time constant (at −132 mV) of VTA and vlPAG/DRN neurons (VTA, 397 ms; vlPAG/DRN, 260 ms, n = 7 and 6 respectively) as opposed to the much faster kinetics of IH current activation in SNc neurons (114 ms, n = 7). (JPEG 39 kb)
Online resource 2
Comparative properties of IA currents isolated via three different methods in vlPAG/DRN DA neurons. a. A second, slow, inactivation time constant (τslow) could be fitted to the two protocol subtracted IA currents recorded at more positive potentials than −30 mV. Unlike the fast inactivation constant (τfast) that exhibited voltage sensitivity and faster kinetics at more positive holding potentials (Fig. 2h), τslow was largely voltage-independent and accounted for about half of the current’s amplitude (Amax) at a potential of +8 mV (mean τfast, 51 ms; mean τslow 562 ms at +8 mV, n = 6). b. Constructed steady-state activation curve (G/Gmax against holding voltage) after digital subtraction of the 4-AP (2 mM) sensitive current (as shown in Fig. 2b, c). The 4-AP sensitive conductance saturated well within the test voltage range and exhibited a mean V50 and slope of −61.4 ± 0.9 mV and 7.1 ± 0.8 mV respectively (n = 3). The residual conductance (after 4-AP subtraction) did not saturate well within our voltage range and exhibited a much more depolarized V50 estimated 30 to 50 mV more positive than the 4-AP sensitive conductance (data not shown). c. Voltage dependence of the inactivation time constant (τfast and τslow) for the 4-AP sensitive currents. Note that both inactivation time constants were voltage sensitive, becoming faster at more positive voltages. The second inactivation constant (τslow) was consistently evident at holding voltages more positive than −30 mV. Mean τfast and τslow was 63 ± 5 ms and 335 ± 34 ms at +8 mV (n = 3), values similar to the results obtained with the two protocol subtraction method (see Fig. 2i and online resource 2A). d. Contribution of inactivation time constants (τfast and τslow) to current amplitude expressed as a percentage of maximum current amplitude (Amax) at different holding voltages. Note that 4-AP sensitive currents exhibited a slow inactivation time constant (τslow) activating more positively than −30 mV and contributing to a mean of 27 ± 7% and 49 ± 5% of Amax at −22 mV and +8 mV respectively (n = 3) similar to the results obtained with the two protocol subtraction method (see above online resource 2A). e. Constructed steady-state activation curve (G/Gmax against holding voltage) for the IA currents isolated via single activation protocol (protocol 1 as shown in Fig. 2d) in the presence of 10 mM TEA (traces as shown in Fig. 2j). The IA currents saturated within the test voltage range and exhibited a mean V50 and slope of −55.6 ± 1.0 mV and 15.1 ± 1.1 mV respectively (n = 5). f. Voltage dependence of the inactivation time constant (τfast and τslow) for the IA current isolated via a single activation protocol (protocol 1 as shown in Fig. 2d) in the presence of 10 mM TEA (as shown in Fig. 2j). Note that using this method, IA currents exhibited consistently bi-exponential inactivation with time constants that were largely voltage insensitive (compare −72 mV and +8 mV, n = 5, P > 0.05, paired t-test). The second inactivation constant (τslow) was evident at holding voltages more positive than −60 mV. Mean τfast and τslow values were 56 ± 12 ms and 309 ± 47 ms respectively at +8 mV (n = 5) similar to the results obtained with the two protocol subtraction method and the 4-AP-sensitive currents isolated (see Fig. 2i and online resource 2A, C). g. Contribution of inactivation time constants (τfast and τslow) to current amplitude expressed as a percentage of maximum current amplitude (Amax) at different holding voltages. Note that IA currents isolated via a single activation protocol (protocol 1 as shown in Fig. 2d) in the presence of 10 mM TEA (as shown in Fig. 2j) exhibited a slow inactivation time constant (τslow) activating more positively than −60 mV and contributing to a mean of 35 ± 3% and 59 ± 5% of Amax at −22 mV and +8 mV respectively (n = 5) analogous to the results obtained with the two protocol subtraction method and the 4-AP-sensitive currents isolated (see Fig. 2d, i and online resource 2A, D). (JPEG 54 kb)
Online resource 3
Properties of an IM potassium current in vlPAG/DRN DA neurons. a. Typical averaged electrophysiological traces during a standard deactivation protocol for the M-type potassium current (IM) (Koyama and Appel 2006b). Neurons were recorded with a KGlu based-internal solution in the presence of TTX (1 μM). Neurons were held at −72 mV and were given a depolarizing prepulse to −32 mV for 1 s to fully activate the M current before stepping down from −42 to −72 mV for 1 s to record the resultant IM current deactivation tail. Currents were sensitive to the KCNQ blocker XE991 (30 μM) and to TEA (10 mM, n = 4 data not shown) suggesting the involvement of KV7.2 subunits in mediating the responses (scale bars, 50 pA, 250 ms). b. Overlay of electrophysiological traces showing details of IM current relaxation measurement (step hyperpolarization from −32 to −62 mV) before and after the application of XE991 (30 μM) (scale bars, 10 pA, 250 ms). c. Voltage-dependence of IM tail current amplitude and deactivation time constant. Deactivation time constant was significantly slower at more positive potentials (mean of 62 ± 6 ms at −62 mV and 235 ± 17 ms at −42 mV, n = 13, P < 0.0001, paired t-test) in close agreement with reports of IM currents in VTA DA neurons (Koyama and Appel 2006b). d. Percentage inhibition caused by XE991 (30 μM) on the amplitude of the IM deactivation tail current measured at different holding voltages following a prepulse to −32 mV (black squares). For comparison, the amplitude of the sustained outward current recruited after a depolarizing step from −72 to −32 mV is given (single point white square). Note that XE991 not only reduced the IM current relaxation but also the sustained outward current upon depolarizing pulses (mean 67%, n = 4). (JPEG 36 kb)
Online resource 4
The effects of nimodipine on IBaHVA and IBALVA currents in vlPAG/DRN DA neurons. a. Fast voltage-ramp (200 mV/s, −107 to +13 mV) depicting barium currents in the presence and absence of the L-type calcium channel blocker nimodipine (10 μM). Nimodipine-sensitive barium current was fitted with a single Boltzmann function (bottom to top) and had a steady state activation V50 of −22.1 mV and a slope of 4.2. b. Percentage block of barium LVA and HVA currents by nimodipine at different holding voltages studied by a series of voltage steps (from a holding potential of −87 mV, 10 mV increments from −77 to −7 mV). Nimodipine (10 μM) inhibited the persistent HVA barium current by 47 ± 8% (at −37 mV) but left the transient LVA barium current relatively unaffected (4 ± 3% reduction at −57 mV, n = 3). (JPEG 32 kb)
Online resource 5
Contribution of IH, IA, IM and Ikdr on DB threshold in vlPAG/DRN DA neurons. Representative 5 s simulation traces depicting the responses of model DA neurons to a sequence of depolarizing current injections (500 ms, as shown in Fig. 10a) leading to DB. a. Lack of effect of IH on the threshold of DB. b. Lack of major effects of IA on the threshold of DB. c. Modulation of DB threshold by IM. d. Strong modulation of DB threshold by Ikdr (JPEG 56 kb)
Appendix
Appendix
1.1 General model features
General equations for the construction and the workings of the NEURON simulator and the implementation of neuronal model within NEURON have been described extensively previously (see Hines and Carnevale 1997) and are briefly discussed and presented below together with specific equations used for the working of vlPAG/DRN DA neuron.
To follow the time evolution of neuronal membrane potential (Vm) for a neuron with a membrane capacitance Cm one must obtain the sum of each operant ionic current (denoted as (ion)) flowing through ionic channels on the neuron’s membrane. The general eq. (6) (current balance equation) below describes the relationship of membrane voltage and ionic current flowing through individual ionic channels for any neuron with membrane capacitance Cm.
The ionic current (I(ion)) passing through any ionic channel is both a voltage and time-dependent function. It can be calculated as the product of the ion’s maximal conductance (Gmax) times the driving force at any given potential (Vm-Erev, where Erev is the reversal potential for the conductance, Eq. (7))
The ionic currents in the model were described by standard, Hodgkin-Huxley–type equations in which generalized Boltzmann-type equations defined the voltage- and time-dependent activation and inactivation of conductances. Specifically, ionic conductances were evaluated by solving general eq. (8). Conductance (G(ion)) of any given ion at any given time t at any given Vm can be described as the product of the ion’s maximal conductance (Gmax) times the activation function (A(ion)) times the inactivation function (B(ion)) of the ion. A(ion) (Vm,t) and B(ion) (Vm,t) are functions describing the voltage and time dependence of activation and inactivation associated with G(ion), while p and n is the power to which A(ion) and B(ion)were raised and was taken as the standard value for a given ionic channel. P and n can be physically represented by the number of gating stages/steps for the ion channel activation and inactivation function respectively and were given a value of 3 and 1 for sodium channels and 4 and zero for potassium channel activation and inactivation functions respectively as described previously by Hodgkin and Huxley (1952).
A(ion)and B(ion)were given by the solution to the general differential eqs. (9) and (10) below:
where A00 (ion) and B00 (ion) are the voltage-dependent, steady-state values of the activation and inactivation functions, respectively; and τA(ion) and τB(ion) are the voltage-dependent time constants of the activation and inactivation functions, respectively. The values of A00 (ion) and B00 (ion) were determined from the general eqs. (11) and (12) below:
where Vm is the membrane voltage, whereas hA, hB) and sA, sB) determine the midpoints (V50) and slopes of the steady-state activation and inactivation functions, respectively. The voltage dependence of the activation and inactivation time constants (τA(ion) and τB(ion)) were represented by one of the two following functions respectively. Otherwise, τ was held constant.
where Vm is the membrane voltage; τA max, τA min and τB max, τB min are the maximal and minimal values for the activation and inactivation time constants, respectively; hτA, hτB and sτA, sτB determine the (V50) midpoints and slopes of the time constant functions, respectively. Equation (13) & (14) were used since the voltage dependence of the time constants was best fit by a sigmoid in the physiological range.
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Dougalis, A.G., Matthews, G.A.C., Liss, B. et al. Ionic currents influencing spontaneous firing and pacemaker frequency in dopamine neurons of the ventrolateral periaqueductal gray and dorsal raphe nucleus (vlPAG/DRN): A voltage-clamp and computational modelling study. J Comput Neurosci 42, 275–305 (2017). https://doi.org/10.1007/s10827-017-0641-0
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DOI: https://doi.org/10.1007/s10827-017-0641-0