IL-6 Mediates a Proinflammatory Response that Exacerbates Renal Injury

To determine the physiologic role of IL-6 in the development of renal injury, we compared the sensitivity of IL-6–deficient (IL-6^−/−) and wild-type (IL-6^+/+) mice with HgCl₂-induced AKI. IL-6^+/+ mice treated with HgCl₂ developed AKI manifested by an elevation of blood urea levels culminating in mortality of up to 70% of treated animals. In contrast, IL-6^−/− mice showed remarkable resistance to HgCl₂ toxicity (Figure 2A) and better survival (Figure 2B). A dose-response analysis of HgCl₂ toxicity showed that whereas IL-6^−/− mice were significantly more resistant to HgCl₂ toxicity than IL-6^+/+ mice at dosages ranging from 5 to 7 mg/kg, higher dosages of HgCl₂ (≥8 mg/kg) led to levels of renal failure that were indistinguishable between the two strains (blood urea nitrogen [BUN] at 24 h = 210 ± 160 (n = 5) versus 281 ± 188 mg/dl (n = 6) in IL-6^−/− and IL-6^+/+ mice, respectively; NS). These results indicated that IL-6 participates as a proinflammatory agent contributing toward the development of AKI.

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Figure 2.

IL-6^−/−, TNF-α^−/−, and immune-deficient mice are partially resistant to HgCl₂-induced AKI. (A) Renal function as indicated by BUN levels in IL-6^+/+ and IL-6^−/− mice administered HgCl₂ (6 mg/kg). Data are means ± SEM of surviving mice. *P 0.001 versus IL-6^+/+ mice (n = 14 to 15). (B) Kaplan-Meier survival plot of mice treated in A; log rank test, P 0.001 IL-6^−/− versus IL-6^+/+ mice. (C) Renal function in TNF-α^+/+ (TNF^+/+) and TNF-α^−/− (TNF^−/−) mice after HgCl₂ administration. Data are means ± SEM of surviving mice. *P 0.04 (n = 5 to 9). (D) Kaplan-Meier survival plot of mice treated in C; log rank test, P 0.04 TNF^+/+ versus TNF^−/− mice. (E) Renal function as indicated by BUN levels in BALB/c and BALB/c nu/nu mice. Data are means ± SEM. *P 0.008, **P 0.03 (n = 8). No mortality was observed.

To determine whether other inflammatory pathways mediated HgCl₂-induced AKI, we examined the renal toxicity of HgCl₂ in TNF-α–deficient (TNFα^−/−) mice. Similar to the IL-6^−/− mice, TNF-α^−/− mice displayed relative resistance to HgCl₂-induced AKI and a corresponding reduction in mortality (Figure 2, C and D). Interestingly, serum IL-6 levels resulting from HgCl₂ administration in TNF-α^−/− mice were not diminished in comparison with those of the wild-type mice (serum IL-6 = 2575 ± 830 pg/ml versus 2735 ± 3980 pg/ml in TNF-α^+/+ [n = 4] and TNF-α^−/− mice [n = 5], respectively; NS), indicating that HgCl₂-induced IL-6 expression is not TNF-α dependent.

Various leukocyte subsets, including lymphocytes and neutrophils, have been implicated as key cellular mediators in the development of renal ischemic/reperfusion injury.^14,15 To examine further the role of the inflammatory response, in particular that of T lymphocytes in HgCl₂-induced AKI, we compared the sensitivity of athymic BALB/c nu/nu mice versus wild-type BALB/c mice to HgCl₂ toxicity. The results of this analysis (Figure 2E) showed that BALB/c nu/nu mice, like IL-6^−/− mice and TNF-α^−/− mice, were significantly more resistant to moderate dosages of HgCl₂ than wild-type BALB/c mice. Similar results were also obtained in a single experiment comparing HgCl₂-induced AKI in SCID/bg versus wild-type BALB/c mice (BUN at 48 h = 41.8 ± 3.5 versus 437.5 ± 216.2 mg/dl, in SCID/bg [n = 6] versus wild-type [n = 8] mice, respectively; P < 0.003; mortality at 120 h 25 versus 66%, respectively).

Neutrophils participate in the development of AKI and are considered to be a source of exacerbation of injury in ischemic- and sepsis-induced AKI.^16–18 To determine whether neutrophil accumulation was related to IL-6 expression in HgCl₂-induced AKI, we compared neutrophil infiltration to kidneys in wild-type and IL-6^−/− mice after HgCl₂-induced injury. Twenty-four hours after HgCl₂ administration, robust accumulation of neutrophils within the peritubular capillaries and interstitium was observed in wild-type mice but was significantly less in IL-6^−/− mice (Figure 3A). This difference was also apparent in the few IL-6^−/− mice displaying more extensive morphologic injury. Substantial macrophage infiltration to the inner cortex was also observed after HgCl₂-induced injury but did not seem to be IL-6 dependent (Figure 3B). A corresponding infiltration of CD3⁺ T cells after HgCl₂-induced injury was not observed in either wild-type or IL-6^−/− mice (data not shown). Depletion of neutrophils before HgCl₂ administration dramatically prevented the development of AKI (creatinine at 24 h 1.10 ± 0.21 versus <0.5 mg/dl in control [n = 7] and antineutrophil serum–treated [n = 5] mice, respectively; P = 0.01; Figure 3C). Thus, IL-6 intrinsically links the cellular inflammatory response to the development of AKI.

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Figure 3.

Neutrophilic infiltration to the renal parenchyma after injury is IL-6 dependent and promotes renal injury. (A) Few peritubular neutrophils are present at baseline in IL-6^+/+ mice. Accumulation of neutrophils in peritubular capillaries at the inner cortex and outer medulla accompanied by neutrophilic extravasation into the renal interstitium is evident 24 h after HgCl₂ administration. Peritubular accumulation of neutrophils in IL-6^−/− mice after HgCl₂ administration was significantly diminished compared with IL-6^+/+ mice but not significantly different than in naïve IL-6^+/+ mice. Quantification of renal neutrophilic infiltration in IL-6^+/+ and IL-6^−/− mice 24 h after HgCl₂ administration is shown. Data are means ± SEM. *P 0.04 (n = 7) versus other groups. (B) Macrophage infiltration after AKI is not IL-6 dependent. Staining and quantification of renal macrophages in the inner cortex in IL-6^+/+ and IL-6^−/− mice 24 h after HgCl₂ administration. Data are mean ± SEM. *P < 0.05 (n = 7) versus other groups. (C) Effect of neutrophil depletion on HgCl₂-induced AKI. BUN levels in antineutrophil serum (□), control serum (), and untreated (baseline; □) are shown. Data are means ± SEM. *P 0.003 and 0.01 versus control serum + HgCl₂–treated and untreated mice, respectively. HPF, high-power field. Magnification, ×200.

In the Absence of IL-6R, IL-6 Trans-Signaling but not Classical Signaling Mediates a Protective Response to Kidney Injury

IL-6 is known to have pleiotropic effects, participating in both inflammatory processes and tissue protection.^19–23 We therefore questioned whether pretreatment of mice with IL-6 would affect HgCl₂-induced AKI. Mice treated with IL-6 before HgCl₂ administration displayed BUN levels and a mortality rate similar to those of saline-treated control mice (Figure 4, A and B). Prolonged exposure to IL-6 by hydrodynamics-based in vivo transfection of the IL-6 expression plasmid phAAT-IL-6 did not affect HgCl₂-induced AKI (data not shown).

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Figure 4.

The absence of IL-6R expression in murine kidney precludes protection by IL-6 treatment, but sIL-6R is elevated after AKI. (A) Pretreatment with exogenous human IL-6 fails to protect mice from HgCl₂-induced AKI. Renal function as indicated by BUN levels measured in mice treated with human IL-6 protein (20 μg, intravenously) or normal saline 4 h before administration of HgCl₂ (6 mg/kg). Data are means ± SEM of surviving mice. P = NS, IL-6 treated versus control (n = 10). (B) Kaplan-Meier plot of survival in mice treated in A. Log rank test, P = NS. (C) Western blot analysis of IL-6R from normal murine liver and kidney and from kidney after HgCl₂. The blots were stripped and reprobed for β-actin protein as a loading control. (D) IL-6R mRNA analysis by RT-PCR of RNA extracts from normal liver, normal kidney, and kidney tissue 6 h after HgCl₂ administration. RT-PCR analysis of β-actin mRNA is shown for comparison. OD analysis: 141.7 ± 2.9 (liver), 28.8 ± 3.4 (normal kidney), and 58.7 ± 2.8 (kidney after HgCl₂); P 0.008 for normal kidney versus kidney after HgCl₂. (E) Serum sIL-6R ELISA analysis from HgCl₂-treated (6 mg/kg) mice. Data are means ± SEM (n = 6 [48 h] to 12 mice [24 h]).*P < 0.00001, **P 0.002 versus 0 h. (F) Effect of neutrophil depletion on sIL-6R production after HgCl₂-induced AKI. sIL-6R ELISA analysis on serum samples from antineutrophil serum (□) and control serum–treated mice () after HgCl₂ administration and from untreated mice (□) is shown. Data are means ± SD. *P 0.01 versus other groups; **P 0.01 versus control serum and P = NS versus untreated mice.

Because responsiveness to IL-6 via the classical IL-6 signaling pathway depends on the expression of IL-6R on the target cell, we examined IL-6R expression in the renal parenchyma. Western blot and reverse transcriptase–PCR (RT-PCR) analyses of tissue extracts showed that the IL-6R protein and mRNA are expressed at very low levels in the normal mouse kidney in comparison with the liver, which was used as a positive control (Figure 4C). Six hours after treatment with HgCl₂, a slight but clear increase in IL-6R mRNA was evident; however, no change in the level of IL-6R protein was apparent at this or later times (Figure 4, C and D). Thus, the absence of IL-6R in the kidney precludes the activation of gp130 in the renal parenchyma via the classical IL-6 signaling pathway.

To account for the remarkable increase in STAT3 activation after renal injury (Figure 1, B and D), we postulated that gp130 signaling through a mechanism of sIL-6R–mediated trans-signaling may occur. Analysis of serum sIL-6R levels revealed a three-fold increase in sIL-6R during the 48 h after HgCl₂ administration (Figure 4E), which, together with the concurrent rise in IL-6 expression (Figure 1A), strongly points to the presence of IL-6 trans-signaling after kidney injury. Receptor shedding by activated neutrophils has recently been attributed as being a significant source of sIL-6R production.²⁴ Neutrophil depletion before HgCl₂ administration significantly diminished the sIL-6R levels (Figure 4F), suggesting that the rise in sIL-6R levels during HgCl₂-induced injury is substantially due to IL-6R shedding by neutrophils.

To determine the effect of IL-6 trans-signaling on the kidney in the absence of injury, we administered to mice an injection of the IL-6/sIL-6R fusion protein Hyper-IL-6 (HIL-6).²⁵ Analysis of renal STAT3 activation as a marker of IL-6 signaling clearly demonstrated that treatment with HIL-6, as opposed to IL-6, strongly stimulates gp130 signaling in the kidney (Figure 5A). pSTAT3 immunostaining after HIL-6 treatment revealed substantial nuclear staining in epithelial cells of the distal and proximal renal tubules (Figure 5B).

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Figure 5.

HIL-6 treatment protects mice from HgCl₂-induced AKI. (A) Western blot analysis of p-STAT3 (Tyr 705) and STAT3 in the kidney after treatment with PBS, IL-6 (20 μg), or HIL-6 (4 μg) demonstrates the effect of HIL-6 on gp130 stimulation in the kidney. (B) pSTAT3 (Tyr705) immunostaining of kidney sections 1 h after HIL-6 treatment reveals strong STAT3 activation (expressed as nuclear staining), particularly in the distal tubules, medulla and glomeruli (strong staining), and proximal tubules (mild staining) (pSTAT3-positive tubular epithelial cells 307.7 ± 36.3 versus 0.0 ± 0.0 per HPF for HIL-6–and saline-treated mice, respectively; P 0.007). (C) Renal function in mice treated with HIL-6 or normal saline 4 h before administration of HgCl₂. Data are means ± SEM. *P 0.002; **P 0.005 (n = 10). (D) Kaplan-Meier survival plot of mice treated as in B; log rank test, P 0.007, HIL-6 (n = 19) versus saline (n = 21). (E) Hematoxylin and eosin staining of paraffin-embedded renal tissue shows histologic changes 24 h after HgCl₂ administration in mice pretreated with normal saline or HIL-6 (8 μg, intravenously) 4 h before HgCl₂ administration. Saline-pretreated mice show extensive necrosis of tubular epithelial cells (black arrows), dilation of the tubular lumina filled with proteinaceous material (green arrow), and accumulation of neutrophils in the peritubular capillaries (arrowhead). HIL-6–pretreated mice display subtle tubular injury with occasional apoptotic tubular epithelial cells (arrowhead). Magnifications: ×400 in B and ×200 in E, inset; ×400 in E.

We next assessed the effect of HIL-6 on the development of AKI. Mice treated with HIL-6 protein before HgCl₂ administration were dramatically resistant to AKI (serum creatinine at 48 h 1.55 ± 0.684 mg/dl [n = 13] versus <0.5 mg/dl in saline- and HIL-6–treated mice, respectively; P = 0.001; Figure 5C). Moreover, whereas HgCl₂-treated mice displayed significant mortality, all mice treated with HIL-6 survived (Figure 5D). Morphologic analysis of renal tissue 24 h after HgCl₂-induced AKI (Figure 5E) revealed extensive necrosis of proximal tubules and widespread areas with signs of tubular injury (Table 1). In contrast, the HIL-6–treated mice exhibited significantly less evidence of tubular injury, presenting with mild focal tubular dilation and occasional apoptotic epithelial cells.

Animals

Male BALB/c and C57BL/6 mice (19 to 21 g) were purchased from Harlan Laboratories (Jerusalem, Israel). IL-6^−/− mice and TNF^−/− mice, both on a C57BL/6 background, were bred in-house from breeding pairs originally purchased from the Jackson Laboratory (Bar Harbor, ME).^45,46 Weight-matched C57BL/6 control mice were used in all experiments involving IL-6^−/− or TNF-α^−/− mice. BALB/c nu/nu mice and SCID/bg were purchased from Harlan UK (Blackthorn, Bicester, Oxon, England). Procedures and maintenance (see Supplemental Concise Methods) were performed in accordance with the Institutional Animal Care and Use Committee–approved animal treatment protocol (license no. OPRR-A01-5011).

Mercury-induced AKI was induced by intraperitoneal injection of a freshly prepared solution of HgCl₂ (6 mg/kg) dissolved in PBS.⁴¹ Glycerol-induced AKI was induced in anesthetized (Isoflurane) BALB/c mice by injection of 50% glycerol, at a total dosage of 8 ml/kg body wt, one-half dose injected into the anterior thigh muscle of each hind leg. HO-1 was inhibited by administration of SnMP,¹³ as described in the Supplemental Concise Methods.

Neutrophil Depletion

Circulating neutrophils were depleted by intraperitoneal injection of 0.2 ml of rabbit antineutrophil serum (Accurate Chemical and Scientific Corp, Westbury, NY.) 24 h before HgCl₂ administration.⁴⁷ This procedure removed 83 ± 17% of polymorphonuclear cells from the peripheral circulation. Previous studies reported that treatment with this antibody does not have a significant effect on other leukocyte subpopulations in the peripheral circulation.^47,48

In Vivo DNA Transfection

Animals were treated by hydrodynamics-based in vivo plasmid DNA transfection^49,50 with phAAT-IL-6 (10 μg), phAAT-HIL-6 (2.5 μg), or a control plasmid, pGEM-7 (20 μg). Details of plasmid DNA construction and preparation are in the Supplemental Concise Methods.

Determination of BUN and Creatinine

Blood samples were obtained by tail-vein bleeding. BUN levels and creatinine were determined in heparinized serum using the Reflotron system and Urea or Creatinine test strips (Roche Diagnostics, Basel, Switzerland).

Histologic and Immunohistochemical Analysis

Kidneys were removed 24 to 48 h after HgCl₂ administration and fixed in 4% buffered formaldehyde, followed by 80% ethanol, and embedded in paraffin blocks. Tissue sections were stained with hematoxylin and eosin. Neutrophils were stained with rat anti-mouse neutrophil antibody (Serotec, Oxford, England) diluted 1:3000 followed by biotinylated rabbit anti-rat (Dako, Glostrup, Denmark), and developed with horseradish peroxidase (HRP)-streptavidin (Invitrogen, Carlsbad, CA) using 3-amino-9-ethyl-carbazol (AEC) (Dako). Phospho-STAT3 was stained using monoclonal rabbit anti-mouse pSTAT3 (Tyr 705; Cell Signaling, Danvers, MA) diluted 1:500, followed by biotinylated goat anti-rabbit (Jackson Laboratory) diluted 1:5000, amplified using Tyramide Signal Amplification kit (PerkinElmer, Boston, MA) and developed with AEC. Macrophages were stained using rat anti-mouse F4/80 antigen (Serotec) diluted 1:200, followed by anti-rat HRP Histofine (Nichirei, Tokyo, Japan) and developed with AEC. CD3⁺ cells were stained using rat anti-human CD3 antigen (Serotec) diluted 1:200, followed by biotinylated rabbit anti-rat diluted 1:50 and developed with HRP-streptavidin using AEC. The number of positively stained cells per high-power field (Magnification, ×400) by immunohistochemistry was counted in 20 fields for each sample from coded specimens. Morphologic analysis of tubular injury was performed as described in the Supplemental Concise Methods.

Western Blot Analysis

Protein extracts were prepared from tissue samples (approximately 100 mg) by homogenization in 1 ml of whole-cell lysis buffer (1% NP-40, 10 mM Tris [pH 7.8], 150 mM NaCl, 40 mM EDTA, 10 mM Na-pyrophosphate, 10 mM NaF, 1 mM PMSF, 4 mM orthovanadate, 1 μg/ml pepstatin A, and 2 μg/ml leupeptin). Protein extracts for analysis of IL-6R were prepared by homogenization in m-PER buffer (Pierce, Rockford, IL). Protein extracts (50 μg) were separated by PAGE and subjected to Western blot analysis. For analysis of murine IL-6R, Western blots were probed with goat anti-mouse IL-6R antibody (R&D Systems, Minneapolis, MN) followed by rabbit anti-goat antibody (Zymed) and anti-rabbit HRP polymer (Dako) and developed using the ECL-Plus Western blotting Detection System (GE Healthcare, Upsala, Sweden). For analysis of pSTAT3 and STAT3, Western blots were probed with mouse monoclonal anti-phosphorylated STAT3 (sc-8059) and mouse monoclonal anti-STAT3 (sc-8019; Santa Cruz Biotechnology, Santa Cruz, CA), respectively. As a loading control, the blots were stripped with 0.1 M glycine (pH 2.8) and reprobed with a monoclonal anti–β-actin antibody, clone AC-74 (Sigma), and developed with HRP Envision (Dako).

IL-6 and sIL-6R ELISA

IL-6 and sIL-6R levels were determined using a mouse IL-6 and a mouse sIL-6R DuoSet ELISA kit (R&D Systems) according to the manufacturer's instructions on serum samples that were collected and frozen at −20°C until analysis.

RNA Extraction, RT-PCR, and Real-Time PCR Analysis

RNA samples were prepared from approximately 100 mg of snap-frozen tissue by homogenization in Trizol Reagent (Invitrogen, Carlsbad, CA) according to the manufacturer's instructions using a Polytron high-speed homogenizer, followed by treatment with DNA-free DNase (Ambion, Austin, TX). The primer sequences and details for RT-PCR and real-time PCR analysis are provided in the Supplemental Concise Methods.

Lipid Peroxidation Analysis

MDA, an end product of lipid peroxidation, was analyzed in serum and tissue samples by measurement of thiobarbituric acid reactive substances as described previously.^51,52 A detailed description is provided in the Supplemental Concise Methods.

These studies were supported by a grant from the Israel Science Foundation (Jerusalem, Israel; ISF 853/04) to J.H.A. and E.G. and by a grant from the Deutsche Forschungsgemeinschaft (Bonn, Germany; SFB415) to S.R.J. E.G. is supported by the Israeli Ministry of Science through a grant to the National Gene Therapy Knowledge Center and through EC grants LSHB-CT-2004-512034 and LSHB-CT-2005-018961. E.G. and J.H.A. are also supported by grants from the Blum, the Harold Grinspoon, the Horowitz, and the Wolfson Foundations.

Parts of this study were presented at the American Society of Nephrology Renal Week Conference; November 14 through 19, 2006; San Diego, CA.

We thank Amnon Peled for invaluable advice, Deborah Olam and Carol Levy for expert assistance in the care and breeding of IL-6–deficient mice, Ido Weiss and Hadas Shoham for TNF-α–deficient mice, Ariel Orfaig for assistance with computer graphics, and Tally Bdolah-Abraham for assistance with statistical analyses.