Intrathecal injection of Lenti-GFP, Lenti-IL27HA, and Lenti-IL35HA in EAE mice drives the release of GFP, IL-27, and IL-35 in the CSF

We injected Lenti-IL-27HA, Lenti-IL-35HA, and Lenti-GFP into the cisterna magna of EAE mice, as previously described²⁰. We obtained efficient infection of leptomeningeal (Fig. 2A, left panel) and ependymal (Fig. 2A, right panels) cells, and we confirmed the release, in comparable amounts, of the expected cytokines in the CSF by WB using the anti-HA antibody (Fig. 2B).

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Figure 2

IL-27, but not IL-35 gene therapy inhibits clinical EAE development. Intracisternally injected lentiviruses infected leptomeningeal (A, right panel) and ependymal (A, inset) cells releasing transgenes product into the CSF (A), and as shown by WB (dotted vertical line) are stitching of adjacent pictures (B). Mean clinical score of EAE mice injected with Lenti-IL-27HA and Lenti-IL-35HA (open dots) or Lenti-GFP (closed dots) both preventively (C,D), on the day after immunization, and therapeutically, on the day of disease onset (E,F). *p<0.05; **p<0.001 (EAE is evaluated as cumulative score using Mann Whitney; n=15/group). We show here one representative out of three independent experiments (see Supplementary Figure ⁵ for the other two EAE experiments). Mice were sacrificed between 28–34 days post immunization. Blot in panel (B) has been cropped, and full blot is presented in Supplementary Fig. ⁷.

IL-27, but not IL-35, gene therapy protects from neuroinflammation

We then induced neuroinflammation in C57BL/6 female mice by immunization with MOG_35-55. We treated EAE mice either the day after immunization (Fig. 2C,D; Supplementary Fig. ^5A–D) or the day of clinical disease onset, corresponding to 12–16 days after immunization for most mice (Fig. 2E,F; Supplementary Fig. ^5E–H). IL-27 (Fig. 2C,E; Supplementary Figure ⁵), but not IL-35 (Fig. 2D,F; Supplementary Figure ⁵) significantly decreased clinical disease severity, both preventively (Fig. 2C; Supplementary Figure ^5A–C) and on established disease (Fig. 2E; Supplementary Figure ^5E–G), as compared to Lenti-GFP treated EAE mice. We confirmed, by neuropathological analysis (Fig. 3A–D), a significant protection from demyelination and axonal loss only in Lenti-IL-27HA-treated EAE mice (Fig. 3E,F), while in Lenti-IL-35HA-treated mice only the decrease of inflammatory infiltrates reached statistical significance (Fig. 3G). Lenti-IL-27HA displayed also a significant decrease of CD3⁺ T cells (Fig. 3H). We confirmed by FACS the significant decrease of blood-derived CD45⁺CD11b⁻ (lymphoid cells), CD45^hiCD11b⁺ cells (myeloid cells), and CD45^lowCD11b⁺ (microglia) in the CNS (Fig. 4D–F) in Lenti-IL-27HA-treated EAE mice.

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Figure 3

Intrathecal IL-27, and IL-35 gene therapy protects EAE mice from tissue damage. Neuropathological analysis of demyelination (A), axonal loss (B), infiltrates (C), and CD3⁺ T cells (D). The protective effect of IL-27HA gene therapy is associated to a significant decrease of demyelination (E), axonal damage (F), inflammatory infiltrates (G), and number of infiltrating CD3⁺ T cells (H) (mean±sd). IL-35HA gene therapy promoted a significant decrease of inflammatory infiltrates (G). *p<0.05; (1 way anova; E–H n=5/group). We show here one representative out of three independent experiments.

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Figure 4

IL-27HA and IL35HA modulate the number of microglia and CNS infiltrating lymphocytes and macrophages. FACS analysis of CNS-infiltrating cells from Lenti-GFP (A), IL-27HA (B) and IL-35HA (C) treated EAE mice, for total CD45⁺CD11b⁻ lymphoid cells, CD45^hiCD11b⁺ infiltrating macrophages, and CD45^lowCD11b⁺ resident microglia. Lenti-IL-27HA exhibited ability to reduce the number of CNS-infiltrating lymphocytes (D) and infiltrating macrophages (E). *p<0.05; (1 way anova; (D–F) n=6/group).

IL-27 gene therapy reduces the absolute number of infiltrating GM-CSF⁺ and IL-17⁺ CD4⁺ T cells

We collected the brains and spinal cords of EAE mice treated with Lenti-IL-27HA and Lenti-IL-35HA and purified infiltrating cells to perform flow cytometric analysis as shown in Supplementary Fig. ⁴. The decrease of CD45⁺CD4⁺ cells in IL-27-treated EAE mice did not reach statistical significance (Fig. 5A,B), as opposed to the significant decrease in CD4⁺ T cells expressing GM-CSF (Fig. 5E,F), IL-17 (Fig. 5G,H) or both (Fig. 5I,L) in Lenti-IL-27HA-treated but not in Lenti-IL-35HA-treated EAE mice. The latter displayed decreased levels not reaching, however, statistical significance with this sample size (Fig. 5D,F,H,L). Also the decrease of CD4⁺IFNγ⁺ T cells was not significant neither in IL-27, nor in IL-35-treated EAE mice (Fig. 5C,D).

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Figure 5

IL-27 gene therapy decreases CNS infiltrating CD4⁺ T cells expressing gm-csf and IL-17. FACS analysis of CNS-infiltrating CD45⁺CD4⁺ T cells isolated from gene therapy-treated EAE mice (A,F). Intracellular staining for IFNγ (B), GM-CSF (C), IL-17 (D), or GM-CSF/IL-17 (E). IL-27, but not IL-35, significantly decreased GM-CSF and IL-17 expression in CD4⁺ T cells (H,I). Gating strategy is shown in Supplementary Figure. ⁶. *p<0.05 (1 way Anova, n=6/group).

IL-27HA and IL-35HA purification

HEK293T cells were grown in IMDM supplemented with 10% of fetal bovine serum (FBS), 2mM ultra-glutamin and 100Uml penicillin/streptomycin (Lonza, Braine-lAlleud, Belgium). Cells were seeded at 8×10⁶ in a 15cm petri disch (Corning Incorporated Life Sciences, Lowell, MA, USA) and, 24h later, infected with Lenti-IL-27HA, Lenti-IL-35HA, or Lenti-GFP. After 48h, IL-27HA, IL-35HA conditioned medium were collected for HA affinity column purification. 50mL supernatant from IL-27HA- or IL-35HA-expressing cells were centrifuged at room temperature for 15minutes at 20.000×g and then passed through a 0.22µm filter. Clarified supernatants were incubated at RT over-night with 0.2mL of anti-HA antibody agarose resin (cat. A2095, Sigma Aldrich) using an Amicon Pro centrifuge purification system (Merck Millipore). After three washes with PBS, bound material was eluted by applying 1mL of 0.1mg/mL HA peptide (cat. I2149, Sigma Aldrich) in PBS. Purified proteins were stored at −80°C.

CD4⁺ T cells polarization assay

Duplicate cultures of CD4⁺ cells/well in 200μl of RPMI were isolated from the spleens of C57Bl/6N mice. CD4⁺ T cells were purified using anti-CD4 beads (Milteny). Polarization was performed by stimulating with 5µg/mL of plated-bound anti-CD3 and 5µg/mL soluble anti-CD28 (BD Biosciences, Mountain View, CA) for 72h. Stimulation of T cells was set up under optimal culture conditions with or without recombinant cytokines and/or neutralizing antibodies. Th0: anti-CD3/anti-CD28; Th1: anti-CD3/anti-CD28, anti-IL4 (5µg/mL), mouse IL-12 (10ng/mL); Th17: anti-CD3/anti-CD28, mouse IL-6 (30ng/mL), human tgf-β (3ng/mL). After 24h, polarized T cells were treated with purified IL-27HA, IL-35HA, and recombinant IL-27 (R&D system) or recombinant IL-35 (Sigma Aldrich) at 10 and 50ng/mL. IL-27HA concentration was determined using the commercial ELISA described below. IL-35HA concentration was estimated by WB using IL-27HA as comparison. After 48h of cytokine stimulation, T cells were collected for RNA extraction and supernatants for cytokine determination.

RT-PCR

Total RNA was extracted from CD4⁺ T cells and from CNS infiltrated cells of the EAE mice with RNeasy Mini Kit (Qiagen). Genomic DNA was removed by treatment with DNAse I type (Qiagen). cDNA synthesis was performed using Thermoscript^TM RT-PCR system (Invitrogen). Arg-1 (Mm00475988_m1); inos (Mm00440502_m1); ym1 (Mm00657889_mH); cd274 (Mm00452054_m1); tbx21 (Mm00450960_m1); csf2 (Mm01290062_m1); IL-17a (Mm00439618_m1); rorc (Mm00441144_g1); foxp3 (Mm00475156_m1); IL-2 (Mm00434256_m1); IL-10 (Mm00439614_m1) and gapdh (4352339E) mRNA levels were measured by real-time RT-PCR (Applied Biosystem, Invitrogen). The 2^−ΔΔCT method was used to calculate relative changes in gene expression³⁵.

Isolation of CNS infiltrating leukocytes

Extracted brain and spinal cord tissues were incubated for 30minutes with 0.4mg/mL type IV collagenase (Sigma-Aldrich) and dissociated using a 19G syringe to obtain a homogenous cell suspension. Finally, CNS cells were enriched by a Percoll gradient as previously described³⁶.

Flow cytometry and sorting

Flow cytometry was performed using a CantoII (Becton Dickinson) and analysed with FlowJo software (tree star). Fluorochrome-conjugates monoclonal antibody (mABs) specific for CD45 (clone 30-F11), CD11b (clone M1/70), CD4 (clone RM4-5), CD3 (17A2), Ly6C (clone AL-21), Ly6G (clone 1A8), CCR2 (clone #47503) were purchased either from BD Biosciences, eBioscience, R&D and Biolegend.

For intracellular staining, cells were stimulated for 4h with phorbol 12-myristate 13-acetate (50ng/ml) and ionomycin (500ng/ml) in the presence of GolgiPlug (1:1000, BD Pharmigen), permeabylized using a Cytofix/Cytoperm Plus kit (BD Bioscience) and stained with the following fluochrome-conjugates monoclonal antibodies: GM-CSF (clone MP1-22E9), IL-17A (TC11-18H10) and IFNγ (clone XMG1.2) from BD Pharmingen. Dead cells were excluded using a Zombie Nir, Biolegend.

ELISA assay for mIL-27

Mouse IL-27 was measured in supernatants from the HA purification assay, in conditioned media and in CSF, withdrawn from mice cisterna magna by capillarity, of Lenti-IL-27HA-injected EAE mice, using a DUOset ELISA for mouse IL-27 (R&D Systems).

Western blot analysis

30μg of proteins or 10μl of Lenti-IL-27HA and Lenti-IL-35HA treated-mice CSF were subjected to SDS-12% polyacrylamide gel electrophoresis before blotting onto a PVDF membrane, PROTRAN Nitrocellulose Transfer Membrane (Cat. No. 8160576 WHATMAN). Membranes were blocked with 5% skimmed milk in Tris-buffered saline with 0.05% Tween 20 for 1h at RT, and were probed with Purified rabbit anti-HA tag polyclonal (ab175880) O/N at 4°C. A suitable secondary peroxidase-conjugated antibody was used for detection using ECL Immobilon Western Chemiluminescent HRP-substrate detection system (Millipore, Cat.No. WBK 250500) according to manufacturer’s instructions.

Mice

All procedures involving animals were performed according to the animal protocol guidelines prescribed by the Institutional Animal Care and Use Committee (IACUC) authorization no. 644 at San Raffaele Scientific Institute (Milan, Italy).

Six- to eight-weeks-old C57Bl/6 female mice were purchased from Charles River Laboratories (Calco, Italy). All mice were housed in specific pathogen-free conditions, in roomy cages, allowing free access to food and water. All efforts were made to minimize animal suffering and to reduce the number of mice used, in accordance with the European Communities Council Directive of November 24, 1986 (86/609/EEC).

IL-27HA and IL-35HA gene therapy

Chronic EAE was induced in female C57BL/6 mice by subcutaneous immunization with 300μl of 200μg per mouse of MOG_35–55 in Freund’s Adjuvant Incomplete liquid, IFA, (Sigma) supplemented with 8mgml−1 Mycobacterium tuberculosis (strain H37Ra; Difco, Lawrence, KS, USA). Pertussis toxin (500ng, List Biological Laboratories, Campbell, CA, USA) was injected i.v. on the day of the immunization and again 2 days later. IL-27HA and IL-35HA-expressing lentivirus or GFP-expressing lentivirus were injected in the cisterna magna (i.c of the mice) in preventive, one day post immunization, or in therapeutic, disease onset²⁰. Mice were weighed and scored for clinical signs daily up to the day of culling. Clinical assessment of EAE was performed according to the following scoring criteria: 0=healthy; 1=limp tail; 2=ataxia and/or paresis of hindlimbs; 3=paralysis of hindlimbs and/or paresis of forelimbs; 4=tetraparalysis; and 5=moribund or death. EAE mice were killed at 28–34 d.p.i for real-time PCR, histological, and FACS analysis.

Histological evaluation

At least five mice per group were perfused through the left cardiac ventricle with saline plus EDTA 0.5mM for 10min followed by fixation with cold 4% paraformaldehyde, PFA, (Sigma). Spinal cords and brains from EAE mice were dissected out and post-fixed in 4% PFA overnight. Four different staining were used: Hematoxylin and Eosin to detect inflammatory infiltrates, demyelination (Kluver Barrera), axonal damage (Bielshowsky), and immunohistochemistry for CNS infiltrating CD3+T (MCA1477, Serotec). Findings were quantified on an average of 10 complete cross-sections of spinal cord per mouse taken at eight different levels. The number of perivascular inflammatory infiltrates were calculated and expressed as the number of inflammatory infiltrates per mm², demyelinated areas and axonal loss were expressed as percentage of damaged area, and CD3+T cells were calculated and expressed as the number of cells per square millimetre.

The authors would like to thank G. Gullotta, T. Croese, and S. Di Toro for their assistance on FACS analysis. This work has been supported by Fondazione Italiana Sclerosi Multipla – FISM, grant no. 2010/R/20 (R.F.) and no. 2011/R/16 and 2015/R/11 (M.D.). We are grateful to Prof. Luigi Naldini for providing the lentiviral backbone and to Prof. P. Brown for helpful discussion.