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Neurons are MHC class i-Dependent Targets for CD8 t cells upon neurotropic viral infection

PLoS Pathogens (2011) 7(11)
DOI: 10.1371/journal.ppat.1002393
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Abstract

Following infection of the central nervous system (CNS), the immune system is faced with the challenge of eliminating the pathogen without causing significant damage to neurons, which have limited capacities of renewal. In particular, it was thought that neurons were protected from direct attack by cytotoxic T lymphocytes (CTL) because they do not express major histocompatibility class I (MHC I) molecules, at least at steady state. To date, most of our current knowledge on the specifics of neuron-CTL interaction is based on studies artificially inducing MHC I expression on neurons, loading them with exogenous peptide and applying CTL clones or lines often differentiated in culture. Thus, much remains to be uncovered regarding the modalities of the interaction between infected neurons and antiviral CD8 T cells in the course of a natural disease. Here, we used the model of neuroinflammation caused by neurotropic Borna disease virus (BDV), in which virus-specific CTL have been demonstrated as the main immune effectors triggering disease. We tested the pathogenic properties of brain-isolated CD8 T cells against pure neuronal cultures infected with BDV. We observed that BDV infection of cortical neurons triggered a significant up regulation of MHC I molecules, rendering them susceptible to recognition by antiviral CTL, freshly isolated from the brains of acutely infected rats. Using real-time imaging, we analyzed the spatio-temporal relationships between neurons and CTL. Brain-isolated CTL exhibited a reduced mobility and established stable contacts with BDV-infected neurons, in an antigen- and MHC-dependent manner. This interaction induced rapid morphological changes of the neurons, without immediate killing or impairment of electrical activity. Early signs of neuronal apoptosis were detected only hours after this initial contact. Thus, our results show that infected neurons can be recognized efficiently by brain-isolated antiviral CD8 T cells and uncover the unusual modalities of CTL-induced neuronal damage. © 2011 Chevalier et al.

Figures

  • Figure 1. BDV infection induces MHC I expression on neurons. (A), Immunofluorescence analysis of non-infected (NI) and (B), BDV-infected neurons, 14 days post infection with cell-free BDV. BDV Nucleoprotein was detected using a rabbit polyclonal antibody, followed by an Alexa 488- coupled secondary antibody (green), while ßIII-tubulin neuronal protein was detected using a mouse monoclonal antibody, followed by an Alexa 594-coupled secondary antibody (red). (C) Representative dot plot examples of MHC I and neuron-specific Tau expression in non-infected (NI) or BDVinfected neurons. (D) Quantification of MHC I positive neurons. Data are represented as percentage of Tau+ neurons expressing MHC I. Results are expressed as means 6 sem of at least four independent experiments. ***, p,0.001 by Mann-Whitney U-test. (E) Representative fluorescence intensity profiles for MHC I expression between BDV-infected neurons (green) and non-infected neurons treated with either IFN-b (blue) or IFN-c+TTX (red). doi:10.1371/journal.ppat.1002393.g001
  • Figure 2. Characteristics of brain-purified CD8 T cells from BDV-infected rats. (A) Percentages of CD8+ versus CD4+ cells among TCRab+ cells purified from brain or cervical lymph nodes of infected rats. Values are expressed as means 6 sem of six independent experiments **, p,0.01 by Mann-Whitney U-test. (B) Determination by real-time quantitative RT-PCR of the relative mRNA levels of IFN-c, Granzyme B (GzmB), Fas-ligand (FasL) and Perforin in brain-purified CD8 T cells compared to cervical lymph node CD8 T cells of the same animal. Values were normalized for actin mRNA levels. Values are expressed as means 6 sem of four independent experiments. ***, p,0.001; **, p,0.01; and *, p,0.05 by paired Student’s t-test. (C) Percentage of IFN-c-producing cells amongst TCRab+CD8+ cells after 48h restimulation with BDV-infected (BDV-Lew) or non-infected (NI-Lew) Lewis fibroblasts, as determined by intracellular FACS staining. Results are expressed as means 6 sem of four independent experiments. *, p,0.05; **, p,0.01 by Mann-Whitney U-test. (D) Cytokine levels in supernatants of cocultures of CD8 T cells with neurons. Supernatants were assayed after 48 hours of culture using Luminex multiplex kits. Only levels of IFN-c and IL-10 are shown (see Figure S1 for other cytokines). Values are expressed as mean concentrations 6 sem of four independent experiments. **, p,0.01 by Mann-Whitney U-test. doi:10.1371/journal.ppat.1002393.g002
  • Figure 3. Quantitative analysis of CD8 T cell movement behavior in contact with neurons. CD8 T cells purified from the brain of BDVinfected rats were labeled with PKH-26 (red) and added to Calcein-AM labeled neurons (green) which were non-infected (A) or infected (B) with BDV. Randomly chosen trajectories of individual cells were automatically tracked using Imaris software. Trajectories are depicted as color-coded tracks to represent increasing time, from blue (start of imaging) to yellow (end of imaging). A representative imaging session of 15 min is shown in each case. (C), Determination of average CD8 T cell velocities for the different experimental conditions. Dots represent average cell velocities of individual cells (200 to 700 cells analyzed depending on the condition, see numbers below the graph), red bars indicate mean values. Analyses were performed using non-infected neurons (NI), non-infected neurons treated for 48 h with IFN-c+TTX, BDV-infected neurons or BDV-infected neurons treated with a neutralizing MHC I monoclonal antibody 1 h prior to washes and addition of CD8 T cells. P values were calculated using Kruskal-Wallis test. ***, p,0.001; n.s., not significant. (D) Relative frequencies of brain CD8 T cells as a function of their individual mean velocity, under the different conditions of culture. Arrows point to the mean velocity for each condition. doi:10.1371/journal.ppat.1002393.g003
  • Figure 4. Interaction with brain-purified CD8 T cells induces early morphological changes of BDV-infected neurons. (A) A representative BDV-infected neuronal network loaded with calcein AM (green) at the start (t = 0 min) and (B) 45 min after coculture with PKH-26 stained brain-derived CD8 T cells. (C) Representative example of the image analysis performed to quantify the formation of calcein beading figures. Upon subtraction between images shown in (A) and (B), the residual fluorescence signal corresponds to calcein beading. (D) Quantification of the differences in fluorescence values, expressed as arbitrary units (AU). Values are expressed as means6sem of 5 to 6 independent experiments. *, p,0.05; **, p,0.01 by Mann-Whitney U-test. doi:10.1371/journal.ppat.1002393.g004
  • Figure 5. Analysis of electrical properties of neurons upon contact with brain CD8 T cells. (A) Representative view of cortical neurons cultured in an MEA dish. Electrodes are spaced by 200 mm; electrode diameter is 30 mm. Original magnification, X50. (B) Quantitative analysis of the mean burst frequency for non-infected (NI) neurons and BDV-infected neurons upon coculture with brain CD8 T cells (at a ratio of 1:1). The mean burst frequency was first calculated under spontaneous conditions and at various times after the beginning of coculture. For each condition, data were acquired from 100 to 460 electrodes, from five independent experiments. Values are expressed as means 6 sem *, p,0.05; ***, p,0.001 by unpaired Student’s t-test. doi:10.1371/journal.ppat.1002393.g005
  • Figure 6. Quantitative analysis of neuronal apoptosis following incubation with brain CD8 T cells. Apoptosis was measured using the fluorescent probe FLICA, and levels of VAD-FMK fluorescence were determined on 5 randomly selected fields for each condition. This analysis was performed upon incubation for 2 hours (white bars) or 4 hours (black bars) with brain purified CD8 T cells (at a ratio of 1:1) using non-infected neurons (NI), BDV-infected neurons, or BDV-infected neurons treated with a blocking MHC I monoclonal antibody 1 h prior to washes and addition of CD8 T cells. Values are expressed as means 6 sem from 5 separate experiments. ***, p,0.001 by Mann-Whitney U-test. doi:10.1371/journal.ppat.1002393.g006

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CITATION STYLE

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Chevalier, G., Suberbielle, E., Monnet, C., Duplan, V., Martin-Blondel, G., Farrugia, F., … Gonzalez-Dunia, D. (2011). Neurons are MHC class i-Dependent Targets for CD8 t cells upon neurotropic viral infection. PLoS Pathogens, 7(11). https://doi.org/10.1371/journal.ppat.1002393

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