Molecular and Functional Dissection of the H-2Db-Restricted Subdominant Cytotoxic T-Cell Response to Lymphocytic Choriomeningitis Virus

doi:10.1128/JVI.75.5.2468-2471.2001

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Journal of Virology, March 2001, p. 2468-2471, Vol. 75, No. 5
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.5.2468-2471.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Molecular and Functional Dissection of the H-2D^b-Restricted Subdominant Cytotoxic T-Cell Response to Lymphocytic Choriomeningitis Virus

Denis Hudrisier, Joëlle Riond, and Jean Edouard Gairin^*

Laboratoire d'ImmunoPharmacologie Structurale, Institut de Pharmacologie et de Biologie Structurale, CNRS, 31400 Toulouse, France

Received 29 August 2000/Accepted 30 November 2000

	ABSTRACT

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Infection of H-2^b mice with lymphocytic choriomeningitis virus (LCMV) generates an H-2D^b-restricted cytotoxic T-lymphocyte (CTL) response whose subdominantcomponent is directed against the GP92-101 (CSANNSHHYI) epitope.The aim of this study was to identify the functional parametersaccounting for this subdominance. We found that the two naturallyoccurring (genetically encoded and posttranslationally modified)forms of LCMV GP92-101 were immunogenic, did not act as T-cellantagonists, and bound efficiently to but were unable to formstable complexes with H-2D^b, a crucial factor for immunodominance. Thus, the H-2D^b-restricted subdominant CTL response to LCMV resulted not fromaltered T-cell activation but from impaired major histocompatibilitycomplex presentation properties.

	TEXT

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Infection of mice with lymphocytic choriomeningitis virus (LCMV) induces a cellular immune response mediated mainly by CD8⁺ cytotoxic T lymphocytes (CTL). In H-2^b mice, the immunodominant component of this CTL response is directedagainst three H-2D^b-restricted epitopes located in the nucleoprotein (NP) or glycoprotein(GP): NP396-404 (FQPQNGQFI), GP33-41 (KAVYNFATC), and GP276-286(SGVENPGGYCL) (5, 13, 17, 21). More recently, a subdominantcomponent has been identified in the context of H-2D^b restriction, which is directed against GP92-101 (CSANNSHHYI)(8, 18, 24). This epitope bears a glycosylation motif (NXS)which is N glycosylated in the mature viral protein (25) andcan be subject to posttranslational modification. The geneticallyencoded (N95) and posttranslationally modified (D95) forms ofLCMV GP92-101 are copresented at the surfaces of LCMV-infectedH-2^b cells (11).

Understanding the mechanisms responsible for the subdominance (versus immunodominance) of this viral antigen is an importantgoal, not only for a better knowledge of LCMV pathogenesis andits consequent immune response but also for future developmentsof antiviral vaccination strategies based on the use of subdominantepitopes (22, 24). The aim of this study was therefore toidentify the functional parameters that may explain the H-2D^b-restricted subdominant component of the CTL response againstLCMV.

The two naturally presented forms (N95 and D95) of LCMV GP92-101 are subdominant antigens. No efficient primary CTL response has been detected against the genetically encoded form N95 of GP92-101 following LCMV infectionof H-2^b mice (18, 24). However, the ability of the other naturallypresented form (D95) of LCMV GP92-101 to induce an anti-LCMV primaryCTL response has never been tested. C57BL/6 (H-2^b) mice were infected with 2 × 10⁵ PFU of LCMV Arm intraperitoneally. At the peak of the primaryresponse (day 8), spleen cells were explanted and then analyzedin two functional assays. First, an intracellular cytokine stainingassay was performed to determine the frequency of CD8⁺ T cells specific for the LCMV epitopes. Spleens cells were culturedfor 5 h in the absence (no stimulation) or presence of peptidesrepresenting the LCMV epitopes, stained for surface CD8 and intracellulargamma interferon (IFN- $gamma$ ), and analyzed by flow cytometry as previouslydescribed (16). As illustrated in Fig. 1, we confirmed previousstudies (16) by showing that the percentage of the CD8⁺ T-cell population against the two immunodominant epitopes NP396-404and GP33-41 was high (13.0% ± 2.9% and 20.2% ± 4.1%, respectively)and that the percentage of the population against the N95 formof GP92-101 was low (3.5% ± 1.6%). We were also able to detectthe presence of a small number of CD8⁺ T cells specific for the D95 form of GP92-101 (4.0% ± 0.8%),comparable to that of N95-specific CTL. The gated cells in theabsence of stimulation (no peptide) represented 3.0% ± 1.1% ofthe CD8⁺ T cells. These values are the means ± standard errors from fivemice. Second, a classical ⁵¹Cr release assay was performed to measure the lytic activity ofbulk splenocytes in response to target cells pulsed with the LCMVepitopes. As shown in Fig. 2, primary bulk splenocytes from LCMV-infectedC57BL/6 mice efficiently lysed target cells coated with the immunodominantepitope NP396-404 but not cells coated with either the N95 orD95 form of GP92-101, even at the highest concentration tested.These findings allow us to extend the subdominant properties ofLCMV GP92-101 previously observed for its genetically encodedform, N95 (16, 18, 24), to its posttranslationally modifiedform, D95. Clearly, however, the subdominance of LCMV GP92-101does not result from a lack of immunogenicity. Indeed, this viralepitope can efficiently sensitize H-2^b target cells to lysis by secondary CTL obtained after in vitrostimulation of spleen cells from LCMV-infected mice with the syntheticpeptide corresponding to the genetically encoded sequence (24).Also, LCMV GP92-101-specifc CTL were successfully generated afterimmunization of C57BL/6 mice with synthetic peptides followedby in vitro restimulation (11; also this study). The GP92-101-specificCTL we generated against N95 or D95 behaved differently. The anti-N95CTL were not specific for the N95 form used as an immunogen, sincethey also recognized the D95 form, even more efficiently (about100-fold; the 50% effective concentration [EC₅₀] of anti-N95 againstN95 was 1 nM, while that of anti-N95 against D95 was 0.01 nM).In contrast, the anti-D95 CTL recognized specifically and efficiently(EC₅₀ = 0.03 nM) the D95 peptide used as an immunogen but notthe N95 form of the viral antigen (or only at very high concentrations,i.e., an EC₅₀ of >1,000 nM). Regardless of the specificity profile,these results demonstrate that fully functional anti-GP92-101CTL precursors exist in the T-cell repertoire of H-2^b mice.

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FIG. 1. Frequency of CD8⁺ CTL specific for the N95 and D95 forms of GP92-101 during primary LCMV infection of C57BL/6 mice. C57BL/6 (H-2^b) mice were infected with LCMV Arm (2 × 10⁵ PFU) intraperitoneally. At the peak of the primary response (day 8), spleen cells were explanted, cultured in vitro for 5 h either with or without the indicated peptide (0.1 µg/ml), and stained for surface CD8 with anti-CD8 $alpha$ -Red 613 (Gibco BRL) and for intracellular IFN- $gamma$ with anti-IFN- $gamma$ XMG1.2-fluorescein isothiocyanate (Pharmingen), by following the procedure described by Murali-Krishna et al. (16). The numbers indicate the percentage of CD8⁺ cells that were positive for intracellular IFN- $gamma$ . Results shown are from a representative individual mouse from a group of five.

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FIG. 2. Sensitization by the LCMV NP396-404 and GP92-101 epitopes of H-2^b target cells to lysis by primary CTL. ⁵¹Cr-labeled H-2^b target cells were incubated in microtiter plates at 37°C with increasing concentrations of GP92-101 N95 and D95 and of NP396-404 used as a positive control. Bulk splenocytes from C57BL/6 mice infected with LCMV 8 days before the experiment were added at an effector/target ratio of 50:1. After 4 h of incubation at 37°C, the ⁵¹Cr content of supernatants was determined. The specific lysis was calculated as follows: 100 × [(experimental $-$ spontaneous release)/(total $-$ spontaneous release)].

The N95 form of LCMV GP92-101 does not inhibit the lytic activity of D95-specific CTL. Natural variants generated from multiple processing or mutation of the viral antigen can act as T-cell receptor (TCR) antagonists(12), leading to viral evasion from (1, 14, 15) or immunoregulationof (2) the antiviral CTL response. The question arose of whethercopresentation of the two forms of LCMV GP92-101 might be a causeof its subdominance, by means of TCR antagonism (11). The possibilitythat N95 acts as an antagonist of anti-D95 CTL and may play arole in the regulation of the anti-GP92-101 CTL response was thereforeexamined. We used a cold target inhibition assay of TCR antagonism(3) in which ⁵¹Cr-labeled RMA (a murine H-2^b T-lymphoma cell line) were pulsed with a suboptimal concentrationof D95 and cold RMA were pulsed with graded concentrations ofN95 or control peptide NP396-404. Target cells were washed toremove excess peptide and then mixed with D95-specific CTL. Asshown in Fig. 3B, no inhibition of lysis of D95-coated targetcells was observed in the presence of NP396-404 (as expected)or N95, even at the highest concentration tested, indicating thatN95 was unable to antagonize the lytic activity of anti-D95 CTL.This finding indicated that TCR antagonism was not a valid hypothesis.

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FIG. 3. Activation of anti-LCMV GP92-101, D95-specific CTL. (A) Agonism assay. ⁵¹Cr-labeled RMA were pulsed with increasing concentrations of D95 or N95 peptides (10¹² to 10⁷ M), and D95-specific CTL were added at an effector/target ratio of 10:1. After 4 h of incubation at 37°C, the ⁵¹Cr content of supernatants was determined. (B) Antagonism assay (cold target inhibition assay). ⁵¹Cr-labeled RMA were pulsed with a suboptimal concentration (33 pM) of the D95 peptide, and cold RMA were pulsed with increased concentrations (10¹⁰ to 10⁴ M) of N95 or NP396-404 for 1 h at 37°C. After three washes in culture medium to remove excess free peptides, ⁵¹Cr-labeled RMA and cold RMA were mixed at a 1:3 ratio. CTL were then added at a ratio of 10:1 with ⁵¹Cr-labeled RMA. After 4 h at 37°C, the supernatant was analyzed as described above.

Thus, neither a lack of a T-cell response nor altered TCR activation (antagonism) may account for the subdominant CTL responseto LCMV GP92-101. An alternative mechanism should therefore beconsidered. A protective CTL response to a subdominant epitopecan be influenced by the overall spectrum of viral peptides generatedwithin infected cells (6). However, no efficient primary CTLresponse is raised against LCMV GP92-101 even in mice infectedwith the GPV+NPV variant of LCMV, which lacks all three immunodominantH-2D^b epitopes (18), strongly suggesting that intrinsic propertiesof GP92-101 rather than competition with other antigens may beresponsible for itssubdominance.

Within the infected cells, major histocompatibility complex (MHC) class I presentation of the viral antigen is a crucial stepwhich may control its dominance or subdominance. Two distinctparameters must be considered: (i) the capacity of the peptideto bind to the MHC molecule (binding affinity) and (ii) the abilityof the peptide, once bound to the MHC, to form a stable complexwith the MHC (complex stability). These two parameters were thereforeanalyzed.

Both the N95 and D95 forms of LCMV GP92-101 bind to but dissociate rapidly from H-2D^b. By screening of the LCMV glycoprotein sequences for H-2D^b motif-fitting peptides, the nonmodified form (N95) of GP92-101 waspreviously identified as a high (50% inhibitory concentration[IC₅₀], <50 nM) (8) or intermediate (IC₅₀, 50 to 500 nM) (24)H-2D^b binder depending on the biochemical assay used. Interestingly,in both studies, the measured affinity of GP92-101 for H-2D^b was about 1 log better than that of the immunodominant epitopeGP33-41. However, the latter epitope displays somewhat controversialMHC binding properties, and the correlation between its affinityand its immunogenicity remains unclear (8, 9, 24). Nevertheless,the difference observed between the two epitopes suggests thata nonimmunodominant epitope (GP92-101) can compete efficientlywith a known immunodominant epitope (GP33-41) for binding to MHC.Furthermore, binding of GP92-101 to H-2D^b is not affected by mutation of N95 to D95 (11), a result predictablesince the side chain of residues at P4 of H-2D^b-restricted peptides has minimal interaction with the MHC bindinggroove (26). Thus, these data rule out MHC binding deficiencyand intermolecular competition for MHC class I presentation asfactors responsible for the subdominance of GP92-101.

The stability of peptide-MHC complexes is another important binding parameter which has been shown to correlate with the immunogenicityof the antigenic peptide (23). We therefore analyzed the stabilityof the complexes formed between LCMV GP92-101 and H-2D^b and compared it with that obtained with the three immunodominantH-2D^b-restricted LCMV epitopes NP396-404, GP33-41, and GP276-286. Forthat, the RMA-S mutant cells previously cultivated at 26°C werepulsed with the different peptides (1 µM) for 4 h at 37°C, washed,resuspended in culture medium, and incubated for different periodsof time at 37°C. At this temperature, peptides unable to formstable complexes with MHC molecules rapidly dissociate and theempty MHC molecules disappear from the cell surface, whereas stablecomplexes in which peptides are tightly bound to the MHC remainat the cell surface. As shown in Fig. 4 and summarized in Table1, the two immunodominant epitopes NP396-404 and GP33-41 formedvery stable complexes with H-2D^b, in agreement with previous studies (6). In contrast, thecomplexes between H-2D^b and any of the two forms of GP92-101 dissociated rapidly, witha half-life of less than 2 h. Interestingly, GP276-286, whichinduces an immunodominant but moderate CTL response (7, 16),formed molecular complexes of intermediate stability with H-2D^b. Thus, the inability to form stable complexes with the MHC moleculeis likely the main factor responsible for the subdominance ofthe LCMV GP92-101 epitope. However, the contribution of otherfactors, such as an intermediate binding affinity (24), to subdominancecannot be excluded.

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FIG. 4. Stability of the complexes formed between H-2D^b and the LCMV epitopes. RMA-S previously incubated at 26°C were pulsed with 1 µM peptide for 4 h at 37°C. After three washes at 4°C in phosphate-buffered saline containing 2% fetal calf serum, cells were resuspended in medium without fetal calf serum and then transferred to 37°C. At different times (0, 2, and 4 h), aliquots (2.5 × 10⁵ cells) were removed and stained for H-2D^b expression using the 28-14-8S mouse monoclonal antibody. Cells were then stained with a fluorescent (fluorescein isothiocyanate) secondary anti-mouse antibody and analyzed by flow cytometry. Results are expressed as percent fluorescence (100% at 0 h).

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TABLE 1. Characteristics of the H-2D^b-restricted primary CTL response to LCMV infection

The use of subdominant (versus dominant) epitopes presents a certain number of advantages for antiviral vaccination (22).Our demonstration that the H-2D^b-restricted subdominant component of the cytotoxic T-cell responseagainst LCMV does not result from a lack of a T-cell responseor altered T-cell activation but from impaired MHC presentationproperties of GP92-101 is of interest not only for fundamentalknowledge but also for potential therapeutic application. Indeed,manipulating an antigenic sequence to compensate for a defectin T-cell activation is far from mastered, since the rules governingTCR recognition are not fully elucidated. In contrast, the structuralrules governing peptide-MHC interactions are now well establishedand can be manipulated for therapeutic purposes (10). For example,enhanced MHC presentation of viral or tumor antigens can be successfullyachieved by modifying MHC anchor residues (20, 22). van derMost and coworkers showed that vaccination with LCMV GP92-101conferred protective immunity on mice (24). The two anchor residues(N at P5 and I at the C terminus) of LCMV GP92-101 are alreadyoptimal for H-2D^b binding (19). However, other structural elements, such as peptideconformation (4) or nonanchor residues (8), also controlthe presentation of viral peptides by H-2D^b. Identification and manipulation of these elements will helpin the design of a modified analog of LCMV GP92-101 with improvedMHC presentation properties (more specifically MHC complex stability)and thus with potentially increasedimmunogenicity.

	ACKNOWLEDGMENTS

This work was supported in part by grants from the Centre National de la Recherche Scientifique and Association pour la Recherchesur le Cancer (contract5485).

We thank J.-C. Guery for his kind gift of anti-IFN- $gamma$ XMG1.2-fluorescein isothiocyanateantibody.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratoire d'ImmunoPharmacologie Structurale, Institut de Pharmacologie et de BiologieStructurale, CNRS, 205 route de Narbonne, 31400 Toulouse, France.Phone: 33-561-175-530. Fax: 33-561-175-532. E-mail: gairin{at}ipbs.fr.

Present address: INSERM U395, CHU Purpan, 31059 Toulouse Cedex,France.

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1.	Bertoletti, A., A. Sette, F. V. Chisari, A. Penna, M. Levrero, M. De Carli, F. Fiaccadori, and C. Ferrari. 1994. Natural variants of cytotoxic epitopes are T-cell receptor antagonists for antiviral cytotoxic T cells. Nature 369:407-410[CrossRef][Medline].
2.	Carson, R. T., D. D. Desai, K. M. Vignali, and D. A. Vignali. 1999. Immunoregulation of Th cells by naturally processed peptide antagonists. J. Immunol. 162:1-4[Abstract/Free Full Text].
3.	De Magistris, M. T., J. Alexander, M. Coggeshall, A. Altman, F. C. Gaeta, H. M. Grey, and A. Sette. 1992. Antigen analog-major histocompatibility complexes act as antagonists of the T cell receptor. Cell 68:625-634[CrossRef][Medline].
4.	Gairin, J. E., and M. B. A. Oldstone. 1993. Virus and cytotoxic T lymphocytes: crucial role of viral peptide secondary structure in major histocompatibility complex class I interactions. J. Virol. 67:2903-2907[Abstract/Free Full Text].
5.	Gairin, J. E., H. Mazarguil, D. Hudrisier, and M. B. A. Oldstone. 1995. Optimal lymphocytic choriomeningitis virus sequences restricted by H-2D^b major histocompatibility complex class I molecules and presented to cytotoxic T lymphocytes. J. Virol. 69:2297-2305[Abstract].
6.	Gallimore, A., J. Hombach, T. Dumrese, H. G. Rammensee, R. M. Zinkernagel, and H. Hengartner. 1998. A protective cytotoxic T cell response to a subdominant epitope is influenced by the stability of the MHC class I/peptide complex and the overall spectrum of viral peptides generated within infected cells. Eur. J. Immunol. 28:3301-3311[CrossRef][Medline].
7.	Gallimore, A., T. Dumrese, H. Hengartner, R. M. Zinkernagel, and H. G. Rammensee. 1998. Protective immunity does not correlate with the hierarchy of virus-specific cytotoxic T cell responses to naturally processed peptides. J. Exp. Med. 187:1647-1657[Abstract/Free Full Text].
8.	Hudrisier, D., H. Mazarguil, F. Laval, M. B. A. Oldstone, and J. E. Gairin. 1996. Binding of viral antigens to major histocompatibility complex class I H-2D^b molecules is controlled by dominant negative elements at peptide non-anchor residues. Implications for peptide selection and presentation. J. Biol. Chem. 271:17829-17836[Abstract/Free Full Text].
9.	Hudrisier, D., M. B. A. Oldstone, and J. E. Gairin. 1997. The signal sequence of lymphocytic choriomeningitis virus contains an immunodominant cytotoxic T cell epitope that is restricted by both H-2D^b and H-2K^b molecules. Virology 234:62-73[CrossRef][Medline].
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