This Article Abstract Full Text (PDF) Supplementary Data Alert me when this article is cited Alert me if a correction is posted Services Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by De Palma, R. Articles by Bronte, V. Search for Related Content PubMed PubMed Citation Articles by De Palma, R. Articles by Bronte, V.

Therapeutic Effectiveness of Recombinant Cancer Vaccines Is Associated with a Prevalent T-Cell Receptor Usage by Melanoma-specific CD8⁺ T Lymphocytes

¹ Department of Clinical and Experimental Medicine II, University of Naples, Naples, Italy; Departments of ² Oncology and Surgical Sciences, ³ Pediatrics, and ⁴ Medical and Surgical Sciences, University of Padova, Padova, Italy; and ⁵ Department of Dermatology, University of Bonn, Bonn, Germany

	ABSTRACT

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Definition of immune variables that correlate with the antitumor activity of cancer vaccines is critical for monitoring immunotherapy protocols. To define surrogate end points predictive of the therapeutic efficacy of recombinant vaccines based on melanoma antigen tyrosinase-related protein (TRP)-2, we evaluated several properties of antigen-specific CD8⁺ T lymphocytes in single mice undergoing either prophylactic or therapeutic immunization. Predictive markers for the efficacy of genetic vaccination were identified in the prophylactic model used. Interestingly, the number of tetramer⁺ CD8⁺ T lymphocytes expanded in vitro after a single cycle of stimulation with the immunodominant TRP-2 peptide was of the highest predictive value. In the therapeutic model, no variable examined at a single mouse level predicted the long-term therapeutic effect. Mice that survived did not show the highest expansion of antigen-specific lymphocytes or the more functionally active effectors, ex vivo or after in vitro culture with the peptide antigen. Successful therapy correlated strictly with the skewing of the T-cell receptor repertoire of tetramer-sorted, TRP-2–specific CD8⁺ T lymphocytes, which showed a preferential chain usage with a common CDR3 region.

	INTRODUCTION

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Tyrosinase-related protein (TRP)-2 is a melanosomal enzyme defined as a melanocyte differentiation antigen because it is expressed in most mammalian melanocytes and melanomas. TRP-2 is the main antigenic target of the immune response elicited in mice by immunization with genetically modified B16 melanoma vaccine (1 , 2) . Although slight differences have been described under therapeutic versus prophylactic conditions (2) , the mouse immune response to TRP-2 is dominated by the generation of CD8⁺ T lymphocytes responsible for both the antitumor response and autoimmunity, i.e., skin depigmentation (vitiligo) due to normal melanocyte destruction (3) . Tumor-infiltrating lymphocytes isolated from melanoma patients also recognize TRP-2 peptides in the context of different class I HLA alleles. Mouse and human TRP-2 have about 80% homology at the protein level, and the peptide SVYDFFVWL (TRP-2_180–188) is presented in association with mouse H-2 molecule K^b and human HLA molecule A2 (1 , 4 , 5) .

Peripheral tolerance, which seems to limit the anti–TRP-2 response in the C57BL/6 strain, can be broken by xenoimmunization, or immunization with an altered source of antigen. Immunization with a recombinant adenovirus (rAd) encoding human TRP-2, in fact, elicited an immune response against the respective mouse homologue and completely protected C57BL/6 mice from a lethal melanoma challenge (6) . Tolerance could be also broken by linking the mouse self-antigen with a foreign immunogenic protein providing strong CD4 helper sequences, such as the fusion protein between the mouse TRP-2 gene product and the enhanced green fluorescent protein (EGFP) of jellyfish Aequorea victoria (7) . Whereas the induction of an effective immune response against TRP-1/gp75 was often accompanied by vitiligo, immunity to TRP-2, delivered by either plasmid DNA or recombinant viruses, was not always associated with widespread vitiligo (8 , 9) . These interesting findings delineate a window of opportunity between proautoimmune and therapeutic activity that could be exploited to promote the therapeutic effects of recombinant vaccines based on TRP-2.

Based on encouraging preclinical studies, melanoma-specific vaccines were designed and evaluated in clinical trials (10) . Unfortunately, partial or complete tumor regression was reported only in a minority of patients (11) . This was somewhat expected because most initial trials were conducted in patients with advanced metastatic disease. These trials were designed to identify surrogate end points with respect to vaccine efficacy in the absence of overt tumor regression. The most confounding results of cancer vaccine trials concern the absence of a clear-cut correlation between the clinical responses and the antigen-specific immune response detected in patient-derived T lymphocytes. In fact, vaccination with class I major histocompatibility complex (MHC)-restricted peptides can easily generate tumor-specific CD8⁺ T cells among the circulating lymphocytes of immunized patients, but there is no assay that unambiguously identifies those patients who will respond clinically to immunotherapy (11 , 12) .

To simultaneously analyze multiple aspects of the TRP-2–specific, CD8⁺ T lymphocyte-dependent response, we designed an experimental protocol to evaluate different immune variables in single mice after prophylactic or therapeutic immunization. In prevention experiments, after immunization with recombinant vaccines encoding TRP-2 antigen, mice underwent splenectomy. After recovering from surgery, they were challenged with a lethal intravenous inoculum of B16 melanoma cells to monitor tumor development. In the therapeutic model, splenectomy was performed in mice that had been previously inoculated with tumor cells and then vaccinated with recombinant vaccines. Fresh splenocytes were used to quantify the number of TRP-2–specific CD8⁺ T cells by cytofluorometry after staining with H-2 class I tetramers and to enumerate the antigen-specific effectors releasing interferon (IFN)- in an enzyme-linked immunosorbent spot (ELISPOT) assay. Moreover, by stimulating the antigen-specific T lymphocytes with the K^b-restricted, TRP-2_180–188 peptide for 5 days, peptide-stimulated mixed leukocyte cultures (MLPCs) were designed to expand limited numbers of TRP-2–reactive T lymphocytes. Finally, we studied the T-cell repertoire usage in tetramer-sorted, TRP-2–specific T lymphocytes recovered from peptide-stimulated cultures.

	MATERIALS AND METHODS

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Mice and Cell Lines.
C57BL/6 (H-2^b) mice (8 weeks old) were purchased from Charles River (Calco, Como, Italy). Animal care and procedures followed institutional guidelines, in compliance with national and international regulations. Mice used for in vivo tumor growth experiments were examined every day and euthanized when the tumor became ulcerated or when one of two perpendicular diameters reached 10 mm and their product was >50 mm². MBL-2 is a leukemia line (H-2^b) derived from a Moloney murine leukemia virus-infected C57BL/6 mouse; B16 is a melanoma line (H-2^b) spontaneously growing in C57BL/6 mice (provided by Dr. I. J. Fidler; M. D. Anderson Cancer Center, Houston, TX). B16LU8, a metastasizing melanoma cell line derived from repeated in vivo passage of B16, was kindly provided by Dr. James C. Yang (Surgery Branch, National Institutes of Health, Bethesda, MD). The 293-K^b cell line is a human embryonic kidney cell line stably transfected with plasmid expressing the H-2 K^b class I molecule. Cell lines were maintained in Dulbecco’s modified Eagle’s medium (Invitrogen, Carlsbad, CA) supplemented with 2 mmol/L L-glutamine, 10 mmol/L HEPES, 20 µmol/L 2-mercaptoethanol, 150 units/ml streptomycin, 200 units/ml penicillin, and 10% heat-inactivated fetal bovine serum (Invitrogen). TRP-2–specific cytotoxic T lymphocyte (CTL) clones 8 and 24 were obtained from a C57BL/6 mouse immunized with pcDNA3-trp-2 plasmid, as described in ref. 8 , by several in vitro restimulations with syngeneic splenocytes pulsed with TRP-2_181–188 peptide (10 µmol/L) and after limiting dilution cloning.

Viruses.
Adenoviruses used in this study were constructed through Cre-lox recombination with reagents generously provided by Dr S. Hardy (Somatix, Alameda, CA). Adenoviruses were propagated on 293 cells, purified by cesium chloride density gradient centrifugation, dialyzed according to standard protocols (6 , 7) , and then stored at –70°C. All vectors used express only the antigen of interest under the cytomegalovirus immediate early promoter. The recombinant vaccinia virus (rVV) encoding the human gp100 epitope as minigene was a kind gift of Dr. Nicholas P. Restifo (National Institutes of Health, Bethesda, MD). Immunization was performed as described previously (13) .

DNA Immunization.
Preparation of the VR1055-P15 plasmid encoding the p15E portion of the env gene has been described previously (14) . Plasmid amplification was performed with the Endofree plasmid mega kit (Qiagen, Hilden, Germany), following the manufacturer’s instructions. Plasmids were purified with Qiagen columns assuring an endotoxin-free DNA preparation (Qiagen GmbH, Hilden, Germany). For DNA immunization, C57BL/6 mice were anesthetized by avertin inoculation and received intramuscular injection with 100 pmol/L cardiotoxin (Latoxan, Rosans, France). Five days later, mice received intramuscular injection with 100 µg of plasmid DNA in 100 µL of saline.

In vivo Antibody Treatment.
Mice were depleted of either CD4⁺ or CD8⁺ T cells by four intraperitoneal injections of 200 µg of affinity chromatography-purified GK1.5 (anti-CD4) or 2.43 (anti-CD8) monoclonal antibody (mAb). Depleting mAbs were administered 2 days before and 0, 4, and 8 days after subcutaneous challenge with tumor cells. In therapy experiments, the mAbs were administered 1 day before and 0, 4, and 8 days after vaccination with rAd. Depletion was consistently >98%. As a control, anti-Escherichia coli ß-galactosidase (GL117.14; rat IgG2a) was used at the same dose.

Mixed Leukocyte Peptide Culture.
Three weeks after plasmid DNA inoculation, spleens were removed, and 2.5 x 10⁷ splenocytes were stimulated in vitro in a MLPC with 1 µmol/L of a nonamer peptide corresponding to amino acids 180 to 188 of TRP-2 protein (SVYDFFVWL). K^b-restricted peptides corresponding to amino acids 604 to 611 of p15E protein (KSPWFTTL, p15E peptide) and control peptide corresponding to the amino acids 96 to 103 of ß-galactosidase (ß-gal) protein (DAPIYTNV) were synthesized and purified by Technogen (Naples, Italy) and were >95% pure, as indicated by analytical high-performance liquid chromatography. The peptide KVPRNQDWL, spanning amino acids 25 to 33 of human gp100, was a kind gift of Dr. Nicholas P. Restifo. The cultures were set up in 10 mL of Dulbecco’s modified Eagle’s medium-10% fetal bovine serum, maintained in 25-cm² tissue culture flasks (Falcon; Becton Dickinson, Lincoln Park, NJ) for 5 days at 37°C under 5% CO₂, and then tested in either IFN- or ⁵¹Cr release assay.

Tumor Protection and Therapy.
Three weeks after immunization, mice were challenged subcutaneously with a lethal dose of B16 melanoma cells (2 x 10⁴) and then monitored for 100 days after tumor injection. Tumor growth was monitored every 3 days by caliper measurement. Alternatively, C57BL/6 mice were inoculated intravenously with 10⁵ B16LU8 cells. Lungs were removed 14 days after challenge, and pulmonary metastases were counted in a blind fashion. In therapy experiments, the same dose of tumor cells was used, but tumor was injected 3 days before immunization. All the in vivo experiments were conducted in mice randomized before tumor injection or before treatment for the therapeutic model. Mice were bred in filtered cages placed inside biohazard closets. For the adoptive transfer, B6 mice were inoculated with 10⁵ B16LU8 tumor cells via tail vein injection on day 0. On day 3, 5 x 10⁶ TRP-2–specific CTLs were administered intravenously, and 30,000 IU of recombinant interleukin (IL)-2 were given intraperitoneally twice a day for 3 days.

Synthesis of Major Histocompatibility Complex/Peptide Tetrameric Complexes.
Soluble H-2–peptide tetramers were produced using a previously described method (14) . Soluble purified complexes were biotinylated using BirA enzyme (Avidity, Denver, CO). Phycoerythrin (PE)-labeled tetramers were produced by mixing the biotinylated complexes with Extravidin-PE (Sigma, St. Louis, CO) and validated by staining CTL clones with the appropriate specificity. Each tetramer batch was titrated and used at the optimum concentration (5 µg/mL) of K^b heavy chain.

Cell Staining, Flow Cytometry, and Cell Sorting.
Fresh or in vitro stimulated splenocytes (10⁶ per sample) were resuspended in 50 µL of fluorescence-activated cell sorting (FACS) buffer (0.9% NaCl solution containing 2% bovine serum albumin and 0.02% NaN₃; both from Sigma) with antimouse Fc- receptor 2.4G2 mAb (ATCC HB-197) for 10 minutes at room temperature to reduce the nonspecific staining. Cells were further labeled with either PE-conjugated TRP-2 tetramer-PE (TRP-2-TET, 5 µg/mL) or ß-gal tetramer-PE (ß-gal-TET) for 20 minutes at room temperature. Each sample was then stained at 4°C with rat antimouse CD8-Tricolor (0.1 µg per 10⁶ cells; clone CTCD8; Caltag, Burlingame, CA) and with hamster antimouse CD3-fluorescein isothiocyanate (1 µg per 10⁶ cells; clone 145-2C11; Caltag). Before analysis, cells were washed twice, resuspended in FACS buffer, and analyzed with a FACSCalibur flow cytometer (Becton Dickinson, San Jose, CA). Data were analyzed using Cell Quest software (Becton Dickinson). The triple-positive cells (CD3⁺/CD8⁺/TRP-2-TET⁺) were sorted to obtain highly purified populations using a FACSVantage DiVa (Becton Dickinson) equipped with a 488-nm argon laser (I 305C-BD; Innova Coherent, Santa Clara, CA), at a rate of 8,000 to 12,000 cells per second. The sorted populations used in each experiment were >97% pure. Adequate controls regarding the cell viability were performed using light-scattered parameters and propidium iodide/annexin V staining. The triple-positive dead cells were excluded from the sorting procedure using light-scattered parameter in the back gate approach.

⁵¹Cr Release Assay.
The ⁵¹Cr-labeled target cells (2,000 cells per well) were incubated with effector cells at various effector to target ratios in 96-well microplates (Falcon; Becton Dickinson). After a 6-hour incubation at 37°C, supernatants were harvested, and radioactivity was counted in a microplate scintillation counter (Top-Count; Packard Instruments Co., Meriden, CT). For peptide pulsing, ⁵¹Cr-labeled target cells (10⁶ per mL) were incubated with relevant peptides (1 µmol/L, final concentration) for 30 minutes at 37°C and then washed twice before use. In cold target inhibition assays, 5 x 10⁶ splenocytes from mice immunized with rAd were stimulated in vitro with 10⁵ -irradiated syngeneic MCA38 cells, which were previously infected for 18 hours with Ad-human TRP (hTRP)-2 at a multiplicity of infection = 100, in the presence of 10 IU of recombinant IL-2. For the assay, unlabeled inhibitor B16, YAC-1, ß-gal–loaded 293K^b cells, or TRP-2–loaded 293K^b cells were seeded together with labeled B16 cells at different cold to hot target ratios. CTLs from the cultures were then added at an effector to hot target ratio of 100. The percentage of inhibition by cold targets was calculated as follows: inhibition (%) = 100 x [1 – lysis of CTLs with cold targets (%)/lysis of CTLs in the absence of cold targets (%)].

Enzyme-Linked Immunosorbent Assay.
Splenocytes (10⁵ cells) from MLPCs were restimulated for 24 hours in triplicate wells with an equal amount of target cells; the supernatants were harvested and tested for the IFN- released in a sandwich enzyme-linked immunosorbent assay (ELISA) assay (Endogen, Boston, MA).

Enzyme-Linked Immunosorbent Spot Assays.
The mouse IFN- development Module System Kit (R&D System Inc., Minneapolis, MN) was used according to the manufacturer’s instructions. Development was performed with the ELiSpot Blue color module (R&D System Inc.), and the number of spots was counted blindly by two operators under a dissecting microscope and expressed as the mean number of spots ± SE of triplicate determinations. Each mean value was subtracted from the one derived from effector cells cultured with target cells pulsed with an irrelevant peptide.

RNA and Complementary DNA Preparation for T-Cell Repertoire Analysis.
RNA was extracted using guanidium hydrochloride-containing Trizol reagent (Life Technologies, Inc., Gaithersburg, MD) according to the manufacturer’s instructions. First-strand cDNA synthesis was performed using oligo(dT) as a primer for reverse transcription of 1 µg of total RNA using Moloney murine leukemia virus reverse transcriptase (Life Technologies, Inc.) as described previously (15) .

Polymerase Chain Reaction Amplification for T-Cell Receptor Genes.
Polymerase chain reaction (PCR) amplification was performed as reported in detail elsewhere (15) . Briefly, after titration of the different templates, cDNAs were amplified for 30 cycles under nonsaturating PCR conditions. The T-cell receptor (TCR) repertoire was analyzed using a panel of TCR BV and AV family-specific primers by PCRs as described previously (15 , 16) . In each PCR reaction, the common TCR- or -ß primer was labeled at the 5' end with 5' 6-carboxyfluorescein. In addition to the TCR BV or AV family-specific and constant primers, the single reaction also contained a ß-actin–specific primer pair amplifying a 6-carboxyfluorescein–labeled 320-bp product as an internal PCR control for verification of cDNA integrity and the fidelity of the single PCR reactions (17) . The TCR AV5 repertoire was also screened by a PCR reaction with a specific AJ primer in place of the TCR Constant .

T-Cell Receptor-CDR3 Length Analysis.
After the amplification, the TCR-CDR3 length analysis was evaluated by the method known as spectratyping or immunoscope (15, 16, 17, 18) . According to this technique, the composition of each BV TCR family is visualized by running the PCR products for the different TCR families on a sequencing gel (15, 16, 17, 18) . Normally, each TCR family is resolved by this technique as a series of bands having a Gaussian distribution. Each alteration, in either the distribution or intensity of single bands, represents a perturbation in the given BV TCR family (15, 16, 17, 18) . In brief, an equivalent volume of PCR-labeled product was mixed with formamide dye-loading buffer and 0.2 µL of Rox-labeled size marker (Applied Biosystems, Foster City, CA), heated at 94°C for 2 minutes, and run on a sequencing gel in a fluorescence-based DNA sequencer (377 abi; Applied Biosystems). The data were analyzed by means of Genescan software (Applied Biosystems), which allows for the visualization of gel bands as chromatograms and assigns size and peak areas to different PCR products Sequencing of single TCR AV5 spectratype bands was performed using an internal primer and automated sequencing according to an established protocol (15) .

Clonotypic Analysis of TCR AV5.
The clonotypic analysis and frequency analysis of the given clonotype among the tetramer-enriched lymphocytes was analyzed, as described recently (19 , 20) , using a primer based on the AV5 sequence found in mouse T-cell clone 24 recognizing B16 melanoma. Briefly, real-time PCR was performed in a 5700 Thermal Cycler (Applied Byosistems), using the 5' nuclease assay. For the clonotypic analysis, we designed a primer specific for the CDR3 region of the whole TCR AV plus a primer specific for TCR AV5. All of the primers were designed using Primer Express software (Applied Byosistems). To assess the frequency of the clonotypic transcripts among the transcripts for the entire TCR AV repertoire, two series of quantitative PCRs were carried out in parallel, using the AV5 primer and the TaqMan probe, and either the clonotypic primer or the Constant AV primer. The corresponding threshold cycles (CT) for the clonotype (CTc) and the whole AV (Cta) were measured. Clonotype frequency was determined as the ratio f (clonotype) = Corr x 2 Cta – CTc, where Corr is a correcting factor accounting for the difference in amplification efficiency of different primer pairs (19) .

Statistical Analysis.
The Wilcoxon Mann-Whitney U test was used to examine the null hypothesis of rank identity between two sets of data. Kaplan-Maier plots and the Mantel-Haenszel test were used to compare survival of mice belonging to different treatment groups. Spearman rank correlation, a distribution-free analog of correlation analysis, was applied to compare two independent discrete random variables. All P values presented are two-sided.

	RESULTS

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
Immunization with Recombinant Adenovirus Encoding Human trp-2 (rAd-hTRP-2) Induces Therapeutic CD8⁺ T Lymphocytes Recognizing Mouse TRP-2_180–188 Peptide.
Xenoimmunization with rAd-hTRP-2 prevented the development of lung metastases after challenge with B16 melanoma in all vaccinated mice (Fig. 1A) . This effect was entirely mediated by CD8⁺ T lymphocytes because depletion of CD8⁺ T cells, but not CD4⁺ T cells, abrogated the preventive activity (Fig. 1A) . The vaccination protocol generates an antigen-specific CTL response against the immunodominant K^b-restricted TRP-2_180–188 peptide. In fact, splenocytes from mice immunized with rAd-hTRP-2 and stimulated in vitro with syngeneic cells infected with the same virus showed a strong cytotoxic activity against B16 cells and 293K^b pulsed with the TRP-2_180–188 peptide, but not toward control cells pulsed with the irrelevant ß-gal_96–103 peptide (Fig. 1B) . As expected, cytotoxicity against B16 cells was abrogated in a dose-dependent fashion by the addition of an excess of cold B16. The same competition curve was obtained with TRP-2–pulsed 293K^b cells, but not with either 293K^b cells loaded with the irrelevant ß-gal peptide or the natural killer target YAC-1 cells (Fig. 1B) , suggesting that the TRP-2–specific CTLs were responsible for all or most of the lytic activity of the cultures stimulated with the whole rAd-hTRP-2.

View larger version (25K): [in this window] [in a new window]   Fig. 1. Immune response elicited by rAd-hTRP-2 is dominated by CD8+ T lymphocytes recognizing the mouse epitope. A. Depletion of CD8+ T lymphocyte prevents the prophylactic activity of vaccination with rAd-hTRP-2. Groups of five C57BL/6 mice were immunized intraperitoneally with 109 plaque-forming units (PFU) per mouse of either rAd-hTRP-2 or the control rAd-EGFP. Mice immunized with rAd-hTRP-2 were further depleted of various immune cells with specific mAbs, as described in Materials and Methods. Pulmonary metastases of B16LU8 melanoma were counted in a blind fashion in lungs removed 14 days after challenge and plotted as mean ± SE. No significant statistical difference was found between the mice receiving the control rAd and those depleted of CD8+ T cells. For all other groups, P < 0.001 versus Ad-EGFP. B. CTL response against mouse TRP-2180–188 epitope. Spleens of C57BL/6 mice inoculated with rAd-hTRP-2 were surgically removed 14 days after vaccination, and splenocytes were cultured for 6 days in the presence of -irradiated syngeneic tumor cells infected with rAd-hTRP-2. Splenocytes were then tested in a 6-hour 51Cr release assay against 293Kb cells pulsed with 5 µg/mL of either TRP-2180–188 or ß-gal96–103 peptide or against B16 melanoma cells (left panel). Effector to target cell ratios are indicated; spontaneous release never exceeded 20%. Titrated numbers of cold TRP-2–pulsed 293Kb cells, ß-gal–loaded 293Kb cells, the natural killer target YAC-1 cells, and B16 cells were admixed to hot B16 cells and tested in a standard cytotoxicity assay with the same effectors (right panel). Values are expressed as means of triplicates of the percentages of lysis inhibition of B16 cells at an effector to hot target ratio of 100. The data shown are representative of at least three independent experiments. C. Absence of epitope spreading after tumor rejection. Five C57BL/6 mice in each group were immunized with rAd-hTRP-2, rAd-EGFP, plasmid DNA encoding p15E (p15E-DNA), or rVV expressing the altered (human) peptide of gp100 antigen. Spleens were removed 14 days after immunization and pooled to set up MLPCs with 1 µmol/L of the indicated peptides (No Tumor). Distinct groups of mice immunized with either rAd-EGFP or rAd-hTRP-2 were challenged intravenously with 105 B16LU8 cells and euthanized 14 days later to count pulmonary metastases (>300 and 0.8 ± 0.3 for the two groups, respectively) and set up MLPCs with the indicated peptides (Tumor). Splenocytes (105 cells) from MLPCs were restimulated for 24 hours in triplicate wells with an equal amount of either MBL-2 or B16 melanoma cells; the supernatant was then harvested and tested for released IFN- in a sandwich ELISA assay. The SD of the triplicate determinations for each effector/stimulator combination was <10%, and IFN- measured in control wells containing either effectors or stimulators alone did not exceed the lowest amount of IFN- detectable in our assay (i.e., 200 pg/mL). Data ± SE are from one representative experiment.

Analysis of Preventive Vaccination with Recombinant Adenovirus Encoding trp-2.
To evaluate the efficacy of different immunogens, the rAds encoding either green fluorescent protein fused to mouse TRP-2 [mTRP (rAd-EGFP-mTRP-2)] or murine TRP-2 (rAd-mTRP-2) were compared with rAd-hTRP-2. Mice underwent splenectomy 14 days after vaccination with different rAds. Splenocytes were used for staining with H-2 K^b tetramers assembled with the TRP-2_180–188 peptide (TRP-2-TET) as effectors in the ELISPOT assay and for MLPC. After 5 days, we performed tetramer staining and IFN- release from the MLPC. On day 21, these mice were challenged with an intravenous lethal inoculum of B16 melanoma cells. Fourteen days later, lungs were removed, and pulmonary metastases were counted in a blind fashion (Supplemental Fig. S1A).

As expected, immunization with rAd-mTRP-2 did not prevent tumor take (Fig. 2A) . After immunization with rAd-hTRP-2 but not with rAd-mTRP-2, all mice showed significant changes in the immunologic variables examined (ELISPOT assay, TRP-2-TET⁺ cells ex vivo and in MLPC, and IFN- released by MLPC-derived lymphocytes, Fig. 2B–D ). The fusion product, EGFP-mTRP-2, delivered by rAds also conferred protection from challenge. However, whereas MLPC-derived T lymphocytes released IFN- when cocultured with peptide-pulsed K^b target cells, there was no significant recognition of the B16 melanoma cells, suggesting the generation of low avidity effectors (Fig. 2C) . To further examine their relationship, we compared the number of pulmonary metastases and the percentage of TET⁺ lymphocytes in MLPC. The experimental data fit a two-parameter exponential decay curve (metastasis fraction = 0.48e^{–2.53(%Tet+cells}); Rsqr = 0.996) strongly suggesting that every increment in the number of TRP-2-TET⁺ cells affects the tumor progression at a fixed rate: Small increments are highly effective until a plateau is reached in the antitumor effect (Fig. 2E) . These results indicate that predictive markers of the efficacy of genetic vaccination can be found in a prevention model. In particular, the number of TRP-2-TET⁺ lymphocytes expanded in vitro after a single cycle of stimulation with the peptide had the highest predictive value.

View larger version (24K): [in this window] [in a new window]   Fig. 2. Multivariable analysis of T-cell response in prophylactic vaccination with rAd. A. C57BL/6 mice (n = 10; n = 9 only for mice immunized with rAd-EGFP-mTRP-2) were vaccinated with rAd encoding different antigens. The mice were challenged intravenously with 105 B16LU8 melanoma cells 25 days after vaccination. The reduction in metastasis number observed in mice immunized with rAd-hTRP-2 and rAd-EGFP-mTRP-2 was significant (P < 0.001) in comparison with the control group treated with rAd-EGFP. Data are from two cumulated experiments. B. The same mice described in A were splenectomized 21 days after rAd vaccination (before tumor challenge) for functional analysis. This panel shows IFN- release by whole splenocytes stimulated in vitro with TRP-2180–188 peptide for 24 hours in ELISPOT assay. The number of spots differs significantly (P < 0.01) in the group treated with either rAd-hTRP-2 or rAd EGFP-mTRP-2 compared with those treated with rAd-EGFP control virus and rAd-mTRP-2. C. Splenocytes isolated 21 days after immunization with rAd were cultured in MLPCs, and the cultures were tested for IFN- release against B16 cells, MBL-2 pulsed with TRP-2180–188 peptide, and unpulsed MBL-2. The difference between IFN- released against pulsed and unpulsed MBL-2 is reported. Statistics for pulsed MBL-2 targets are as follows: rAd-EGFP-mTRP-2 versus rAd-EGFP, P = 0.027; and rAd-hTRP-2 versus rAd-EGFP, P < 0.0001. Statistics for B16 target are as follows: rAd-EGFP-mTRP-2 versus rAd-EGFP, P = 0.17; and rAd-hTRP-2 versus rAd-EGFP, P = 0.008. D. Cytoflourometric analysis of CD3+/CD8+/TRP-2-TET+ cells in mice described above. The splenocytes were stained ex vivo, as soon as the spleens were removed, and after 5 days of culture with TRP-2180–188 peptide (MLPC). Statistics for ex vivo stained cells are as follows: rAd-EGFP-mTRP-2 versus rAd-EGFP, P < 0.0001; and rAd-hTRP-2 versus rAd-EGFP, P < 0.0001. Statistics for splenocytes derived from MLPCs are as follows: rAd-EGFP-mTRP-2 versus rAd-EGFP, P = 0.004; and rAd-hTRP-2 versus rAd-EGFP, P = 0.003. E. Analysis of correlation between the number of metastases in mice immunized with rAd-EGFP-mTRP-2 and the number of CD3+/CD8+/TRP-2-TET+ MLPC splenocytes of the same mice. A correlation was detected according to a nonparametric statistic test (Spearman’s rank, correlation = –0.955; P = 0.001). The best curve fitting the data (Rsqr = 0.996) is the two-parameter exponential curve described by the formula Y = 0.44e–2.53X, in which Y = metastasis fraction, and X = percentage of Tet+ cells. One outlier was excluded from the analysis.

View larger version (26K): [in this window] [in a new window]   Fig. 3. rAd encoding hTRP-2 has a therapeutic effect on tumor-bearing mice. A. Mice were injected subcutaneously with 2 x 104 B16 melanoma cells. Three days later, they received a single intraperitoneal inoculation of 109 PFU of rAd encoding EGFP, mTRP-2, or hTRP-2. Results are the sums of two independently performed experiments with five mice in each treatment group. The statistical analysis was performed according to the Mantel-Haenszel test (rAd-EGFP versus rAd-mTRP-2, P > 0.05; rAd-EGFP versus rAd-hTRP-2, P 0.0001; rAd-hTRP-2 versus rAd-mTRP-2, P = 0.0016). B. To identify the effector population responsible for the antitumor effect, mice were depleted by intraperitoneal injections of either anti-CD4, anti-CD8, or control mAb (as described in Materials and Methods) before immunization with rAd-hTRP-2. Mice that received the rAd-EGFP were used as a negative control group. The appearance of tumors greater than 2 x 2 mm was plotted as a function of time. The Mantel-Haenszel test gave P = 0.026 for Ad-EGFP versus Ad-hTRP-2 + control mAb, P = 0.044 for the Ad-EGFP versus Ad-hTRP-2 + anti-CD4 mAb, and P = 0.25 (nonsignificant) for Ad-EGFP versus Ad-hTRP-2 + anti-CD8 mAb. Duplicate experiments confirmed these results.

View larger version (26K): [in this window] [in a new window]   Fig. 4. T-cell repertoire analysis of TRP-2–specific lymphocytes. A. Three-day–old melanoma-bearing mice were immunized with rAd-hTRP-2 and monitored for survival. Three weeks after immunization, spleens were removed, splenocytes stimulated with TRP-2180–188 peptide, and CD3+/CD8+/TRP-2-TET+ cells were isolated by high-speed flow cytometry sorting. T-cell repertoire analysis for BV and AV gene usage in sorted cells was analyzed by spectratyping. A shows a synopsis of AV and BV gene usage in two animals, one tumor regressor and one progressor. White boxes indicate that the corresponding TCR family (AV or BV) has a normal, Gaussian-like repertoire; the incomplete boxes indicate the absence of the given family; right-hatched boxes indicate a skewed TCR family, characterized by a severe alteration in the Gaussian trend; and black boxes indicate a given TCR family in which a predominant peak is found by CDR3-length analysis. Similar results were found in all of the animals studied (shown in B). B. Detailed analysis of the TCR AV5 family in all animals studied. Amplification was performed using a TCR AV5-specific primer paired with a primer amplifying AJ41 in place of a primer amplifying for the Constant region. Left histograms show TCR AV5 in the animals that survived for >90 days after therapy with rAd-hTRP-2. The predominant peak, corresponding to a PCR product of 172 bp, was further characterized by sequencing analysis and found to be composed mainly of the sequence found in the TRP-2–specific CTL clone 24. Right histograms show the peaks for progressor mice. Numbers indicate the day of death after tumor challenge. C. To assess the frequency of clonotype shown in B, clonotypic analysis was performed using a primer for the CDR3 coding region of clone 24. The mean frequency ± SE of the mRNA codifying for this particular TCR AV5 clonotype in comparison with the mRNA of the whole TCR- repertoire is shown for the two groups of mice described in B.

Clonotype Expanded in Tumor Regressors Belongs to CTL Clones That Can Recognize TRP-2 with High Avidity.
As mentioned above, the CDR3 sequence that revealed the T-cell clonotype discriminating tumor regressors from progressors was originally found in CTL clone 24. Interestingly, the CTL clones 8 and 24, obtained by the same cloning procedure from the splenocytes of a TRP-2–vaccinated C57BL/6 mouse, shared a common AV gene (GenBank accession numbers AY089787 and AY089788, respectively) but had different BV rearrangements (GenBank accession numbers AY089784 and AY089785, respectively). This allowed us to investigate the properties of TRP-2–specific clones that differed only in the TCR ß-chain. Both clones 8 and 24 were able to lyse a syngeneic cell line pulsed with TRP-2_180–188 (Fig. 5A) . However, a titration assay performed to evaluate the functional TCR avidity for the TRP-2_180–188-K^b antigenic complexes clearly indicated that CTL clone 24 possessed a somewhat higher avidity (Fig. 5A) . In fact, clone 24 exhibited an EC₅₀ (2 x 10^–11 mol/L) that was about 10 times lower than the EC₅₀ of clone 8 (2.5 x 10^–10 mol/L). In agreement with these results, both clones released similar levels of INF- when stimulated with peptide-pulsed syngeneic cells, but only clone 24 was able to secrete INF- against B16 parental melanoma and the variant B16LU8 (Fig. 5B) . Taken together, these data suggest that TCR- usage is predominantly shaped by the recognition of TRP-2. However, the ß-chain contributes considerably in determining the function and avidity of specific T cells.

View larger version (21K): [in this window] [in a new window]   Fig. 5. CTL clone 24 recognizes TRP-2 antigen with high avidity. A. The lytic activity of TRP-2–specific CTL clones 8 and 24 was evaluated in a 4-hour incubation 51Cr release assay at an effector to target ratio of 5:1 against MBL-2 target cells incubated with different TRP-2180–188 peptide concentrations, as indicated. B. Specific INF- release (pg/mL) was quantified by sandwich ELISA assay in the supernatant of cultures comprising the same CTL clones described in A cocultured for 24 hours with B16 melanoma cell lines, MBL-2 pulsed with the irrelevant ß-gal peptide, or TRP-2 peptide. C. The histograms show the number ± SE of pulmonary metastases in C57BL/6 mice inoculated with IL-2 alone or in conjunction with TRP-2–specific CTL clones 8 or 24 three days after intravenous injection of B16LU8 melanoma cells. Untreated C57BL/6 mice served as controls. Data were derived from the sum of two separate experiments, with n = 10 for each group.

	DISCUSSION

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
In the present study, a multivariable analysis of the CD8⁺ T-cell response in mice vaccinated with different recombinant vaccines encoding the melanoma antigen TRP-2 delineated three main situations. The simplest finding involved the activity of the powerful rAd-hTRP-2 vaccine in prophylaxis of tumor challenge. All of the mice mounted a vigorous immune response against the mouse K^b-restricted epitope, as indicated by the significant changes in the number and functions of TRP-2–specific T lymphocytes. The immune response was so strong that correlation with the number of metastases was not feasible because the majority of the mice did not present countable metastases after challenge with B16 (7 of 10 mice had no metastases). T lymphocytes stimulated with the TRP-2_180–188 peptide in vitro also recognized the wild-type melanoma. Nevertheless, it must be noted that prophylactic vaccination with the xenogeneic form of the antigen, although valuable for several experimental mouse tumor antigens, would be difficult to implement and interpret in a clinical setting.

The second finding involved formulation of a clinically applicable immunogen (chimeric protein between an immunogenic protein and mouse TRP-2 expressed in rAd) that was shown to have some protective effect on tumor challenge, but with a thwarted immune response. TRP-2–specific T lymphocytes, which proliferated after in vitro stimulation, efficiently recognized the immunodominant peptide, but not the B16 melanoma, which displays a low number of K^b-peptide complexes on the surface due to down-regulation of class I H-2 molecules (21) . This finding suggests that T lymphocytes with low avidity TCR were the main effectors elicited by these vaccines. The percentage [and the absolute number (data not shown)] of TRP-2-TET⁺ lymphocytes in peptide-stimulated cultures correlated directly with the antimetastatic activity of the vaccine. Moreover, rAd-EGFP-mTRP-2 vaccination was successful in eliciting effector lymphocytes detected by an ELISPOT assay for IFN-, and the number of effector lymphocytes also correlated with the prophylactic efficacy (data not shown).

The third finding involved the model most similar to the clinical setting. Therapy of established tumors required a strong vaccine formulation, and yet only about half of the treated mice completely rejected the tumor. Even with this small tumor burden, therapy appeared to be a stochastic event, as in human melanoma patients. All mice, in fact, developed an easily detectable immune response against TRP-2, but the breadth of the response did not allow us to distinguish tumor progressors from regressors. Qualitative rather than quantitative differences were thus suspected. Individual differences in the orientation of the CTL response to a tumor antigen were previously explained by the stochastic timing of recruitment of different epitope-specific T cells, a sort of "first come, first served" hypothesis (22) . Indeed, it has been elegantly proven that T cells that encounter the antigen at early time points can account for a significant part of the specific response, even though they are not the most frequent in the preimmune repertoire (23) . Our results might reflect a scenario in which only those mice that present an in vivo expansion of a selected population of T cells bearing particular TCR AV chains are able to reject the preexisting tumor. The properties and dynamics of these "fittest" T cells are currently not known, although we can speculate that lymphocytes possessing the AV5 chain (together with a few other AV clonotypes) might include high avidity TRP-2–specific T cells, whose prototype is represented by clone 24.

Combining the sorting of TRP-2–specific CD8⁺ T cells and quantitative PCR-based T-cell repertoire analysis greatly improves the accuracy in detecting T-cell clones that could not otherwise be detected by using functional assays, semiquantitative TCR analysis, or tetramer sorting alone (19) . Functional assays based on the estimation of the overall immune reactivity against the melanoma antigen could not be sufficiently predictive in therapeutic vaccination because they reflect an oligoclonal expansion that might or might not include the therapeutic CTL clones. In a prophylactic setting, on the other hand, this oligoclonal response might be sufficient to control the growth of the limited number of B16 melanoma cells inoculated in mice regardless of the clonal composition of the TRP-2–responsive population.

Preferential AV usage in tumor regressors was not entirely surprising because antigen recognition by CTLs was shown to require a specific -chain pairing with a variety of TCR ß-chains (24) , suggesting a biased TCR AV usage in peptide recognition that has been confirmed by analysis of TCR-MHC-peptide complex crystals (25 , 26) . Moreover, a restricted TCR- repertoire has been described in CTLs recognizing the Melan-A/MART-1 melanoma antigen in HLA A2 context (27, 28, 29) , although in these studies, different CDR3 rearrangements were found in the presence of the same AV gene usage. In one report, Melan-A–specific T cells isolated from melanoma patients were found to have a frequent usage of the AV 2.1 chain but a large BV chain repertoire (29) . This preferential usage is not related to an antigen-driven narrowing of the TCR affinities or peripheral homeostatic expansion of selected clones in tumor-bearing hosts but rather reflects a constraint already present in the preimmune repertoire. Our data are apparently discrepant; however, some important differences need to be highlighted. We analyzed the TCR repertoire on a T-cell population able to bind TRP-2 tetramers. AV preferential usage was found in animals that regressed the tumor, thus it is possible that we preferentially selected the lymphocytes that recognize TRP-2 with higher efficiency. Moreover, the Melan-A/MART-1 antigenic system is unique in that a sizeable pool of naïve Melan-A/MART-1–specific CD8 T cells is generated during thymic selection (30 , 31) .

Although studies with melanoma patients failed to reveal a correlation between AV 2.1 usage and avidity of antigen recognition, some CDR3 public or homologous sequences within the AV 2.1-AJ 35 rearrangements were more frequently found in CTLs derived from different donors that recognized the tumor with high avidity (29) . Recurrent or homologous AV sequences appeared also to pair preferentially with BV 14, suggesting that additional factors such as the specific CDR3 loop or the pairing with some BV chains could influence the overall avidity. In this regard, the mouse AV5 chain with a conserved CDR3 region described in this article was found in at least four clones isolated from the same bulk culture of mice immunized with pcDNA3-TRP-2: paired with BV7 in clones CTL24 and CTL20 and paired with BV8.2 in clones CTL7 and CTL8. As shown in Fig. 5 , these CTL clones possessed different avidities toward TRP-2-K^b complexes, thus confirming the relevance of the -chain to guide antigen recognition and the requirement for - and ß-chain pairs to shape the strength of interaction with the antigen-MHC complex.

Our data strongly support the concept that the presence of specific T-cell clonotypes is a requirement in breaking peripheral tolerance and mounting a therapeutic immune response in tumor-bearing hosts toward a tumor-associated antigen such as TRP-2. Additional studies are needed to investigate whether an efficient expansion of the protective T-cell clonotype requires a preimmune bias in the T-cell repertoire of single animals, as proposed in human studies (28 , 29 , 31) , or is due to a stochastic usage of unselected repertoire. However, the possibility of identifying a close correlation between a particular TCR usage or a given T-cell clonotype and the efficacy of the immune response against a tumor antigen may open new scenarios in the immunotherapy of tumors.

	ACKNOWLEDGMENTS

 
The authors would like to thank Susanna Mandruzzato and Jack Gorski for helpful discussions and critical reading of the manuscript, Pierantonio Gallo for assistance with graphics, Vito Barbieri for technical assistance in mouse studies, and Lisa Smith for the editing.

	FOOTNOTES

 
Grant support: Fondo per gli Investimenti della Ricerca di Base (FIRB)-Ministero Italiano Universitá e Ricerca (MIUR) (Contract RBNEO17B4C), Italian Association for Cancer Reseach, MIUR-Consiglio Nazionale delle Ricerche Progetto Strategico Oncologia, and the Italian Ministry of Health (Ricerca Finalizzata). I. Marigo and P. Serafini are supported by a fellowship from the Italian Foundation for Cancer Research.

The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

Note: Supplementary data for this article can be found at Cancer Research Online (http://cancerres.aacrjournals.org). P. Serafini is currently at Johns Hopkins University, Baltimore, Maryland.

Requests for reprints: Vincenzo Bronte, Department of Oncology and Surgical Science, Oncology Section, Via Gattamelata 64, 35128 Padua, Italy. Phone: 39-049-8215897; Fax: 39-049-8072854; E-mail: enzo.bronte{at}unipd.it

Received 1/ 9/04. Revised 7/29/04. Accepted 8/24/04.

	REFERENCES

Top ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 

1. Bloom MB, Perry-Lalley D, Robbins PF, et al Identification of tyrosinase-related protein 2 as a tumor rejection antigen for the B16 melanoma. J Exp Med 1997;185:453-9.[Abstract/Free Full Text]
2. van Elsas A, Sutmuller RP, Hurwitz AA, et al Elucidating the autoimmune and antitumor effector mechanisms of a treatment based on cytotoxic T lymphocyte antigen-4 blockade in combination with a B16 melanoma vaccine: comparison of prophylaxis and therapy. J Exp Med 2001;194:481-9.[Abstract/Free Full Text]
3. Bowne WB, Srinivasan R, Wolchok JD, et al Coupling and uncoupling of tumor immunity and autoimmunity. J Exp Med 1999;190:1717-22.[Abstract/Free Full Text]
4. Parkhurst MR, Fitzgerald EB, Southwood S, et al Identification of a shared HLA-A*0201-restricted T-cell epitope from the melanoma antigen tyrosinase-related protein 2 (TRP2). Cancer Res 1998;58:4895-901.[Abstract/Free Full Text]
5. Tuting T, Gambotto A, DeLeo A, et al Induction of tumor antigen-specific immunity using plasmid DNA immunization in mice. Cancer Gene Ther 1999;6:73-80.[CrossRef][Medline]
6. Steitz J, Bruck J, Steinbrink K, et al Genetic immunization of mice with human tyrosinase-related protein 2: implications for the immunotherapy of melanoma. Int J Cancer 2000;86:89-94.[CrossRef][Medline]
7. Steitz J, Bruck J, Gambotto A, Knop J, Tuting T Genetic immunization with a melanocytic self-antigen linked to foreign helper sequences breaks tolerance and induces autoimmunity and tumor immunity. Gene Ther 2002;9:208-13.[CrossRef][Medline]
8. Bronte V, Apolloni E, Ronca R, et al Genetic vaccination with "self" tyrosinase-related protein 2 causes melanoma eradication but not vitiligo. Cancer Res 2000;60:253-8.[Abstract/Free Full Text]
9. Mendiratta KS, Thai G, Elashi NK, et al Therapeutic tumor immunity induced by polyimmunization with melanoma antigens gp100 and TRP-2. Cancer Res 2001;61:859-63.[Abstract/Free Full Text]
10. Engelhard VH, Bullock TN, Colella TA, Sheasley SL, Mullins DW Antigens derived from melanocyte differentiation proteins: self-tolerance, autoimmunity, and use for cancer immunotherapy. Immunol Rev 2002;188:136-46.[CrossRef][Medline]
11. Parmiani G, Castelli C, Dalerba P, et al Cancer immunotherapy with peptide-based vaccines: what have we achieved? Where are we going?. J Natl Cancer Inst (Bethesda) 2002;94:805-18.[Abstract/Free Full Text]
12. Keilholz U, Weber J, Finke JH, et al Immunologic monitoring of cancer vaccine therapy: results of a workshop sponsored by the Society for Biological Therapy. J Immunother 2002;25:97-138.
13. Overwijk WW, Tsung A, Irvine KR, et al gp100/pmel 17 is a murine tumor rejection antigen: induction of "self"-reactive, tumoricidal T cells using high-affinity, altered peptide ligand. J Exp Med 1998;188:277-86.[Abstract/Free Full Text]
14. Bronte V, Cingarlini S, Apolloni E, et al Effective genetic vaccination with a widely shared endogenous retroviral tumor antigen requires CD40 stimulation during tumor rejection phase. J Immunol 2003;171:6396-405.[Abstract/Free Full Text]
15. De Palma R, Gorski J Restricted and conserved T-cell repertoires involved in allorecognition of class II major histocompatibility complex. Proc Natl Acad Sci USA 1995;92:8836-40.[Abstract/Free Full Text]
16. Yassai M, Ammon K, Goverman J, et al A molecular marker for thymocyte-positive selection: selection of CD4 single-positive thymocytes with shorter TCRB CDR3 during T cell development. J Immunol 2002;168:3801-7.[Abstract/Free Full Text]
17. Bacsi S, De Palma R, Visentin GP, Gorski J, Aster RH Complexes of heparin and platelet factor 4 specifically stimulate T cells from patients with heparin-induced thrombocytopenia/thrombosis. Blood 1999;94:208-15.[Abstract/Free Full Text]
18. Pannetier C, Even J, Kourilsky P T-cell repertoire diversity and clonal expansions in normal and clinical samples. Immunol Today 1995;16:176-81.[CrossRef][Medline]
19. Lim A, Baron V, Ferradini L, et al Combination of MHC-peptide multimer-based T cell sorting with the immunoscope permits sensitive ex vivo quantitation and follow-up of human CD8+ T cell immune responses. J Immunol Methods 2002;261:177-94.[CrossRef][Medline]
20. Baron V, Bouneaud C, Cumano A, et al The repertoires of circulating human CD8⁺ central and effector memory T cell subsets are largely distinct. Immunity 2003;18:193-204.[CrossRef][Medline]
21. Seliger B, Wollscheid U, Momburg F, Blankenstein T, Huber C Characterization of the major histocompatibility complex class I deficiencies in B16 melanoma cells. Cancer Res 2001;61:1095-9.[Abstract/Free Full Text]
22. Brichard VG, Warnier G, Van Pel A, et al Individual differences in the orientation of the cytolytic T cell response against mouse tumor P815. Eur J Immunol 1995;25:664-71.[Medline]
23. Bousso P, Levraud JP, Kourilsky P, Abastado JP The composition of a primary T cell response is largely determined by the timing of recruitment of individual T cell clones. J Exp Med 1999;189:1591-600.[Abstract/Free Full Text]
24. Yokosuka T, Takase K, Suzuki M, Nakagawa Y, et al Predominant role of T cell receptor (TCR)-alpha chain in forming preimmune TCR repertoire revealed by clonal TCR reconstitution system. J Exp Med 2002;195:991-1001.[Abstract/Free Full Text]
25. Garcia KC, Degano M, Pease LR, et al Structural basis of plasticity in T cell receptor recognition of a self peptide-MHC antigen. Science (Wash DC) 1998;279:1166-72.[Abstract/Free Full Text]
26. Ding YH, Baker BM, Garboczi DN, Biddison WE, Wiley DC Four A6-TCR/peptide/HLA-A2 structures that generate very different T cell signals are nearly identical. Immunity 1999;11:45-56.[CrossRef][Medline]
27. Trautmann L, Labarriere N, Jotereau F, et al Dominant TCR V alpha usage by virus and tumor-reactive T cells with wide affinity ranges for their specific antigens. Eur J Immunol 2002;32:3181-90.[CrossRef][Medline]
28. Mantovani S, Palermo B, Garbelli S, et al Dominant TCR-alpha requirements for a self antigen recognition in humans. J Immunol 2002;169:6253-60.[Abstract/Free Full Text]
29. Dietrich PY, Le Gal FA, Dutoit V, et al Prevalent role of TCR alpha-chain in the selection of the preimmune repertoire specific for a human tumor-associated self-antigen. J Immunol 2003;170:5103-9.[Abstract/Free Full Text]
30. Pittet MJ, Zippelius A, Valmori D, et al Melan-A/MART-1-specific CD8 T cells: from thymus to tumor. Trends Immunol 2002;23:325-8.[CrossRef][Medline]
31. Dutoit V, Rubio-Godoy V, Pittet MJ, et al Degeneracy of antigen recognition as the molecular basis for the high frequency of naive A2/Melan-a peptide multimer⁺ CD8⁺ T cells in humans. J Exp Med 2002;196:207-16.[Abstract/Free Full Text]

This article has been cited by other articles:

				J. N. Kochenderfer and R. E. Gress A Comparison and Critical Analysis of Preclinical Anticancer Vaccination Strategies Experimental Biology and Medicine, October 1, 2007; 232(9): 1130 - 1141. [Abstract] [Full Text] [PDF]

				J. N. Kochenderfer, C. D. Chien, J. L. Simpson, and R. E. Gress Synergism between CpG-Containing Oligodeoxynucleotides and IL-2 Causes Dramatic Enhancement of Vaccine-Elicited CD8+ T Cell Responses J. Immunol., December 15, 2006; 177(12): 8860 - 8873. [Abstract] [Full Text] [PDF]

				R. De Palma, F. Del Galdo, G. Abbate, M. Chiariello, R. Calabro, L. Forte, G. Cimmino, M. F. Papa, M. G. Russo, G. Ambrosio, et al. Patients With Acute Coronary Syndrome Show Oligoclonal T-Cell Recruitment Within Unstable Plaque: Evidence for a Local, Intracoronary Immunologic Mechanism Circulation, February 7, 2006; 113(5): 640 - 646. [Abstract] [Full Text] [PDF]

This Article Abstract Full Text (PDF) Supplementary Data Alert me when this article is cited Alert me if a correction is posted Services Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire