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IMMUNOBIOLOGY
From the Department of Surgery and Department of
Molecular Genetics and Biochemistry, University of Pittsburgh Medical
Center, Pittsburgh, PA.
Immunotherapy trials targeting the induction of
tumor-reactive T-cell responses in cancer patients appear to hold
significant promise. Because nonmutated lineage-specific antigens and
mutated idiotypic antigens may be coexpressed by tumor cells, the use of autologous tumor material to promote the broadest range of antitumor
T-cell specificities has significant clinical potential in cancer
vaccination trials. As a model for vaccination in the cancer setting,
we chose to analyze the promotion of T-cell responses against
Epstein-Barr virus (EBV)-transformed B-lymphoblastoid cell line
(B-LCL)-derived antigens in vitro. A series of bulk antigenic formats
(freeze-thaw lysate, trifluoroacetic acid lysate, extracted membranes,
affinity-purified MHC class I- and class II-presented peptides,
acid-eluted peptides) prepared from EBV B-LCLs were tested for their
ability to stimulate EBV B-LCL-reactive CD4+ and
CD8+ T lymphocytes in vitro when pulsed onto autologous
dendritic cells (DCs). DC presentation of freeze-thaw lysate material
derived from (either autologous or allogeneic) EBV B-LCLs with an Mr of 10 kd or larger stimulated optimal anti-EBV B-LCL responsiveness from
freshly isolated CD4+ and CD8+ peripheral blood
T cells. These in vivo "memory" T-cell responses were observed only
in EBV-seropositive donors. CD4+ T-cell responses to
lysate-pulsed DCs were Th1 type (ie, strong interferon- Effective vaccines designed to treat cancer or
alternate malignancies should elicit both CD4+ and
CD8+ T-cell responses to epitopes derived from tumor- or
pathogen-associated antigens.1 This may be most
effectively accomplished by accessing or implementing autologous
dendritic cells (DCs) in the design of the vaccine. DCs have been shown
to efficiently stimulate both primary and secondary CD4+
and CD8+ T-cell immune responses and are therefore
considered to represent potent biologic adjuvants for application to
vaccination trials.2 After so-called immature DCs capture
and process antigens in the periphery, they migrate to lymphoid organs.
Terminally differentiated, or "mature," DCs stimulate
antigen-specific T cells via the presentation of peptide antigens in
association with HLA class I and II molecules, the provision of T-cell
costimulation, and the secretion of T-cell growth and differentiation
cytokines. DC maturation may be induced by a number of stimuli,
including pathogens, cognate T-cell interaction, or proinflammatory
cytokines.3
Immature DCs efficiently acquire and process exogenous antigens (such
as those extracted from tumor or transformed cells) and can be easily
matured into optimal T-cell stimulatory antigen-presenting cells.4,5 Given these characteristics, we have evaluated the ability of this induction system (DCs plus "tumor" extracts) to
promote "tumor"-specific CD4+ and CD8+
T-cell immune responses in vitro using Epstein-Barr virus
(EBV)-transformed B-lymphoblastoid cell line (B-LCL) as a model
"tumor." The results of this EBV B-LCL model system allow for the
construction of vaccines for the treatment or prevention of
cancer or alternate malignancies, such as the EBV-associated
malignancies posttransplantation lymphoproliferative disorder (PTLD),
Burkitt lymphoma, Hodgkin lymphoma, and undifferentiated nasopharyngeal carcinoma.
Donors and cell lines
LCLs were established by EBV (B95.8 strain) transformation of
peripheral blood mononuclear cells (PBMCs) in the presence of 0.1 µg/mL cyclosporine (Sandoz, Basel, Switzerland). Anti-µ B-cell blasts were generated by stimulating PBMCs with 10 µg/mL rabbit antihuman IgM immunobeads (Irvine Scientific, Santa Ana, CA) in the
presence of 100 U/mL recombinant human interleukin-4 (rhIL-4; Schering-Plough, Kenilworth, NJ). Phytohemagglutinin (PHA)-activated T-cell blasts were prepared by stimulating PBMCs with 5 µg/mL PHA
(Sigma, St. Louis, MO). Cell lines were maintained in RPMI 1640 supplemented with 10% heat-inactivated fetal calf serum (FCS), 2 mmol/L L-glutamine, 100 IU/mL penicillin, 100 µg/mL streptomycin, and
1 mmol/L sodium pyruvate. All cell culture reagents were
purchased from Life Technologies (Gaithersburg, MD).
Antigen-presenting cells
Bulk antigenic formats Autologous LCL cells, B-, or T-cell blasts were expanded in RPMI/10% FCS, washed, and subsequently recultured for an additional 3 days in AIM-V to remove calf serum proteins and to reduce the number of FCS-derived HLA-presented epitopes on the cell surface. At the time of cell harvest, cells (109 each) were washed twice with HBSS prior to extraction of cell-associated antigens using the procedures indicated below.Freeze-thaw lysate Cells were resuspended in 2 mL of HBSS and lysed by 5 freeze (on methanol and dry ice)-thaw (room temperature) cycles. Total cell disruption was microscopically validated using trypan blue staining. After sonication for 10 minutes, lysate was centrifuged at 15 000g (30 minutes, 4°C). Supernatant (SN; without top lipid layer) was recovered and fractionated on Centricon-10 ultrafiltration devices (Amicon, Cambridge, MA) by centrifugation at 3000 rpm for 2 to 3 hours at 4°C. Upper (10-kd proteins or larger) and lower (smaller than 10-kd proteins/peptides) fractions were individually harvested and stored at 70°C until use.
Trifluoroacetic acid lysates Cells were resuspended in trifluoroacetic acid (TFA) 0.1% or 1% in distilled, deionized water (ddH2O) and dounce homogenized until qualitative cell disruption had occurred (typically 150-200 cycles). The resulting lysate was sonicated for 10 minutes, followed by centrifugation at 15 000g over 30 minutes at 4°C. SN (without top lipid layer) was removed and placed on Centricon-10 ultrafiltration devices as outlined above. After centrifugation at 3000 rpm for 2 to 3 hours at 4°C, top and bottom fractions were recovered, lyophilized in a Labconco Speed-Vac until near dryness, and resuspended in 1 mL phosphate-buffered saline (PBS)/10% dimethyl sulfoxide (DMSO). Lysate was stored at70°C
until use.
Extraction of cell membranes Pelleted membranes resulting from centrifugation of TFA 1% lysates were extracted using 1% TFA in 90% acetonitrile (ACN)/9% ddH2O overnight at 4°C following an additional centrifugation at 15 000g at 4°C over 30 minutes. The SN was recovered, lyophilized to remove organic solvent, and resuspended in 1 mL PBS/10% DMSO. Extract was stored at70°C
until use.
Extraction of naturally processed peptides from viable cells Cells were incubated with 50 mL citrate-phosphate buffer, pH 3.0,6 for 1 minute following centrifugation over 3 minutes at 2000 rpm. To remove remaining cell fragments, the SN was spun down at 4000 rpm over 10 minutes (both at 4°C). Cell-free SN containing eluted peptides was concentrated on a SepPak C18 cartridge (Millipore, Bedford, MA) according to the manufacturer's instructions. Bound peptides were eluted by 60% (vol/vol) followed by 100% (vol/vol) acetonitrile (in ddH2O) and concentrated in a Speed-Vac. They were resuspended in 1 mL PBS/10% DMSO and stored at70°C until use.
Extraction of naturally processed peptides from affinity-purified HLA-A2.1 and HLA-DR molecules Pellets from 1.5 × 109 LCL cells were lysed in 20 mL Chaps detergent (Sigma, 5% in ddH2O) containing protease inhibitors (Boehringer Mannheim, Mannheim, Germany) for 45 minutes on ice. After centrifugation at 2000 rpm for 10 minutes, followed by 15 000g for 30 minutes (both at 4°C), SN was passed through chromatography columns filled with either Sepharose beads coupled with monoclonal antibodies (mAbs) BB7.2 (anti-HLA-A2.1) or L243 (anti-HLA-DR monomorphic). Antibodies were coupled to Sepharose-4B matrix (Sigma) per the manufacturer's instructions. Matrices were then treated with 0.1% TFA (in ddH2O) for 15 minutes at room temperature to denature the major histocompatibility complex (MHC) peptide complexes, allowing for the harvest of soluble peptides. After initial centrifugation to pellet the Sepharose beads (3000 rpm, 10 minutes), SN was recovered and fractionated on Centricon-3 ultrafiltration devices over 2 to 3 hours at 4°C. Top (3 kd or larger) and bottom (smaller than 3 kd) fractions were lyophilized and resuspended in 1 mL PBS/10% DMSO and then stored at70°C
until use.
Flow cytometry For immunophenotyping, DC or T-cell responders were washed in HBSS supplemented with 1% bovine serum albumin and 0.1% NaN3 and incubated (30 minutes at 4°C) with one of the following antibodies: fluorescein isothiocyanate (FITC)-conjugated anti-HLA class I (Serotec, Oxford, England), phycoerythrin (PE)-conjugated anti-HLA-DR (Becton Dickinson, Mountain View, CA), FITC-conjugated anti-CD8 (Becton Dickinson), PE-conjugated anti-CD54 (Becton Dickinson), FITC-conjugated anti-CD80 (Ancell, Bayport, MN), PE-conjugated anti-CD83 (Coulter-Immunotech, Miami, FL), and FITC-conjugated anti-CD86 (PharMingen, San Diego, CA). Unconjugated anti-CD45RO and anti-CD45RA mAbs were obtained from the Sixth International Leukocyte Typing Workshop and were used in indirect immunofluorescence assays. Cells were also stained with corresponding isotype-matched control mAb (PharMingen). For indirect staining, FITC-conjugated goat antimouse IgG F(ab)2 antibody (Becton Dickinson) was used (30 minutes, 4°C). Surface expression was analyzed using a FACScan flow cytometer (Becton Dickinson) and Lysis II software. Data were collected on 10 000 viable cells.T-cell cultures CD4+ and CD8+ T lymphocytes were positively isolated from PBMCs by immunomagnetic CD4/CD8 MicroBeads and were seeded at 3 × 106 cells per well in 24-well plates (Costar). Autologous irradiated DCs (105 per well) prepulsed with a freeze-thaw lysate (10 kd or larger) of LCLs, B- or T-cell blasts (for loading, see above), or intact autologous irradiated LCL cells (7.5 × 104 per well) were then added. Radiation dose was 2500 rad for DCs and 4000 rad for LCLs. Culture medium was AIM-V supplemented with 5% human AB serum (Sigma) at a final volume of 2 mL/well. For cultures containing CD8+ T cells, 1000 U/mL rhIL-6 (Sandoz) and 1 ng/mL rhIL-12 (Genetics Institute, Bedford, MA) were added on day 0.7 Cultures containing CD4+ T cells were supplemented on day 3 with 10 IU/mL rhIL-2 (Chiron, Emeryville, CA). Responding T cells were restimulated on day 7 and day 14 using irradiated, antigen-pulsed DCs or irradiated LCL cells at a responder-to-stimulator ratio of 30:1 (DC) or 40:1 (LCL) in AIM-V medium containing 10 IU/mL IL-2 and 5 ng/mL rhIL-7 (Genzyme).Elispot assays for interferon-  (1-D1K; Mabtech, Stockholm, Sweden) or antihuman IL-5
(18051D; PharMingen) and detection biotinylated mAbs antihuman IFN-
(7-B6-1; Mabtech) or antihuman IL-5 (18522D; PharMingen). Nonirradiated
autologous monocytes (4 × 104 per well), immature or
mature DCs (2 × 104 per well) prepulsed with bulk
antigenic formats (for loading, see above), or autologous LCL cells
(5 × 104 per well, not irradiated) were used as
stimulator cells. CD4+ and CD8+ T-cell
responders were positively isolated from PBMCs by immunomagnetic CD4/CD8 MicroBeads and were more than 95% pure. Control wells contained unstimulated T cells, T cells in the presence of unloaded APC, and LCL cells alone. Spot numbers were automatically determined with the use of a computer-assisted video image analyzer
(Zeiss-Kontron, Jena, Germany).9 To calculate the number
of T cells responding to a particular antigen, the mean numbers of
spots induced by DCs alone were subtracted from mean spot numbers
induced by antigen-loaded DCs. For statistical evaluation, a
t test for unpaired samples was used. Values of P < .05 were considered significant.
Cytotoxicity assays CD8+ responder populations were tested for their cytolytic activity after 2 weekly (days 7, 14) restimulations on days 23 to 25 against LCLs, PHA blasts, and the natural killer target K562 in a standard 6-hour 51Cr release assay.6 In some assays, natural killer activity was blocked by the addition of 40 000 nonlabeled K562 per well. Blocking antibodies W6/32 (anti-HLA class I) and L243 (anti-HLA-DR, class II) were added at 20 µg/well.
Subcellular fractions of EBV B-LCLs contain immunogenic antigens In IFN- Elispot analyses, we generally observed that autologous
EBV B-LCLs induced strong spot production when admixed with purified
blood-derived T cells obtained from EBV-seropositive, healthy
individuals. In donor IP1, for example, the frequencies of LCL-reactive
T lymphocytes were 203 per 105 for CD4+ T cells
and 845 per 105 for CD8+ T cells (data not
shown), suggesting that the autologous EBV B-LCLs express immunogenic
HLA class I and class II complexes presenting viral epitopes recognized
by donor T cells.
For the purposes of DC-based vaccine construction, we sought to
determine those extracts that might be obtained from a given target
cell (ie, tumor, EBV B-LCL) to effectively promote CD4+ and
CD8+ T-cell reactivity against target antigens. In our
model system, we prepared lysates from 109 EBV B-LCL cells
of donor IP1 (IP1-LCL) by freeze-thaw cycles or mechanical disruption
in 0.1% or 1% TFA, with a subsequent fractionation of extracted
proteins/peptides into material with Mr smaller than 10 kd or Mr 10 kd
or larger performed using ultrafiltration devices. In addition to
lysates, naturally processed peptides were isolated from viable IP1-LCL
cells or from HLA-A2.1 and HLA-DR complexes affinity-purified from
IP1-LCL by acid-denaturation. Eluted peptides were divided into small
and large peptides (ie, those with Mr smaller than 3 kd or Mr 3 kd or
larger) using 3-kd ultrafiltration devices. These EBV B-LCL-derived
bulk antigenic proteins/peptides were then loaded on autologous
immature, endocytic DCs and were screened for recognition by purified
CD4+ and CD8+ "memory" T cells freshly
isolated from the blood of donor IP1 using IFN-
Mature DCs loaded with LCL-derived freeze-thaw lysates stimulate both CD4+ and CD8+ T-cell responses to EBV B-LCL antigens We compared autologous monocytes with immature and mature DCs for their ability to induce IFN- spot production by purified CD4+ and CD8+ T lymphocytes after being pulsed
with freeze-thaw lysates (10 kd or larger) from autologous EBV B-LCLs
or B-cell or T-cell blasts. As shown in Figure
3, mature DCs were the only APC capable
of stimulating both CD4+ and CD8+ T cells
reactive against epitopes derived from autologous EBV B-LCL
freeze-thaw lysates. Of note, mature DCs that were prepulsed with EBV
B-LCL lysates at the time when maturation was initiated (ie, mature
DC-I) exhibited stronger T-cell stimulatory capacity than DCs that were
loaded with EBV B-LCL lysates after DC maturation (ie, mature DC-II)
was already achieved. Accordingly, for all subsequent experiments
involving mature DCs, day 6 autologous immature DCs were first fed with
freeze-thaw lysates (10 kd or larger) and then matured in vitro for 2 days using TNF- , IL-1 , IL-6, and PGE2. In the control
groups evaluated, autologous monocytes pulsed with EBV B-LCL lysates
were less efficient in inducing significant IFN- spot production in
donors' T cells, and T-cell responsiveness to lysates prepared from
autologous B- or T-cell blasts was not observed. Interestingly,
CD4+ and CD8+ T cells isolated from both donors
displayed cross-reactivity against autologous mature DCs pulsed with
allogeneic EBV B-LCL lysates, whereas they did not recognize lysates
prepared from the corresponding matched allogeneic B-cell or T-cell
blasts pulsed onto autologous DCs (Figure
4).
To further confirm the specificity of the T-cell response to allogeneic
EBV B-LCL lysates obtained in donors IP1 and IP2 (Figure 4) and in
several other healthy EBV carriers evaluated (results not shown), we
performed IFN- We next investigated how effectively repeated in vitro stimulations of
CD4+ and CD8+ T cells with EBV B-LCL
lysate-pulsed mature DCs were able to generate effector T lymphocytes
exhibiting reactivity against EBV B-LCL target cells. CD4+
T cells purified from donor IP1 were stimulated weekly with autologous mature DCs preloaded with freeze-thaw lysates (10 kd or larger) derived from autologous EBV B-LCLs or T-cell blasts. In parallel, T
cells were also stimulated on a weekly basis with the autologous EBV
B-LCL. Compared with freshly isolated CD4+ T cells of donor
IP1, day 21-cultured CD4+ responder lymphocytes induced
with autologous DCs and lysate prepared from the autologous EBV B-LCL
showed a 6- to 13-fold increase in the frequency of T cells recognizing
autologous EBV B-LCL cells or EBV B-LCL lysate-pulsed DCs as determined
by IFN-
CD8+ T cells were stimulated weekly with autologous intact
EBV B-LCL cells or with autologous mature DCs preloaded with
freeze-thaw lysates (10 kd or larger) prepared from autologous EBV
B-LCL, autologous T-cell blasts, or allogenic EBV-B LCL. Responder
lymphocytes generated in this way were predominantly
CD45RO+ as assessed by flow cytometry, indicating the
expansion of "memory" CD8+ T lymphocytes. When we
tested the cytolytic activity of day 23-cultured T-cell responders,
maximum reactivity was observed against the autologous EBV B-LCL if
T-cell cultures were stimulated with intact EBV B-LCL cells (Figure
6). Lower, but still significant, levels of lysis against autologous EBV B-LCL cells were obtained if responder lymphocytes were instead induced with autologous mature DCs preloaded with freeze-thaw lysates prepared from either autologous or allogenic EBV B-LCLs (Figures 6 and 7). In contrast, responder T cells stimulated with autologous mature DCs prepulsed with the freeze-thaw lysate derived from autologous T-cell blasts did not recognize autologous EBV
B-LCL cells (Figure 6). Further, cytolytic activity against autologous
T-cell blasts was not observed in any of the responder lymphocyte
populations tested.
CD8+ T cells stimulated by autologous DCs pulsed with either auto- or allo-EBV B-LCL freeze-thaw lysates killed in a class I-restricted manner (Figure 7) and recognized autologous EBV B-LCL targets but not completely HLA-mismatched allogeneic EBV B-LCL (Figure 7). The inability of cytotoxic T lymphocytes (CTL) induced by autologous DCs plus allogeneic EBV B-LCL lysates to recognize the EBV B-LCL from which the lysate was derived (Figure 7B) argues strongly against the induction of allospecific CTL using this in vitro induction protocol.
Among bulk antigenic formats prepared from autologous EBV B-LCLs, freeze-thaw lysates were clearly the most efficient in stimulating CD4+ T lymphocytes when processed and presented by autologous DCs (Figure 1). The superior immunogenicity of freeze-thaw lysates is not intuitively obvious but may reflect differential antigen extraction efficiency, differential retention of immunogenic proteins in freeze-thaw lysates, differential uptake of freeze-thaw antigens by DCs, or the differential presence of DC activators in freeze-thaw lysates5,10 among other reasons. The fact that lysates obtained from identically grown B- or T-cell
blasts were not recognized by CD4+ T cells argues against
reactivity directed towards epitopes derived from autoantigens or FCS
proteins (Figures 2-5). Furthermore, freshly isolated T-cell responses
directed against EBV B-LCL-derived material was only observed in
EBV-seropositive donors, supporting the anti-EBV "specificity" of
these "memory" T-cell reactivities. Immune reactivity against EBV
B-LCL lysates was primarily Th1 type because most responder T cells
secreted IFN- Interestingly, T cells isolated from EBV-seropositive donors responded to autologous DCs pulsed with freeze-thaw lysates prepared from either autologous or allogeneic EBV B-LCLs but not DCs loaded with lysates derived from the corresponding B- or T-cell blasts (Figure 4). We confirmed this finding in several other healthy individuals previously infected with EBV (data not shown). The fact that "memory" T-cell reactivity against allogeneic EBV B-LCL lysates was only observed in anti-EBV-positive individuals (and not in donors seronegative for EBV; data not shown) provides further evidence that T cells responding to EBV B-LCL lysate-loaded DCs recognize EBV-related antigens. In addition, these results suggest that EBV B-LCL lysates, irrespective of the donor from which they were derived, contain "shared" antigens that can yield epitopes that are "cross-presented" by DCs and recognized by CD4+ and CD8+ T cells. This phenomenon might be explained by the general observation that reactivity against lysates was exclusively found in lysate fractions containing molecules larger than 10 kd (Figure 1). Naturally processed and presented HLA-binding oligopeptides are expected to be smaller than 10 kd, whereas the EBV B-LCL lysate fractions 10 kd and larger obviously contain large "shared" EBV proteins that after appropriate processing and presentation by autologous, mature DCs are recognized by the individual T-cell systems. The finding that EBV B-LCL lysates can stimulate LCL-specific CD8+ T-cell responses is in agreement with earlier studies by others demonstrating that MHC class I presentation of exogenous, soluble antigens can be achieved by professional APC both in vitro and in vivo but requires high concentrations of antigens.11-15 This has also recently been documented for alternate "antigens" such as nonreplicating microbes16 and apoptotic or infected cells,17 in which DCs were observed to process and present epitopes in MHC class I complexes that are derived from these endocytosed organisms that conceptually have limited access to the DC cytosol. Of note, by processing dying cells, DCs were even able to "cross-prime" T cells exhibiting specificity for "shared" viral antigens.17 In general, the use of tumor freeze-thaw lysates as a source of antigen for pulsing autologous DCs appears to represent an attractive approach to optimally activate a broad repertoire of antigen-specific CD4+ and CD8+ T cells. This is particularly compelling for prospective clinical vaccines designed to treat cancer histologies for which well-characterized tumor antigens are limited in number or are yet to be defined. Further, this approach incorporates any idiotypic epitopes or antigens that may derive from mutational events associated with the tumorigenic process of a given individual. It has recently been reported that certain human melanoma vaccines generated from mechanical or freeze-thaw lysates can stimulate melanoma-specific T cells.18-20 There is also evidence from murine studies that DCs pulsed with whole tumor lysates mediate potent antitumor immune responses in vitro and in vivo.21,22 Indeed, our own preliminary data support the ability of this procedure to promote the expansion of CD4+ and CD8+ T cells specific for melanoma, renal cell carcinoma, or squamous cell carcinoma of the head and neck from patient peripheral blood lymphocyte responders (W.J.S., unpublished data). The use of tumor (autologous or allogeneic) lysate as an antigen source for vaccine construction circumvents the need for viable fresh tumor cells and the need to establish tumor cell lines in vitro, which may prove logistically difficult to acquire or time-consuming to produce. Because human cancers have been shown to elicit multi-epitope-specific immune responses in vivo, the approach of using tumor lysates pulsed onto DCs would offer the potential advantage of inducing a broader T-cell response to tumor-associated antigens than could be achieved by pulsing DCs with a single or with several defined synthetic tumor peptides. This strategy potentially lessens the possibility of immune escape by evolving tumors in the face of a broader, polyspecific antitumor T-cell immune response. In addition, greater potential exists for the simultaneous presentation of CTL-defined and T-helper-defined epitopes by lysate-pulsed DCs for adoptive application in clinical vaccines. This may be particularly true for mature DCs. After maturation, DCs express enhanced levels of HLA and costimulatory molecules and heightened cytokine production that may optimally activate and maintain both CD4+ and CD8+ antigen-specific T cells in vivo.3 In this regard, although several HLA class I-presented tumor-associated epitopes have been defined by human CTL,23 limited knowledge exists about the identity of CD4+ T-cell-defined tumor-associated epitopes. This represents a glaring deficiency in our knowledge base because there is clear evidence from both in vitro and in vivo studies that the successful induction of durable cellular immunity in chronic diseases (ie, viral infections or cancer) requires the activation of both antigen-specific CD4+ and antigen-specific CD8+ T cells.24,25 The use of tumor lysates as a vaccine component, however, has the potential disadvantage that this approach might induce pathologic autoimmune reactivity to normal tissue antigens as a consequence of the processing and presentation of "housekeeping" or "lineage-associated" epitopes by autologous DCs. However, our studies evaluating T-cell responsiveness to DCs loaded with EBV B-LCL lysates were unable to demonstrate responder T-cell cross-reactivity against B- or T-cell blasts. Furthermore, DCs pulsed with lysates derived from T-cell blasts were unable to promote the expansion of reactivity to "self" T-cell-associated antigens. This may reflect the comparative threshold density of a given epitope presented by MHC molecules on the surface of a tumor cell (ie, overexpressed antigens) versus normal cells.26,27 The use of this approach, applied in clinical vaccine trials, may be of significant value in the treatment of cancer or transformed cells such as EBV-associated lymphomas observed in PTLD,28,29 which is a frequent tumor in allograft recipients that develops mostly after prolonged immunosuppression. There is also evidence that EBV plays a major role in the etiology of Burkitt's lymphoma, Hodgkin's lymphoma, and undifferentiated nasopharyngeal carcinoma.30 The rationale for using EBV B-LCL lysates as a vaccine in patients suffering from EBV-associated tumors derives from the observation that at least some of the latent EBV proteins expressed in EBV B-LCL represent potential targets for viral-specific T-cell responses in EBV-positive malignancies.31,32 We observed that CD4+ and CD8+ T cells reactive against autologous EBV B-LCL cells could be coordinately generated by in vitro stimulation with mature DCs preloaded with lysates from allogenic (HLA completely mismatched) EBV B-LCL. Importantly, this anti-EBV B-LCL reactivity occurred in the absence of detectable allospecific T-cell reactivity (cytokine secretion or cytotoxicity). This encourages the potential use of a single "off-the-shelf" standard EBV B-LCL lysate preparation to be applied to DCs in generating a general vaccine for these tumor-bearing patients irrespective of their HLA type. This may prove logistically attractive in the clinical setting, where the generation of autologous EBV B-LCL for clinical application is not always attained and requires extended culture periods of 4 to 5 weeks. Overall, these observations may be extrapolated to alternative tumor histologies using either freshly resected tumor material or a reference lineage-matched tumor cell line from which to generate the lysate for clinical application.
The authors thank Drs Lisa Salvucci Kierstead, Russell Salter, and Jan Mueller-Berghaus for careful review and helpful discussion in the generation of this manuscript.
Submitted September 28, 1999; accepted May 8, 2000.
Supported by National Institutes of Health grant CA 57840 (W.J.S.), a clinical investigator award from the Cancer Research Institute (W.J.S.), CNR-NATO grant 216.1919 (L.G.), NATO collaborative research grant CRG.CRG 973153 (L.G., W.J.S.), and a fellowship from the Deutsche Forschungsgemeinschaft (He 2896/1-1; W.H.).
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: Walter J. Storkus, W1555 Biomedical Sciences Tower, University of Pittsburgh School of Medicine, 200 Lothrop St, Pittsburgh, PA 15261; e-mail: storkuswj{at}msx.upmc.edu.
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Top
Abstract
Introduction
) or CD8+ T lymphocytes (
) initially
seeded per well. Calculation of lysate-responsive T-cell frequencies
were performed as outlined in Figure 
); against autologous mature DCs preloaded
with freeze-thaw lysates (10 kd or larger) isolated from autologous
EBV B-LCL (
), B-cell blasts (
), or T-cell blasts (
). Resulting spots were developed and evaluated as
described in Figure 
), IP3
EBV B-LCL (