Thirty-three metastatic melanoma patients were vaccinated according to a phase I-II study with an allogeneic melanoma cell line that was genetically modified by transfection with a plasmid containing the gene encoding human interleukin 2 (IL-2). The cell line expresses the major melanoma-associated antigens and the HLA class I alleles HLA-A1, -A2, -B8, and Cw7. All patients shared one or more HLA class I alleles with this cell line vaccine. Patients were immunized by three vaccinations, each consisting of 60 x 10(6) irradiated (100 Gy) melanoma cells (secreting 120 ng of IL-2/10(6) cells/24 hr) administered subcutaneously at weekly intervals for 3 consecutive weeks. Side effects of treatment consisted of swelling of locoregional lymph nodes and induration at the site of injection, i.e., a delayed-type hypersensitivity (DTH) reaction. In three patients, vaccination induced inflammatory responses in distant metastases containing necrosis or apoptosis along with T cell infiltration. Apoptosis occurred only in Bcl-2-negative areas, not in Bcl-2-expressing parts of the metastases. Two other patients experienced complete or partial regression of subcutaneous metastases. Seven patients had protracted stabilization (4 to >46 months) of soft tissue metastases, including one patient who developed vitiligo after vaccination. Immune responses to the vaccine could be detected in 67% of the 27 patients measured. Vaccination was shown to induce a variable change in the number of anti-vaccine cytotoxic T lymphocytes (CTLs) in peripheral blood, which did not correlate with response to treatment. However, in two of five patients the frequency of anti-autologous tumor CTLs measured was significantly higher than before vaccination. This study demonstrates the feasibility, safety, and therapeutic potential of vaccination of humans with allogeneic, gene-modified tumor cells, and that frequencies of vaccine-specific CTLs among patient lymphocytes can be determined by using a modified limited dilution analysis (LDA).
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页码:739 / 750
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Aarnoudse CA, 1999, INT J CANCER, V82, P442, DOI 10.1002/(SICI)1097-0215(19990730)82:3<442::AID-IJC19>3.3.CO
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ROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLANDROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLAND
BORYSIEWICZ, LK
GRAHAM, S
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ROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLANDROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLAND
GRAHAM, S
HICKLING, JK
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ROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLANDROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLAND
HICKLING, JK
MASON, PD
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ROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLANDROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLAND
MASON, PD
SISSONS, JGP
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ROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLANDROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLAND
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ROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLANDROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLAND
BORYSIEWICZ, LK
GRAHAM, S
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ROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLANDROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLAND
GRAHAM, S
HICKLING, JK
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ROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLANDROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLAND
HICKLING, JK
MASON, PD
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ROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLANDROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLAND
MASON, PD
SISSONS, JGP
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ROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLANDROYAL POSTGRAD MED SCH, DEPT MED, MRC, CLIN IMMUNOL RES GRP, LONDON W12 0HS, ENGLAND