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一种黑色素瘤多表位多肽可诱导特异性CD8 + T细胞反应。

A melanoma multiepitope polypeptide induces specific CD8+ T-cell response.

作者信息

Levy Adva, Pitcovski Jacob, Frankenburg Shoshana, Elias Orit, Altuvia Yael, Margalit Hanna, Peretz Tamar, Golenser Jacob, Lotem Michal

机构信息

Migal, Kiryat Shmona, Israel.

出版信息

Cell Immunol. 2007 Nov-Dec;250(1-2):24-30. doi: 10.1016/j.cellimm.2008.01.001. Epub 2008 Feb 13.

Abstract

Strategies using epitope-based vaccination are being considered for melanoma immunotherapy, in an attempt to overcome failure of other modalities. In the present study, we designed and produced a multiepitope polypeptide for melanoma (MEP-mel), which contains three repeats of four antigenic epitopes (gp100: 209-217 (210M); gp100: 280-288 (288V); Mart1: 26-35 (27L); tyrosinase: 368-376 (370D). The peptides were attached to each other by linkers containing sequences recognized by the proteasome, to improve protein cleavage and antigen presentation. The results show that peptide-specific T cells produced IFN-gamma when stimulated with MEP-mel-transfected dendritic cells. The presentation of peptides by MEP-mel-transfected dendritic cells was proteasome-dependent and was more long-lasting than the presentation of exogenously delivered native peptides. When dendritic cells were loaded with MEP-mel protein, weak cross presentation was induced. The production of multiepitope molecules based on several peptides linked by sequences sensitive to proteasomal cleavage represents a promising new tool for the improvement of cancer immunotherapy.

摘要

基于表位的疫苗接种策略正被考虑用于黑色素瘤免疫治疗,试图克服其他治疗方式的失败。在本研究中,我们设计并制备了一种用于黑色素瘤的多表位多肽(MEP-mel),它包含四个抗原表位的三个重复序列(gp100:209 - 217(210M);gp100:280 - 288(288V);Mart1:26 - 35(27L);酪氨酸酶:368 - 376(370D))。这些肽通过含有蛋白酶体识别序列的接头相互连接,以改善蛋白质切割和抗原呈递。结果表明,当用MEP-mel转染的树突状细胞刺激时,肽特异性T细胞产生γ干扰素。MEP-mel转染的树突状细胞对肽的呈递是蛋白酶体依赖性的,并且比外源性递送的天然肽的呈递更持久。当树突状细胞负载MEP-mel蛋白时,诱导了较弱的交叉呈递。基于通过对蛋白酶体切割敏感的序列连接的几种肽产生多表位分子,是改善癌症免疫治疗的一种有前景的新工具。

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