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Induction of neoantigen-reactive T cells from healthy donors

表位 T细胞受体 生物信息学 CD8型 T细胞 抗原 细胞生物学 主要组织相容性复合体 癌症免疫疗法 链霉菌 抗原提呈细胞 细胞毒性T细胞 免疫学 免疫疗法 生物 计算生物学 免疫系统 体外 遗传学 基因
作者
Muhammad Ali,Zsófia Földvári,Eirini Giannakopoulou,Maxi-Lu Böschen,Erlend Strønen,Weiwen Yang,Mireille Toebes,Benjamin Schubert,Oliver Kohlbacher,Ton N. Schumacher,Johanna Olweus
出处
期刊:Nature Protocols [Springer Nature]
卷期号:14 (6): 1926-1943 被引量:102
标识
DOI:10.1038/s41596-019-0170-6
摘要

The identification of immunogenic neoantigens and their cognate T cells represents the most crucial and rate-limiting steps in the development of personalized cancer immunotherapies that are based on vaccination or on infusion of T cell receptor (TCR)-engineered T cells. Recent advances in deep-sequencing technologies and in silico prediction algorithms have allowed rapid identification of candidate neoepitopes. However, large-scale validation of putative neoepitopes and the isolation of reactive T cells are challenging because of the limited availablity of patient material and the low frequencies of neoepitope-specific T cells. Here we describe a standardized protocol for the induction of neoepitope-reactive T cells from healthy donor T cell repertoires, unaffected by the potentially immunosuppressive environment of the tumor-bearing host. Monocyte-derived dendritic cells (DCs) transfected with mRNA encoding candidate neoepitopes are used to prime autologous naive CD8+ T cells. Antigen-specific T cells that recognize endogenously processed and presented epitopes are detected using peptide–MHC (pMHC) multimers. Single multimer-positive T cells are sorted for the identification of TCR sequences, after an optional step that includes clonal expansion and functional characterization. The time required to identify neoepitope-specific T cells is 15 d, with an additional 2–4 weeks required for clonal expansion and downstream functional characterization. Identified neoepitopes and corresponding TCRs provide candidates for use in vaccination and TCR-based cancer immunotherapies, and datasets generated by this technology should be useful for improving algorithms to predict immunogenic neoantigens. The percentage of cancer neoantigens that are spontaneously recognized by T cells is generally very low. This protocol describes how CD8+ T cells from healthy donors can be used for enhanced targeting of these neoantigens.
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