Rapid identification of tumor-reactive T-cell receptors by RNA preamplification-based single-cell sequencing

T细胞受体 桑格测序 T细胞 生物 分子生物学 细胞 癌症研究 计算生物学 DNA测序 DNA 免疫学 免疫系统 遗传学
作者
Yipeng Ma,Fenglan Liu,Bin Li,Hong Zhou,Dongjuan Qiao,Lijuan Deng,Hao Wu,Fuyuan Fang,Youyu Wang,Da Yao,Guilin Hu,Youhui Qian,Mingjun Wang
出处
期刊:Journal of Immunological Methods [Elsevier]
卷期号:504: 113260-113260 被引量:1
标识
DOI:10.1016/j.jim.2022.113260
摘要

T-cell receptor (TCR)-transduced T (TCR-T) cell therapy has shown promising efficacy in the clinical treatment of malignant cancers. However, the populations covered by reported TCRs are still limited. Tumor infiltrating lymphocytes (TILs) are natural reservoirs of tumor-reactive T cells and TCRs. Approaches are required for the fast and cost-effective identification of tumor-reactive TCRs from TILs. The widely employed TCR identification approaches by the clonal expansion of TILs involve a TCR singularization process for the direct pairing of TCR Vα and the Vβ chain. However, the clonal expansion of T cells is well known to require extensive time and effort due to the involvement of T cell cultures. Several single-cell multiplexing PCR methods followed by Sanger sequencing have been developed, representing a cost-effective and fast approach for single-cell TCR identification. In this study, an RNA-based preamplification step was included in the single-cell TCR sequencing, which can reduce the multiplexing PCR amplification to one round. Moreover, the cDNA product of RNA preamplification is derived from the whole genome mRNA, instead of TCR mRNA only by multiplexing primers-based DNA preamplification, which is valuable for many other analyses (e.g., phenotypic analysis) of the tumor-reactive T cells that can be correlated with the identified TCRs. The feasibility for both single α chain and dual α chain TILs of this approach highlights its potential value as a rapid and cost-effective sequencing strategy for the development of TCR-T therapies for solid cancers.
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