Linking the T cell receptor to the single cell transcriptome in antigen-specific human T cells

被引:85
|
作者
Eltahla, Auda A. [1 ]
Rizzetto, Simone [1 ]
Pirozyan, Mehdi R. [1 ]
Betz-Stablein, Brigid D. [1 ]
Venturi, Vanessa [2 ]
Kedzierska, Katherine [3 ]
Lloyd, Andrew R. [1 ]
Bull, Rowena A. [1 ]
Luciani, Fabio [1 ]
机构
[1] Univ New S Wales, Sch Med Sci, Syst Med Infect Dis Inflammat & Infect Res Ctr, Sydney, NSW 2052, Australia
[2] Univ New S Wales, Kirby Inst Infect & Immun, Sydney, NSW, Australia
[3] Univ Melbourne, Peter Doherty Inst Infect & Immun, Dept Microbiol & Immunol, Melbourne, Vic, Australia
基金
澳大利亚国家健康与医学研究理事会; 英国医学研究理事会;
关键词
RNA-SEQ; FATE DECISIONS; DIFFERENTIATION; REPERTOIRE; SEQUENCE; HETEROGENEITY; SMART-SEQ2; INFECTION; ALIGNMENT; EFFECTOR;
D O I
10.1038/icb.2016.16
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Heterogeneity of T cells is a hallmark of a successful adaptive immune response, harnessing the vast diversity of antigen-specific T cells into a coordinated evolution of effector and memory outcomes. The T cell receptor (TCR) repertoire is highly diverse to account for the highly heterogeneous antigenic world. During the response to a virus multiple individual clones of antigen specific CD8+ (Ag-specific) T cells can be identified against a single epitope and multiple epitopes are recognised. Advances in single-cell technologies have provided the potential to study Ag-specific T cell heterogeneity at both surface phenotype and transcriptome levels, thereby allowing investigation of the diversity within the same apparent sub-population. We propose a new method (VDJPuzzle) to reconstruct the native TCR alpha beta from single cell RNA-seq data of Ag-specific T cells and then to link these with the gene expression profile of individual cells. We applied this method using rare Ag-specific T cells isolated from peripheral blood of a subject who cleared hepatitis C virus infection. We successfully reconstructed productive TCR alpha beta in 56 of a total of 63 cells (89%), with double a and double beta in 18, and 7% respectively, and double TCR alpha beta in 2 cells. The method was validated via standard single cell PCR sequencing of the TCR. We demonstrate that single-cell transcriptome analysis can successfully distinguish Ag-specific T cell populations sorted directly from resting memory cells in peripheral blood and sorted after ex vivo stimulation. This approach allows a detailed analysis of the TCR diversity and its relationship with the transcriptional profile of different clones.
引用
收藏
页码:604 / 611
页数:8
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