Rapid screening of T-cell receptor (TCR) variable gene usage by multiplex PCR: Application for assessment of clonal composition

被引:55
作者
Akatsuka, Y
Martin, EG
Madonik, A
Barsoukov, AA
Hansen, JA
机构
[1] Fred Hutchinson Canc Res Ctr, Div Clin Res, Seattle, WA 98109 USA
[2] PE Appl Biosyst, Foster City, CA USA
[3] Univ Washington, Sch Med, Dept Med, Seattle, WA 98195 USA
来源
TISSUE ANTIGENS | 1999年 / 53卷 / 02期
关键词
multiplex PCR; spectratyping; T-cell cloning; TCR;
D O I
10.1034/j.1399-0039.1999.530202.x
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
The selection of various T-cell receptor (TCR) gene families and complex rearrangements during intra-thymic differentiation provide the basis for the expression of antigen specificity by mature T cells. TCR beta variable (TCRBV) transcripts can be identified by RT PCR, but multiple reactions are required to detect ail genes of the TCRBV subfamilies. We describe here a multiplex PCR method that amplifies 46 functional genes comparing 23 TCRBV families in 5 reactions where each reaction contains 4 iv 7 specific primers together with a single fluorescence-tagged TCR beta constant region primer. Between 8 and 10 distinct subtypes within each of the 23 TCRBV families can be identified by analysis of the CDR3 length. Multiplex PCR products isolated from agarose gels can be subjected to direct sequencing fur confirmation and definitive clonotyping ii necessary. The data illustrated here show that the multiplex PCR technique is useful for screening TCRBV usage and can be easily adapted for analysis of clonal composition in T-cell populations.
引用
收藏
页码:122 / 134
页数:13
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