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The application of real-time PCR to the analysis of T cell repertoires

机译:实时荧光定量PCR在T细胞库分析中的应用

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摘要

The diversity of T-cell populations is determined by the spectrum of antigen-specific T-cell receptors (TCRs) that are heterodimers of α and β subunits encoded by rearranged combinations of variable (AV and BV), joining (AJ and BJ), and constant region genes (AC and BC). We have developed a novel approach for analysis of β transcript diversity in mice with a real-time PCR-based method that uses a matrix of BV- and BJ-specific primers to amplify 240 distinct BV–BJ combinations. Defined endpoints (Ct values) and dissociation curves are generated for each BV–BJ combination and the Ct values are consolidated in a matrix that characterizes the β transcript diversity of each RNA sample. Relative diversities of BV–BJ combinations in individual RNA samples are further described by estimates of scaled entropy. A skin allograft system was used to demonstrate that dissection of repertoires into 240 BV–BJ combinations increases efficiency of identifying and sequencing β transcripts that are overrepresented at inflammatory sites. These BV–BJ matrices should generate greater investigation in laboratory and clinical settings due to increased throughput, resolution and identification of overrepresented TCR transcripts.
机译:T细胞群体的多样性取决于抗原特异性T细胞受体(TCR)的光谱,该受体是α和β亚基的异二聚体,由受体(AJ和BJ),和恒定区基因(AC和BC)。我们已经开发了一种新颖的方法,用于通过基于实时PCR的方法分析小鼠β转录物多样性,该方法使用BV和BJ特异性引物的矩阵来扩增240种不同的BV–BJ组合。为每种BV–BJ组合生成明确的终点(Ct值)和解离曲线,并将Ct值合并到一个表征每个RNA样品β转录本多样性的矩阵中。各个RNA样品中BV–BJ组合的相对多样性通过比例熵的估计进一步描述。使用皮肤同种异体移植系统证明,将所有组成部分解剖为240个BV–BJ组合可提高识别和测序炎症部位过度表达的β转录本的效率。由于通量,分辨率和鉴定过高的TCR转录本的增加,这些BV–BJ基质应在实验室和临床环境中进行更多的研究。

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