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Very rapid cloning, expression and identifying specificity of T-cell receptors for T-cell engineering

机译:T细胞工程T细胞受体的非常快速的克隆,表达和鉴定特异性

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摘要

Neoantigens can be predicted and in some cases identified using the data obtained from the whole exome sequencing and transcriptome sequencing of tumor cells. These sequencing data can be coupled with single-cell RNA sequencing for the direct interrogation of the transcriptome, surfaceome, and pairing of αβ T-cell receptors (TCRαβ) from hundreds of single T cells. Using these 2 large datasets, we established a platform for identifying antigens recognized by TCRαβs obtained from single T cells. Our approach is based on the rapid expression of cloned TCRαβ genes as Sleeping Beauty transposons and the determination of the introduced TCRαβs' antigen specificity and avidity using a reporter cell line. The platform enables the very rapid identification of tumor-reactive TCRs for the bioengineering of T cells with redirected specificity.
机译:可以预测Neoantigens,并且在一些情况下使用从肿瘤细胞的全外壳测序和转录组测序获得的数据鉴定。这些测序数据可以与单细胞RNA测序偶联,用于直接询问来自数百个T细胞的转录组,表面体和对αβT细胞受体(TCRαβ)的配对。使用这两个大型数据集,我们建立了一种用于识别由单T细胞获得的TCRαβ识别的抗原的平台。我们的方法是基于克隆TCRαβ基因作为睡眠美容转座的快速表达,并使用报告细胞系测定引入的TCRαβS抗原特异性和亲和力。该平台能够通过重定向的特异性来实现对T细胞生物工程的肿瘤反应性TCR的快速鉴定。

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