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Targeting individual cells by barcode in pooled sequence libraries

机译:通过汇集序列库中的条形码定位个体细胞

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Transcriptional profiling of thousands of single cells in parallel by RNA-seq is now routine. However, due to reliance on pooled library preparation, targeting analysis to particular cells of interest is difficult. Here, we present a multiplexed PCR method for targeted sequencing of select cells from pooled single-cell sequence libraries. We demonstrated this molecular enrichment method on multiple cell types within pooled single-cell RNA-seq libraries produced from primary human blood cells. We show how molecular enrichment can be combined with FACS to efficiently target ultra-rare cell types, such as the recently identified AXL(+)SIGLEC6(+) dendritic cell (AS DC) subset, in order to reduce the required sequencing effort to profile single cells by 100-fold. Our results demonstrate that DNA barcodes identifying cells within pooled sequencing libraries can be used as targets to enrich for specific molecules of interest, for example reads from a set of target cells.
机译:RNA-SEQ并联成千上万的单细胞的转录剖析现在是常规的。 然而,由于依赖于汇集的图书馆制剂,难以瞄准对感兴趣的特定细胞的分析。 这里,我们介绍了一种用于来自池的单小区序列库的选择单元的有针对性测序的多路复用PCR方法。 我们在汇集的单细胞RNA-SEQ文库内展示了这种分子富集法在原代人血细胞产生的汇集的单细胞RNA-SEQ文库中。 我们展示了分子富集如何与FACS合并,以有效地靶向超稀有细胞类型,例如最近鉴定的AXL(+)SigleC6(+)树突状细胞(作为DC)子集,以减少所需的序列概况 单细胞100倍。 我们的结果表明,鉴定汇集的测序文库内的细胞的DNA条形码可以用作富集特定感兴趣的分子的靶标,例如从一组靶细胞读取。

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