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Multiplexed single-cell RNA-seq via transient barcoding for simultaneous expression profiling of various drug perturbations

机译:通过瞬时条形码的多路复用单细胞RNA-seq可同时进行各种药物干扰的表达谱分析

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摘要

The development of high-throughput single-cell RNA sequencing (scRNA-seq) has enabled access to information about gene expression in individual cells and insights into new biological areas. Although the interest in scRNA-seq has rapidly grown in recent years, the existing methods are plagued by many challenges when performing scRNA-seq on multiple samples. To simultaneously analyze multiple samples with scRNA-seq, we developed a universal sample barcoding method through transient transfection with short barcode oligonucleotides. By conducting a species-mixing experiment, we have validated the accuracy of our method and confirmed the ability to identify multiplets and negatives. Samples from a 48-plex drug treatment experiment were pooled and analyzed by a single run of Drop-Seq. This revealed unique transcriptome responses for each drug and target-specific gene expression signatures at the single-cell level. Our cost-effective method is widely applicable for the single-cell profiling of multiple experimental conditions, enabling the widespread adoption of scRNA-seq for various applications.
机译:高通量单细胞RNA测序(scRNA-seq)的发展使人们可以获得有关单个细胞中基因表达的信息以及对新生物学领域的见识。尽管近年来对scRNA-seq的兴趣迅速增长,但是在对多个样品进行scRNA-seq时,现有方法受到许多挑战的困扰。为了同时用scRNA-seq分析多个样品,我们开发了一种通过短条形码寡核苷酸瞬时转染的通用样品条形码方法。通过进行物种混合实验,我们验证了我们方法的准确性,并确认了识别多重态和阴性的能力。收集来自48种药物治疗实验的样品,并通过单次Drop-Seq分析。这揭示了每种药物的独特转录组反应和单细胞水平的靶标特异性基因表达特征。我们具有成本效益的方法广泛适用于多种实验条件的单细胞分析,从而使scRNA-seq广泛用于各种应用。

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