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利用合成长读测序进行靶向转录组分析揭示了结直肠癌进展中的异构体重编程。

Targeted transcriptome analysis using synthetic long read sequencing uncovers isoform reprograming in the progression of colon cancer.

机构信息

Department of Pathology, University of Pittsburgh School of Medicine, Pittsburgh, PA, 15261, USA.

High Throughput Genome Center, University of Pittsburgh School of Medicine, Pittsburgh, PA, 15261, USA.

出版信息

Commun Biol. 2021 Apr 27;4(1):506. doi: 10.1038/s42003-021-02024-1.

Abstract

The characterization of human gene expression is limited by short read lengths, high error rates and large input requirements. Here, we used a synthetic long read (SLR) sequencing approach, LoopSeq, to generate accurate sequencing reads that span full length transcripts using standard short read data. LoopSeq identified isoforms from control samples with 99.4% accuracy and a 0.01% per-base error rate, exceeding the accuracy reported for other long-read technologies. Applied to targeted transcriptome sequencing from colon cancers and their metastatic counterparts, LoopSeq revealed large scale isoform redistributions from benign colon mucosa to primary colon cancer and metastatic cancer and identified several previously unknown fusion isoforms. Strikingly, single nucleotide variants (SNVs) occurred dominantly in specific isoforms and some SNVs underwent isoform switching in cancer progression. The ability to use short reads to generate accurate long-read data as the raw unit of information holds promise as a widely accessible approach in transcriptome sequencing.

摘要

人类基因表达的特征受限于短读长、高错误率和大的输入需求。在这里,我们使用一种合成长读(SLR)测序方法 LoopSeq,利用标准的短读数据生成跨越全长转录本的准确测序读长。LoopSeq 以 99.4%的准确率和 0.01%的每碱基错误率识别出对照样本的异构体,超过了其他长读技术报告的准确率。将 LoopSeq 应用于结肠癌及其转移性肿瘤的靶向转录组测序,揭示了从良性结肠黏膜到原发性结肠癌和转移性癌症的大规模异构体重新分布,并鉴定了几种以前未知的融合异构体。引人注目的是,单核苷酸变异(SNVs)主要发生在特定的异构体中,并且在癌症进展过程中一些 SNVs 发生了异构体转换。使用短读长生成准确的长读长数据作为原始信息单位的能力,有望成为转录组测序中一种广泛适用的方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f59c/8079361/c649e5830714/42003_2021_2024_Fig1_HTML.jpg

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