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通过热稳定的 II 型内含子逆转录酶模板转换,实现人类血浆 DNA 的简易单链 DNA 测序。

Facile single-stranded DNA sequencing of human plasma DNA via thermostable group II intron reverse transcriptase template switching.

机构信息

Institute for Cellular and Molecular Biology, University of Texas at Austin, Austin, Texas, 78712, USA.

Department of Molecular Biosciences, University of Texas at Austin, Austin, Texas, 78712, USA.

出版信息

Sci Rep. 2017 Aug 21;7(1):8421. doi: 10.1038/s41598-017-09064-w.

Abstract

High-throughput single-stranded DNA sequencing (ssDNA-seq) of cell-free DNA from plasma and other bodily fluids is a powerful method for non-invasive prenatal testing, and diagnosis of cancers and other diseases. Here, we developed a facile ssDNA-seq method, which exploits a novel template-switching activity of thermostable group II intron reverse transcriptases (TGIRTs) for DNA-seq library construction. This activity enables TGIRT enzymes to initiate DNA synthesis directly at the 3' end of a DNA strand while simultaneously attaching a DNA-seq adapter without end repair, tailing, or ligation. Initial experiments using this method to sequence E. coli genomic DNA showed that the TGIRT enzyme has surprisingly robust DNA polymerase activity. Further experiments showed that TGIRT-seq of plasma DNA from a healthy individual enables analysis of nucleosome positioning, transcription factor-binding sites, DNA methylation sites, and tissues-of-origin comparably to established methods, but with a simpler workflow that captures precise DNA ends.

摘要

高通量单链 DNA 测序(ssDNA-seq)技术可对血浆和其他体液中的游离 DNA 进行检测,是一种用于非侵入性产前检测和癌症及其他疾病诊断的强大方法。在这里,我们开发了一种简便的 ssDNA-seq 方法,该方法利用了热稳定的 II 组内含子逆转录酶(TGIRTs)的新型模板转换活性来构建 DNA-seq 文库。这种活性使 TGIRT 酶能够在 DNA 链的 3'端直接启动 DNA 合成,同时在无需末端修复、加尾或连接的情况下连接 DNA-seq 接头。使用该方法对大肠杆菌基因组 DNA 进行测序的初步实验表明,TGIRT 酶具有惊人的强大 DNA 聚合酶活性。进一步的实验表明,健康个体血浆 DNA 的 TGIRT-seq 可分析核小体定位、转录因子结合位点、DNA 甲基化位点和组织来源,与已建立的方法相当,但具有更简单的工作流程,可捕获精确的 DNA 末端。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e0f4/5566474/cf2ebb4d725b/41598_2017_9064_Fig1_HTML.jpg

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