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用于大规模平行靶向测序的超长寡核苷酸溶液杂交选择法。

Solution hybrid selection with ultra-long oligonucleotides for massively parallel targeted sequencing.

作者信息

Gnirke Andreas, Melnikov Alexandre, Maguire Jared, Rogov Peter, LeProust Emily M, Brockman William, Fennell Timothy, Giannoukos Georgia, Fisher Sheila, Russ Carsten, Gabriel Stacey, Jaffe David B, Lander Eric S, Nusbaum Chad

机构信息

Broad Institute of MIT and Harvard, 7 Cambridge Center, Cambridge, Massachusetts 02142, USA.

出版信息

Nat Biotechnol. 2009 Feb;27(2):182-9. doi: 10.1038/nbt.1523. Epub 2009 Feb 1.

Abstract

Targeting genomic loci by massively parallel sequencing requires new methods to enrich templates to be sequenced. We developed a capture method that uses biotinylated RNA 'baits' to fish targets out of a 'pond' of DNA fragments. The RNA is transcribed from PCR-amplified oligodeoxynucleotides originally synthesized on a microarray, generating sufficient bait for multiple captures at concentrations high enough to drive the hybridization. We tested this method with 170-mer baits that target >15,000 coding exons (2.5 Mb) and four regions (1.7 Mb total) using Illumina sequencing as read-out. About 90% of uniquely aligning bases fell on or near bait sequence; up to 50% lay on exons proper. The uniformity was such that approximately 60% of target bases in the exonic 'catch', and approximately 80% in the regional catch, had at least half the mean coverage. One lane of Illumina sequence was sufficient to call high-confidence genotypes for 89% of the targeted exon space.

摘要

通过大规模平行测序靶向基因组位点需要新的方法来富集待测序的模板。我们开发了一种捕获方法,该方法使用生物素化的RNA“诱饵”从DNA片段“池”中捞出目标。RNA是从最初在微阵列上合成的PCR扩增寡脱氧核苷酸转录而来的,产生足够的诱饵用于多次捕获,其浓度足以驱动杂交。我们使用Illumina测序作为读出方式,用靶向超过15,000个编码外显子(2.5 Mb)和四个区域(总计1.7 Mb)的170聚体诱饵测试了该方法。约90%的唯一比对碱基落在诱饵序列上或其附近;高达50%位于外显子本身。其均匀性使得外显子“捕获”中约60%的目标碱基以及区域捕获中约80%的目标碱基具有至少一半的平均覆盖率。Illumina测序的一个泳道足以对89%的靶向外显子空间进行高置信度基因型分型。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/df20/2663421/d4702162f3e5/nihms86158f1.jpg

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