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一种用于病原体基因组学的杂交目标富集方法。

A hybridization target enrichment approach for pathogen genomics.

机构信息

Department of Biomolecular Engineering, University of California Santa Cruz , Santa Cruz, California, USA.

Center for Laboratory Sciences, California Department of Public Health, Microbial Diseases Laboratory Branch , Richmond, California, USA.

出版信息

mBio. 2023 Oct 31;14(5):e0188923. doi: 10.1128/mbio.01889-23. Epub 2023 Oct 13.

Abstract

Emerging infectious diseases require continuous pathogen monitoring. Rapid clinical diagnosis by nucleic acid amplification is limited to a small number of targets and may miss target detection due to new mutations in clinical isolates. Whole-genome sequencing (WGS) identifies genome-wide variations that may be used to determine a pathogen's drug resistance patterns and phylogenetically characterize isolates to track disease origin and transmission. WGS is typically performed using DNA isolated from cultured clinical isolates. Culturing clinical specimens increases turn-around time and may not be possible for fastidious bacteria. To overcome some of these limitations, direct sequencing of clinical specimens has been attempted using expensive capture probes to enrich the entire genomes of target pathogens. We present a method to produce a cost-effective, time-efficient, and large-scale synthesis of probes for whole-genome enrichment. We envision that our method can be used for direct clinical sequencing of a wide range of microbial pathogens for genomic epidemiology.

摘要

新发传染病需要持续进行病原体监测。通过核酸扩增进行快速临床诊断的局限性在于可检测的靶标数量有限,并且由于临床分离株的新突变,可能会错过靶标检测。全基因组测序(WGS)可识别基因组范围内的变异,这些变异可用于确定病原体的耐药模式,并对分离株进行系统发生特征分析以追踪疾病的起源和传播。WGS 通常使用从培养的临床分离株中提取的 DNA 进行。培养临床标本会增加周转时间,并且对于苛刻的细菌可能无法进行培养。为了克服这些限制中的一些,已经尝试使用昂贵的捕获探针直接对临床标本进行测序,以富集目标病原体的整个基因组。我们提出了一种经济高效、耗时少且能大规模合成探针进行全基因组富集的方法。我们设想,我们的方法可用于对广泛的微生物病原体进行直接临床测序,以进行基因组流行病学研究。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/da5f/10653935/ee8a0d2aa1d9/mbio.01889-23.f001.jpg

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