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通过饱和转座子诱变对结核分枝杆菌基因组进行综合必需性分析。

Comprehensive Essentiality Analysis of the Mycobacterium tuberculosis Genome via Saturating Transposon Mutagenesis.

作者信息

DeJesus Michael A, Gerrick Elias R, Xu Weizhen, Park Sae Woong, Long Jarukit E, Boutte Cara C, Rubin Eric J, Schnappinger Dirk, Ehrt Sabine, Fortune Sarah M, Sassetti Christopher M, Ioerger Thomas R

机构信息

Department of Computer Science and Engineering, Texas A&M University, College Station, Texas, USA.

Department of Immunology and Infectious Diseases, Harvard TH Chan School of Public Health, Boston, Massachusetts, USA.

出版信息

mBio. 2017 Jan 17;8(1):e02133-16. doi: 10.1128/mBio.02133-16.

Abstract

UNLABELLED

For decades, identifying the regions of a bacterial chromosome that are necessary for viability has relied on mapping integration sites in libraries of random transposon mutants to find loci that are unable to sustain insertion. To date, these studies have analyzed subsaturated libraries, necessitating the application of statistical methods to estimate the likelihood that a gap in transposon coverage is the result of biological selection and not the stochasticity of insertion. As a result, the essentiality of many genomic features, particularly small ones, could not be reliably assessed. We sought to overcome this limitation by creating a completely saturated transposon library in Mycobacterium tuberculosis In assessing the composition of this highly saturated library by deep sequencing, we discovered that a previously unknown sequence bias of the Himar1 element rendered approximately 9% of potential TA dinucleotide insertion sites less permissible for insertion. We used a hidden Markov model of essentiality that accounted for this unanticipated bias, allowing us to confidently evaluate the essentiality of features that contained as few as 2 TA sites, including open reading frames (ORF), experimentally identified noncoding RNAs, methylation sites, and promoters. In addition, several essential regions that did not correspond to known features were identified, suggesting uncharacterized functions that are necessary for growth. This work provides an authoritative catalog of essential regions of the M. tuberculosis genome and a statistical framework for applying saturating mutagenesis to other bacteria.

IMPORTANCE

Sequencing of transposon-insertion mutant libraries has become a widely used tool for probing the functions of genes under various conditions. The Himar1 transposon is generally believed to insert with equal probabilities at all TA dinucleotides, and therefore its absence in a mutant library is taken to indicate biological selection against the corresponding mutant. Through sequencing of a saturated Himar1 library, we found evidence that TA dinucleotides are not equally permissive for insertion. The insertion bias was observed in multiple prokaryotes and influences the statistical interpretation of transposon insertion (TnSeq) data and characterization of essential genomic regions. Using these insights, we analyzed a fully saturated TnSeq library for M. tuberculosis, enabling us to generate a comprehensive catalog of in vitro essentiality, including ORFs smaller than those found in any previous study, small (noncoding) RNAs (sRNAs), promoters, and other genomic features.

摘要

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几十年来,确定细菌染色体中对生存能力至关重要的区域一直依赖于在随机转座子突变体文库中绘制整合位点,以找到无法维持插入的基因座。迄今为止,这些研究分析的是未饱和文库,因此需要应用统计方法来估计转座子覆盖缺口是生物选择而非插入随机性导致的可能性。结果,许多基因组特征,尤其是小特征的必要性无法得到可靠评估。我们试图通过在结核分枝杆菌中创建一个完全饱和的转座子文库来克服这一限制。在通过深度测序评估这个高度饱和文库的组成时,我们发现Himar1元件存在一种先前未知的序列偏差,使得大约9%的潜在TA二核苷酸插入位点不太允许插入。我们使用了一个关于必要性的隐马尔可夫模型来解释这种意外偏差,这使我们能够自信地评估包含少至2个TA位点的特征的必要性,这些特征包括开放阅读框(ORF)、实验鉴定的非编码RNA、甲基化位点和启动子。此外,还鉴定出了几个与已知特征不对应的必需区域,这表明存在一些生长所必需的未表征功能。这项工作提供了结核分枝杆菌基因组必需区域的权威目录以及将饱和诱变应用于其他细菌的统计框架。

重要性

转座子插入突变体文库测序已成为在各种条件下探究基因功能的广泛使用的工具。一般认为Himar1转座子在所有TA二核苷酸处插入的概率相等,因此其在突变体文库中的缺失被视为对相应突变体的生物选择。通过对一个饱和的Himar1文库进行测序,我们发现有证据表明TA二核苷酸对插入的允许程度并不相同。这种插入偏差在多种原核生物中都有观察到,并影响转座子插入(TnSeq)数据的统计解释以及必需基因组区域的表征。利用这些见解,我们分析了一个针对结核分枝杆菌的完全饱和的TnSeq文库,使我们能够生成一份体外必需性的综合目录,包括比以往任何研究中发现的都小的ORF、小(非编码)RNA(sRNA)、启动子和其他基因组特征。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4073/5241402/dae96c8f3c1f/mbo0021731370001.jpg

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