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Use of a Mycobacterium tuberculosisH37Rv Bacterial Artificial Chromosome Library for Genome Mapping, Sequencing, and Comparative Genomics

机译:结核分枝杆菌H37Rv细菌人工染色体文库在基因组作图,测序和比较基因组学中的应用

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The bacterial artificial chromosome (BAC) cloning system is capable of stably propagating large, complex DNA inserts in Escherichia coli. As part of the Mycobacterium tuberculosis H37Rv genome sequencing project, a BAC library was constructed in the pBeloBAC11 vector and used for genome mapping, confirmation of sequence assembly, and sequencing. The library contains about 5,000 BAC clones, with inserts ranging in size from 25 to 104 kb, representing theoretically a 70-fold coverage of the M. tuberculosisgenome (4.4 Mb). A total of 840 sequences from the T7 and SP6 termini of 420 BACs were determined and compared to those of a partial genomic database. These sequences showed excellent correlation between the estimated sizes and positions of the BAC clones and the sizes and positions of previously sequenced cosmids and the resulting contigs. Many BAC clones represent linking clones between sequenced cosmids, allowing full coverage of the H37Rv chromosome, and they are now being shotgun sequenced in the framework of the H37Rv sequencing project. Also, no chimeric, deleted, or rearranged BAC clones were detected, which was of major importance for the correct mapping and assembly of the H37Rv sequence. The minimal overlapping set contains 68 unique BAC clones and spans the whole H37Rv chromosome with the exception of a single gap of ~150 kb. As a postgenomic application, the canonical BAC set was used in a comparative study to reveal chromosomal polymorphisms between M. tuberculosis, M. bovis, and M. bovis BCG Pasteur, and a novel 12.7-kb segment present in M. tuberculosis but absent from M. bovis and M. bovis BCG was characterized. This region contains a set of genes whose products show low similarity to proteins involved in polysaccharide biosynthesis. The H37Rv BAC library therefore provides us with a powerful tool both for the generation and confirmation of sequence data as well as for comparative genomics and other postgenomic applications. It represents a major resource for present and future M. tuberculosis research projects.
机译:细菌人工染色体(BAC)克隆系统能够在大肠杆菌中稳定繁殖大型,复杂的DNA插入片段。作为结核分枝杆菌H37Rv基因组测序项目的一部分,在pBeloBAC11载体中构建了BAC文库,用于基因组作图,序列确认和测序。该文库包含约5,000个BAC克隆,插入片段的大小从25到104 kb不等,理论上覆盖了 M的70倍。结核基因组(4.4 Mb)。确定了来自420个BAC的T7和SP6末端的840个序列,并将其与部分基因组数据库的序列进行了比较。这些序列显示出BAC克隆的估计大小和位置与先前测序的粘粒的大小和位置以及所得重叠群之间的极好的相关性。许多BAC克隆代表了测序的粘粒之间的连接克隆,从而完全覆盖了H37Rv染色体,现在,它们正在H37Rv测序项目的框架内进行shot弹枪测序。此外,未检测到嵌合,缺失或重排的BAC克隆,这对于正确定位和装配H37Rv序列至关重要。最小重叠集包含68个独特的BAC克隆,跨越整个H37Rv染色体,但单个缺口约为150 kb。作为后基因组应用,规范的BAC集用于比较研究中,揭示了 M之间的染色体多态性。结核 M。 bovis M。 bovis BCG Pasteur,以及 M中存在的一个新的12.7-kb片段。结核病,但 M却没有。 bovis M。牛血清BCG的特征。该区域包含一组基因,其产物与参与多糖生物合成的蛋白质显示出低相似性。因此,H37Rv BAC库为我们提供了一个强大的工具,可用于生成和确认序列数据,以及用于比较基因组学和其他后基因组学应用。它代表了当前和未来 M的主要资源。结核病研究项目。

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