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A complete high-quality MinION nanopore assembly of an extensively drug-resistant Mycobacterium tuberculosis Beijing lineage strain identifies novel variation in repetitive PE/PPE gene regions

机译:广泛耐药结核分枝杆菌北京谱系菌株的完整高质量MinION纳米孔组件可鉴定重复PE / PPE基因区域的新变异

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摘要

A better understanding of the genomic changes that facilitate the emergence and spread of drug-resistant Mycobacterium tuberculosis strains is currently required. Here, we report the use of the MinION nanopore sequencer (Oxford Nanopore Technologies) to sequence and assemble an extensively drug-resistant (XDR) isolate, which is part of a modern Beijing sub-lineage strain, prevalent in Western Province, Papua New Guinea. Using 238-fold coverage obtained from a single flow-cell, de novo assembly of nanopore reads resulted into one contiguous assembly with 99.92 % assembly accuracy. Incorporation of complementary short read sequences (Illumina) as part of consensus error correction resulted in a 4 404 064 bp genome with 99.98 % assembly accuracy. This assembly had an average nucleotide identity of 99.7 % relative to the reference genome, H37Rv. We assembled nearly all GC-rich repetitive PE/PPE family genes (166/168) and identified variants within these genes. With an estimated genotypic error rate of 5.3 % from MinION data, we demonstrated identification of variants to include the conventional drug resistance mutations, and those that contribute to the resistance phenotype (efflux pumps/transporter) and virulence. Reference-based alignment of the assembly allowed detection of deletions and insertions. MinION sequencing provided a fully annotated assembly of a transmissible XDR strain from an endemic setting and showed its utility to provide further understanding of genomic processes within Mycobacterium tuberculosis.
机译:当前需要对促进耐药结核分枝杆菌菌株的出现和传播的基因组变化有更好的了解。在这里,我们报告了使用MinION纳米孔测序仪(Oxford Nanopore Technologies)来测序和组装广泛耐药性(XDR)分离株,该分离株是现代北京亚谱系菌株的一部分,该菌株在西方省巴布亚新几内亚普遍存在。使用从单个流通池获得的238倍覆盖率,纳米孔读数的从头组装产生了一个连续组装,组装精度为99.92%。整合互补的短读序列(Illumina)作为共有错误校正的一部分,产生了一个4 404 064 bp基因组,装配精度为99.98%。相对于参考基因组H37Rv,该装配体的平均核苷酸同一性为99.7%。我们组装了几乎所有富含GC的重复性PE / PPE家族基因(166/168),并确定了这些基因中的变异体。根据MinION数据,估计的基因型错误率为5.3%,我们证明了变异体的鉴定,其中包括常规的耐药性突变,以及那些有助于耐药性表型(外排泵/转运蛋白)和毒力的突变。组件的基于参考的对齐方式允许检测缺失和插入。 MinION测序提供了来自地方性环境的可传播XDR菌株的完整注释装配,并显示了其实用性,可提供对结核分枝杆菌内基因组过程的进一步了解。

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