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鱼类病原体的高质量参考基因组。

A high-quality reference genome for the fish pathogen .

机构信息

School of Chemistry & Molecular Biosciences, The University of Queensland, Brisbane, Queensland, Australia.

Australian Infectious Diseases Research Centre, The University of Queensland, Brisbane, Queensland, Australia.

出版信息

Microb Genom. 2022 Mar;8(3). doi: 10.1099/mgen.0.000777.

Abstract

Fish mortality caused by is a major economic problem in aquaculture in warm and temperate regions globally. There is also risk of zoonotic infection by through handling of contaminated fish. In this study, we present the complete genome sequence of strain QMA0248, isolated from farmed barramundi in South Australia. The 2.12 Mb genome of QMA0248 carries a 32 kb prophage, a 12 kb genomic island and 92 discrete insertion sequence (IS) elements. These include nine novel IS types that belong mostly to the IS family. Comparative and phylogenetic analysis between QMA0248 and publicly available complete genomes revealed discrepancies that are probably due to misassembly in the genomes of isolates ISET0901 and ISNO. Long-range PCR confirmed five rRNA loci in the PacBio assembly of QMA0248, and, unlike 89353, no tandemly repeated rRNA loci in the consensus genome. However, we found sequence read evidence that the tandem rRNA repeat existed within a subpopulation of the original QMA0248 culture. Subsequent nanopore sequencing revealed that the tandem rRNA repeat was the most prevalent genotype, suggesting that there is selective pressure to maintain fewer rRNA copies under uncertain laboratory conditions. Our study not only highlights assembly problems in existing genomes, but provides a high-quality reference genome for QMA0248, including manually curated mobile genetic elements, that will assist future comparative genomic and evolutionary studies.

摘要

鱼类死亡由引起,是全球温暖和温带地区水产养殖的主要经济问题。通过处理受污染的鱼类,也有感染的人畜共患病的风险。在本研究中,我们呈现了来自南澳大利亚养殖尖吻鲈的分离株的完整基因组序列。 菌株 QMA0248 的 2.12 Mb 基因组携带一个 32 kb 的前噬菌体、一个 12 kb 的基因组岛和 92 个离散插入序列 (IS) 元件。这些包括属于 IS 家族的九个新型 IS 类型。与公开可用的完整基因组之间的比较和系统发育分析表明,差异可能是由于分离株 ISET0901 和 ISNO 的基因组组装错误造成的。长距离 PCR 证实了 PacBio 组装的 QMA0248 中的五个 rRNA 基因座,与 89353 不同,在共识基因组中没有串联重复的 rRNA 基因座。然而,我们发现序列读取证据表明,串联 rRNA 重复存在于原始 QMA0248 培养物的亚群中。随后的纳米孔测序表明,串联 rRNA 重复是最普遍的基因型,这表明在不确定的实验室条件下存在维持较少 rRNA 拷贝的选择压力。我们的研究不仅突出了现有基因组中的组装问题,而且为 QMA0248 提供了一个高质量的参考基因组,包括手动整理的移动遗传元件,这将有助于未来的比较基因组学和进化研究。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/35f2/9176272/1f12e7a1033a/mgen-8-0777-g001.jpg

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