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使用基于纳米孔的长读测序技术对韩国人群中的旋毛虫进行从头组装的线粒体基因组分析。

De novo assembled mitogenome analysis of Trichuris trichiura from Korean individuals using nanopore-based long-read sequencing technology.

机构信息

Department of Tropical Medicine and Parasitology and Institute of Endemic Diseases, Seoul National University College of Medicine, Seoul, Republic of Korea.

Department of Biomedical Sciences, Seoul National University College of Medicine, Seoul, Republic of Korea.

出版信息

PLoS Negl Trop Dis. 2023 Aug 28;17(8):e0011586. doi: 10.1371/journal.pntd.0011586. eCollection 2023 Aug.

Abstract

Knowledge about mitogenomes has been proven to be essential in human parasite diagnostics and understanding of their diversity. However, the lack of substantial data for comparative analysis is still a challenge in Trichuris trichiura research. To provide high quality mitogenomes, we utilized long-read sequencing technology of Oxford Nanopore Technologies (ONT) to better resolve repetitive regions and to construct de novo mitogenome assembly minimizing reference biases. In this study, we got three de novo assembled mitogenomes of T. trichiura isolated from Korean individuals. These circular complete mitogenomes of T. trichiura are 14,508 bp, 14,441 bp, and 14,440 bp in length. A total of 37 predicted genes were identified consisting of 13 protein-coding genes (PCGs), 22 transfer RNA (tRNAs) genes, two ribosomal RNA (rRNA) genes (rrnS and rrnL), and two non-coding regions. Interestingly, the assembled mitogenome has up to six times longer AT-rich regions than previous reference sequences, thus proving the advantage of long-read sequencing in resolving unreported non-coding regions. Furthermore, variant detection and phylogenetic analysis using concatenated protein coding genes, cox1, rrnL, and nd1 genes confirmed the distinct molecular identity of this newly assembled mitogenome while at the same time showing high genetic relationship with sequences from China or Tanzania. Our study provided a new set of reference mitogenome with better contiguity and resolved repetitive regions that could be used for meaningful phylogenetic analysis to further understand disease transmission and parasite biology.

摘要

关于线粒体基因组的知识对于人类寄生虫诊断和多样性理解至关重要。然而,在旋毛虫研究中,缺乏实质性数据进行比较分析仍然是一个挑战。为了提供高质量的线粒体基因组,我们利用牛津纳米孔技术(ONT)的长读测序技术,更好地解决重复区域,并构建从头组装的线粒体基因组,最大限度地减少参考偏差。在这项研究中,我们得到了三个从头组装的韩国个体分离的旋毛虫线粒体基因组。这些旋毛虫的圆形完整线粒体基因组长度分别为 14508bp、14441bp 和 14440bp。总共鉴定出 37 个预测基因,包括 13 个蛋白质编码基因(PCGs)、22 个转移 RNA(tRNA)基因、两个核糖体 RNA(rrnS 和 rrnL)基因和两个非编码区。有趣的是,组装的线粒体基因组中富含 AT 的区域比以前的参考序列长了六倍之多,这证明了长读测序在解决未报告的非编码区域方面的优势。此外,使用串联编码蛋白基因、cox1、rrnL 和 nd1 基因进行变异检测和系统发育分析,证实了这个新组装的线粒体基因组具有独特的分子身份,同时与来自中国或坦桑尼亚的序列表现出高度的遗传关系。我们的研究提供了一组具有更好连续性和解决重复区域的新参考线粒体基因组,可用于有意义的系统发育分析,以进一步了解疾病传播和寄生虫生物学。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6d8a/10491297/17f02d43dd38/pntd.0011586.g001.jpg

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