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对克氏锥虫进行全转录组水平的 mRNA 处理分析、转录组特征分析和基因组序列优化。

Analysis of mRNA processing at whole transcriptome level, transcriptomic profile and genome sequence refinement of Trypanosoma cruzi.

机构信息

Centro de Biología Molecular Severo Ochoa, Consejo Superior de Investigaciones Científicas, Universidad Autónoma de Madrid, Cantoblanco, Madrid, Spain.

Instituto Sanitario de Investigación Princesa, Madrid, Spain.

出版信息

Sci Rep. 2019 Nov 22;9(1):17376. doi: 10.1038/s41598-019-53924-6.

Abstract

The genomic sequence of Trypanosoma cruzi, the protozoan causative of Chagas disease was published more than a decade ago. However, due to their complexity, its complete haploid predicted sequence and therefore its genetic repertoire remains unconfirmed. In this work, we have used RNAseq data to improve the previous genome assembly of Sylvio X10 strain and to define the complete transcriptome at trypomastigote stage (mammalian stage). A total of 22,977 transcripts were identified, of which more than half could be considered novel as they did not match previously annotated genes. Moreover, for the first time in T. cruzi, we are providing their relative abundance levels. We have identified that Sylvio X10 trypomastigotes exhibit a predominance of surface protein genes, specifically those encoding trans-sialidase and mucin-like proteins. On the other hand, detailed analysis of the pre-mRNA processing sites revealed some similarities but also some differences in the spliced leader and different polyadenylation addition sites compared to close related kinetoplastid parasites. Our results also confirm that transcription is bidirectional as occur in other kinetoplastids and the proportion of forward-sense and reverse-sense transcripts is almost equivalent, demonstrating that a strand-specificity does not exist.

摘要

十多年前,就公布了引起恰加斯病的原生动物克氏锥虫的基因组序列。然而,由于其复杂性,其完整的单倍体预测序列及其遗传库仍然没有得到证实。在这项工作中,我们使用 RNAseq 数据改进了 Sylvio X10 株的先前基因组组装,并定义了在锥虫阶段(哺乳动物阶段)的完整转录组。共鉴定出 22977 个转录本,其中超过一半可以被认为是新的,因为它们与先前注释的基因不匹配。此外,我们首次在克氏锥虫中提供了它们的相对丰度水平。我们已经确定,Sylvio X10 锥虫的表面蛋白基因,特别是那些编码转涎酶和粘蛋白样蛋白的基因占优势。另一方面,对前体 mRNA 加工位点的详细分析表明,与密切相关的动基体寄生虫相比,拼接领导和不同聚腺苷酸化添加位点既有相似之处,也有一些差异。我们的结果还证实,转录是双向的,就像在其他动基体寄生虫中一样,正向和反向转录本的比例几乎相等,表明不存在链特异性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fdea/6874640/ca3be297895b/41598_2019_53924_Fig1_HTML.jpg

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