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微孢子虫核糖体RNA在诊断和系统发育中的应用:综述

Utility of microsporidian rRNA in diagnosis and phylogeny: a review.

作者信息

Weiss L M, Zhu X, Cali A, Tanowitz H B, Wittner M

机构信息

Department of Medicine, Albert Einstein College of Medicine, Bronx, New York 10461.

出版信息

Folia Parasitol (Praha). 1994;41(2):81-90.

PMID:7927064
Abstract

This paper summarizes work done in this laboratory over the last two years on the cloning of microsporidian rRNA by homology PCR and its subsequent use in diagnostic tests and phylogenetic studies. Using highly conserved primers in the 16S or small subunit rRNA (SSU-rRNA) these genes were cloned from human intestinal biopsies with transmission electron microscopy proven Enterocytozoon bieneusi and Septata intestinalis. The SSU-rRNA genes were then used to design and test several primer pairs for the diagnosis of microsporidian infection. Utilizing the polymerase chain reaction and primers V1 and EB450 Ent. bieneusi infected duodenal aspirates or intestinal biopsies could be detected. Using V1 and SI500 infection with S. intestinalis could be detected. In addition to diagnostic tests, phylogenetic relationships were examined using sequence data from the fragment amplified by PCR by primer 530f in the SSU-rRNA and primer 580r in the large subunit rRNA. This data supported the placement of S. intestinalis in the family Encephalitozoonidae. In addition, it confirmed that Encephalitozoon cuniculi, E. hellem and S. intestinalis are distinct organisms. These techniques have broad applications to the study of other microsporidia and the development of a molecular phylogeny.

摘要

本文总结了本实验室在过去两年中通过同源PCR克隆微孢子虫rRNA及其随后在诊断测试和系统发育研究中的应用所开展的工作。使用16S或小亚基rRNA(SSU-rRNA)中的高度保守引物,从经透射电子显微镜证实为比氏肠胞微孢子虫和肠 septata的人肠道活检组织中克隆了这些基因。然后,利用SSU-rRNA基因设计并测试了几对用于诊断微孢子虫感染的引物。利用聚合酶链反应和引物V1和EB450,可以检测到感染比氏肠胞微孢子虫的十二指肠吸出物或肠道活检组织。使用V1和SI500,可以检测到感染肠septata。除了诊断测试外,还利用来自通过SSU-rRNA中的引物530f和大亚基rRNA中的引物580r进行PCR扩增的片段的序列数据来研究系统发育关系。这些数据支持将肠septata归入脑胞微孢子虫科。此外,它证实了兔脑胞内原虫、海伦脑胞内原虫和肠septata是不同的生物体。这些技术在其他微孢子虫的研究和分子系统发育的发展中具有广泛的应用。

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