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聚合酶链反应(PCR)跨越微小隐孢子虫MIC1基因座的ML-2微卫星发生滑动,使得能够开发一种PCR检测方法,该方法能够区分人兽共患的微小隐孢子虫与其他引起人类感染的隐孢子虫物种。

PCR slippage across the ML-2 microsatellite of the Cryptosporidium MIC1 locus enables development of a PCR assay capable of distinguishing the zoonotic Cryptosporidium parvum from other human infectious Cryptosporidium species.

作者信息

Webber M A, Sari I, Hoefel D, Monis P T, King B J

机构信息

Department of Medical Biotechnology, School of Medicine, Flinders University, Bedford Park, SA, Australia.

出版信息

Zoonoses Public Health. 2014 Aug;61(5):324-37. doi: 10.1111/zph.12074. Epub 2013 Aug 17.

DOI:10.1111/zph.12074
PMID:23954136
Abstract

Cryptosporidium are ubiquitous and significant enteropathogens of all classes of vertebrates and a major cause of human morbidity and mortality worldwide. Of the 24 recognized species, the zoonotic Cryptosporidium parvum and the host-specific Cryptosporidium hominis cause the majority of cases of human cryptosporidiosis. Here, we report on structural and transcriptional variability between C. parvum and C. hominis at the MIC1 locus, which encodes a microneme localized thrombospondin-like domain containing protein previously demonstrated to be critical for host cell infection by C. parvum. We demonstrate, using reverse transcription quantitative PCR with the aid of genomic data from the EuPathDB site, that the transcribed product in C. hominis is both truncated and significantly down-regulated in the sporozoite. We hypothesize that CpMIC1 may be a genetic factor involved in facilitating the wider host range of C. parvum in comparison with the specific host range of C. hominis. Furthermore, we show that the presence of a microsatellite (ML-2) within the C. parvum MIC-1 locus enables the development of a PCR marker that can rapidly distinguish the zoonotic C. parvum from C. hominis and other significant human infectious Cryptosporidium species due to reproducible PCR slippage across the ML-2 microsatellite. Additionally, we demonstrate that this locus is tightly linked to the GP60 locus, a locus commonly used in the genetic characterization of C. parvum and C. hominis isolates. This marker should provide a robust and additional tool to aid in the rapid identification of C. parvum from other Cryptosporidium species.

摘要

隐孢子虫是所有脊椎动物普遍存在的重要肠道病原体,也是全球人类发病和死亡的主要原因。在已确认的24个物种中,人兽共患的微小隐孢子虫和宿主特异性的人隐孢子虫导致了大多数人类隐孢子虫病病例。在此,我们报告微小隐孢子虫和人隐孢子虫在MIC1基因座处的结构和转录变异性,该基因座编码一种微线体定位的含血小板反应蛋白样结构域的蛋白质,先前已证明该蛋白质对微小隐孢子虫感染宿主细胞至关重要。我们借助EuPathDB网站的基因组数据,通过逆转录定量PCR证明,人隐孢子虫中的转录产物在子孢子中既被截断又显著下调。我们推测,与宿主特异性的人隐孢子虫相比,微小隐孢子虫的CpMIC1可能是一个参与促进其更广泛宿主范围的遗传因素。此外,我们表明微小隐孢子虫MIC-1基因座内微卫星(ML-2)的存在使得能够开发一种PCR标记,由于ML-2微卫星上可重复的PCR滑动,该标记可以快速区分人兽共患的微小隐孢子虫与人隐孢子虫以及其他重要的人类感染性隐孢子虫物种。此外,我们证明该基因座与GP60基因座紧密连锁,GP60基因座是微小隐孢子虫和人隐孢子虫分离株基因特征分析中常用的基因座。该标记应为从其他隐孢子虫物种中快速鉴定微小隐孢子虫提供一种强大的辅助工具。

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引用本文的文献

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PLoS One. 2016 Dec 14;11(12):e0168169. doi: 10.1371/journal.pone.0168169. eCollection 2016.
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Integrated cryptosporidium assay to determine oocyst density, infectivity, and genotype for risk assessment of source and reuse water.用于确定卵囊密度、感染性和基因型以评估水源水和回用水风险的隐孢子虫综合检测方法
Appl Environ Microbiol. 2015 May 15;81(10):3471-81. doi: 10.1128/AEM.00163-15. Epub 2015 Mar 13.