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开发和评估用于检测和区分健康个体肠道内阿米巴原虫的分子工具。

Development and evaluation of molecular tools for detecting and differentiating intestinal amoebae in healthy individuals.

机构信息

Laboratoire de recherche 'Parasitologie Médicale, Biotechnologies et Biomolécules', LR 16-IPT-06,Université Tunis El-Manar, Institut Pasteur de Tunis, 13 place Pasteur,B.P. 74 1002 Tunis Belvédère,Tunisia.

Department of Bacteria,Unit of Mycology and Parasitology, Parasites & Fungi, Statens Serum Institut,Artillerivej 5, DK-2300 Copenhagen S,Denmark.

出版信息

Parasitology. 2019 May;146(6):821-827. doi: 10.1017/S0031182018002196. Epub 2019 Jan 14.

DOI:10.1017/S0031182018002196
PMID:30638175
Abstract

Amoebae are single-celled parasites frequently colonizing human gut. However, few molecular tools are available for accurate identification. Here, we evaluated a panel of polymerase chain reactions (PCRs) targeting Entamoeba histolytica, Entamoeba dispar, Entamoeba coli, Entamoeba hartmanni, Entamoeba polecki, Endolimax nana and Iodamoeba bütschlii. Thirty-six faecal samples (18 containing at least one amoeba species by microscopy and 18 microscopy negative for amoebae) were tested. Real-time PCRs were used for detection and differentiation of E. histolytica and E. dispar. Conventional PCR with Sanger sequencing were applied for detection and differentiation of E. coli, E. hartmanni, E. polecki, E. nana and I. bütschlii. All microscopy results were confirmed by DNA-based methods. However, more samples were positive for single and mixed amoebic species by DNA-based assays than by microscopy (22 vs 18 and 7 vs 1, respectively). DNA sequencing allowed identification of E. coli subtypes (ST1 and ST2), showed low intra-specific variation within E. hartmanni, identified two phylogenetically distinct groups within E. nana, and identified Iodamoeba at the ribosomal lineage level. Taking into account the high intra-genetic diversity within some of the species at the small subunit (SSU) rRNA gene level, amplification of SSU rRNA genes with subsequent sequencing represents a useful method for detecting, differentiating and subtyping intestinal amoebae.

摘要

变形虫是一种常见于人类肠道的单细胞寄生虫,但目前可用的准确鉴定的分子工具较少。本研究评估了一组针对溶组织内阿米巴、迪斯帕内阿米巴、结肠内阿米巴、哈氏内阿米巴、波列基内阿米巴、内蜒属和碘泡虫的聚合酶链反应(PCR)。36 份粪便样本(18 份通过显微镜检查至少含有一种阿米巴,18 份显微镜检查无阿米巴)进行了检测。实时 PCR 用于检测和区分溶组织内阿米巴和迪斯帕内阿米巴。应用常规 PCR 和 Sanger 测序用于检测和区分结肠内阿米巴、哈氏内阿米巴、波列基内阿米巴、内蜒属和碘泡虫。所有显微镜结果均通过 DNA 方法进行了验证。然而,通过 DNA 方法检测到的单种和混合阿米巴种类的样本比通过显微镜检测到的更多(分别为 22 种和 18 种,7 种和 1 种)。DNA 测序允许鉴定出大肠杆菌亚型(ST1 和 ST2),显示哈氏内阿米巴种内具有低的种内变异,在内蜒属内鉴定出两个系统发育上不同的组,以及在核糖体谱系水平鉴定出碘泡虫。考虑到一些种在小亚基(SSU)rRNA 基因水平具有高度的种内遗传多样性,扩增 SSU rRNA 基因并随后进行测序是一种用于检测、区分和分型肠道阿米巴的有用方法。

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