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首页> 外文期刊>Journal of Clinical Microbiology >Use of PCR-Restriction Fragment Length Polymorphism Analysis To Identify the Main New World Leishmania Species and Analyze Their Taxonomic Properties and Polymorphism by Application of the Assay to Clinical Samples
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Use of PCR-Restriction Fragment Length Polymorphism Analysis To Identify the Main New World Leishmania Species and Analyze Their Taxonomic Properties and Polymorphism by Application of the Assay to Clinical Samples

机译:利用PCR限制性片段长度多态性分析鉴定主要新世界利什曼原虫种类并通过将其应用于临床样品分析其分类学特性和多态性

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摘要

At least 13 characterized Leishmania species are known to infect humans in South America. Five of these parasites are transmitted in the sylvatic ecotopes of the whole French Guianan territory and responsible for cutaneous leishmaniasis. For the diagnosis of cutaneous leishmaniasis, restriction fragment length polymorphism (RFLP) analyses have shown promising results. Thus, the end of the small subunit and internal transcribed spacer 1 of the rRNA genes were sequenced and targeted by PCR-RFLP analysis in the 10 main New World (NW) Leishmania species from the two subgenera. Then, the procedure was tested on 40 samples from patients with cutaneous leishmaniasis, and its results were compared with those of conventional methods. (i) The results of this simple genus-specific method were in agreement with those of previous isoenzyme analyses. (ii) This method distinguished the most medically relevant Leishmania species with only one enzyme (RsaI). (iii) This method could be performed directly on human biopsy specimens (sensitivity of?85.7%). Performing NW Leishmania species typing rapidly and easily in the field constitutes a very valuable improvement for detection of Leishmania spp. Revealing great diversity with several enzymes, this method could also be useful for taxonomic, ecological, and epidemiological studies in space and time.
机译:在南美,已知至少有13种特征性的利什曼原虫物种感染人类。这些寄生虫中有五种在整个法属圭亚那领土的sylvatic生态区中传播,并引起皮肤利什曼病。对于皮肤利什曼病的诊断,限制性片段长度多态性(RFLP)分析显示出令人鼓舞的结果。因此,通过PCR-RFLP分析对两个亚属的10个主要新大陆(Lewismania)物种中rRNA基因的小亚基末端和内部转录间隔区1进行了测序和靶向。然后,对40例皮肤利什曼病患者的样本进行了测试,并将其结果与传统方法进行了比较。 (i)这种简单的属特异性方法的结果与以前的同工酶分析结果一致。 (ii)这种方法仅用一种酶(RsaI)区分了医学上最相关的利什曼原虫物种。 (iii)该方法可直接在人体活检标本上进行(灵敏度约为85.7%)。在野外快速简便地进行NW Leishmania 物种分型,对于检测 Leishmania spp来说是非常有价值的改进。该方法揭示了几种酶的巨大多样性,也可用于时空分类,生态和流行病学研究。

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