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Diversity among clinical isolates of Histoplasma capsulatum detected by polymerase chain reaction with arbitrary primers.

机译:通过与任意引物的聚合酶链反应检测到的荚膜组织胞浆菌临床分离株之间的多样性。

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摘要

Clinical isolates of the fungal respiratory and systemic pathogen Histoplasma capsulatum have been placed in several different classes by using genomic restriction fragment length polymorphisms (RFLPs), but in general have not been distinguished further. We report here that a polymerase chain reaction (PCR)-based DNA fingerprinting method that has been termed arbitrary primer or random amplified polymorphic DNA (RAPD) PCR can distinguish among isolates in a single RFLP class. In this method, arbitrarily chosen oligonucleotides are used to prime DNA synthesis from genomic sites that they fortuitously match, or almost match, to generate strain-specific arrays of DNA fragments. Each of 29 isolates of RFLP class 2, the group endemic in the American Midwest, was distinguished by using just three arbitrary primers. In contrast, laboratory-derived S and E colony morphology variants of two strains were not distinguished from their R parents by using 18 such primers. Thus, the clinical isolates of H. capsulatum are quite diverse, but their genomes remain stable during laboratory culture. These outcomes suggest new possibilities for epidemiological analysis and studies of fungal populations in infected hosts.
机译:通过使用基因组限制性片段长度多态性(RFLP),已将真菌性呼吸道和全身性病原体荚膜组织胞浆菌的临床分离株分为几种不同的类别,但总体上没有进一步区分。我们在这里报告说,一种基于聚合酶链反应(PCR)的DNA指纹方法已被称为任意引物或随机扩增多态性DNA(RAPD)PCR可以区分单个RFLP类中的分离株。在这种方法中,可以使用任意选择的寡核苷酸从它们偶然匹配或几乎匹配的基因组位点引发DNA合成,以生成DNA片段的菌株特异性阵列。仅使用三个任意引物就区分了RFLP 2类(美国中西部地区的地方性)的29种分离株。相反,通过使用18个这样的引物,没有将两个菌株的实验室来源的S和E菌落形态变异与它们的R亲本区分开。因此,荚膜嗜血杆菌的临床分离株非常多样,但是它们的基因组在实验室培养期间保持稳定。这些结果为流行病学分析和感染宿主真菌种群的研究提供了新的可能性。

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