Detection of three different types of 'Tropheryma whippelii' directly from clinical specimens by sequencing, single-strand conformation polymorphism (SSCP) analysis and type-specific PCR of their 16S-23S ribosomal intergenic spacer region.

H P Hinrikson, F Dutly, S Nair, M Altwegg
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引用次数: 56

Abstract

The 16S-23S rDNA intergenic spacer region of organisms identical with or closely related to 'Tropheryma whippelii', the uncultivated causative agent of Whipple's disease, was analysed directly from 38 clinical specimens of 28 patients using a specific nested PCR followed by direct sequencing. As compared to the reference sequence in public databases, two novel 'T. whippelii' spacer types were recognized. In the absence of DNA-DNA hybridization data it is uncertain whether the three types found represent subtypes of a single species or three different but closely related species. Methods were developed to detect all three variants by single-strand conformation polymorphism analysis and by type-specific PCR assays, thus allowing the screening of large numbers of specimens. Further studies may provide a clue to the possible associations between the type of infecting strain and the various clinical presentations of Whipple's disease.

通过测序、单链构象多态性(SSCP)分析和16S-23S核糖体基因间间隔区型特异性PCR检测直接来自临床标本的3种不同类型的“惠氏Tropheryma whippelii”。
从28例患者的38份临床标本中,采用特定的巢式PCR,直接分析了与惠普尔病未培养病原体“惠氏Tropheryma whippelii”相同或密切相关的生物体的16S-23S rDNA基因间隔区。与公共数据库的参考序列进行比较,识别出两种新的“T. whippelii”间隔型。在缺乏DNA-DNA杂交数据的情况下,不确定发现的三种类型是代表单一物种的亚型还是三个不同但密切相关的物种。通过单链构象多态性分析和类型特异性PCR分析,开发了检测所有三种变异的方法,从而可以筛选大量标本。进一步的研究可能为感染菌株的类型与惠普尔病的各种临床表现之间的可能联系提供线索。
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