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基于聚合酶链反应的DNA指纹技术在李斯特菌属鉴定中的比较及其在非典型李斯特菌分离株中的应用

Comparison of PCR-based DNA fingerprinting techniques for the identification of Listeria species and their use for atypical Listeria isolates.

作者信息

Vaneechoutte M, Boerlin P, Tichy H V, Bannerman E, Jäger B, Bille J

机构信息

Department of Microbiology and Immunology, University Hospital, Gent, Belgium.

出版信息

Int J Syst Bacteriol. 1998 Jan;48 Pt 1:127-39. doi: 10.1099/00207713-48-1-127.

DOI:10.1099/00207713-48-1-127
PMID:9542083
Abstract

Four PCR-based DNA fingerprinting techniques were compared for their ability to identify at the species level a heterogeneous collection of isolates belonging to the six valid Listeria species. 16S rDNA-RFLP analysis identified all species and 16S rDNA-SSCP analysis identified almost all species. Also, isolates with unusual biochemical characteristics and/or unusual antigenic composition could be identified correctly. rRNA-intracistronic length polymorphism analysis suffered from high intraspecific variability, a limited number of fragments per profile, and small length differences between the spacers of different species. tRNA-intergenic length polymorphism analysis resulted in identification of all isolates but one, when fluorescent DNA capillary electrophoresis was used such that fragment length differences of 1 bp could be resolved. The four techniques yielded comparable results relevant to the taxonomy of Listeria. They all indicate a high degree of genetic relatedness between L. innocua and L. welshimeri, homogeneity of L. grayi, distinct but clear relatedness of L. grayi to the other Listeria species, a clear distinction between the two subspecies of L. ivanovii, and a clear distinction between Listeria isolates and isolates from closely related taxa or from species which are phenotypically difficult to distinguish from Listeria. New sequence determination of the 16S rRNA gene was necessary to obtain sequences in accordance with the findings of 16S rDNA-RFLP analysis.

摘要

比较了四种基于聚合酶链反应(PCR)的DNA指纹识别技术,以确定它们在物种水平上识别属于六个有效李斯特菌物种的异质分离株集合的能力。16S rDNA限制性片段长度多态性分析(16S rDNA-RFLP分析)能识别所有物种,16S rDNA单链构象多态性分析(16S rDNA-SSCP分析)能识别几乎所有物种。此外,具有异常生化特征和/或异常抗原组成的分离株也能被正确识别。核糖体RNA基因内长度多态性分析存在种内变异性高、每个图谱片段数量有限以及不同物种间隔区长度差异小的问题。当使用荧光DNA毛细管电泳以分辨1 bp的片段长度差异时,tRNA基因间长度多态性分析能识别除一个分离株外的所有分离株。这四种技术在李斯特菌分类学方面产生了可比的结果。它们都表明无害李斯特菌和威氏李斯特菌之间存在高度的遗传相关性,格氏李斯特菌具有同质性,格氏李斯特菌与其他李斯特菌物种有明显但清晰的相关性,伊氏李斯特菌的两个亚种之间有明显区别,并且李斯特菌分离株与密切相关分类群的分离株或与表型上难以与李斯特菌区分的物种的分离株之间有明显区别。需要对16S rRNA基因进行新的序列测定,以获得与16S rDNA-RFLP分析结果一致的序列。

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