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比较五种分子分型方法在突尼斯区分肯塔基沙门氏菌分离株的效果。

Comparison of five molecular subtyping methods for differentiation of Salmonella Kentucky isolates in Tunisia.

机构信息

Laboratoire Traitement et Recyclage des Eaux, Centre de Recherche et des Technologies des Eaux (C.E.R.T.E), Borj Cédria, P.O. BOX 273, 8020, Soliman, Tunisie,

出版信息

World J Microbiol Biotechnol. 2014 Jan;30(1):87-98. doi: 10.1007/s11274-013-1414-1. Epub 2013 Jul 10.

DOI:10.1007/s11274-013-1414-1
PMID:23839713
Abstract

Salmonellosis is one of the most common causes of food-borne infection worldwide. In the last decade, Salmonella enterica serovar Kentucky has shown an increase in different parts of the world with the concurrent emergence of multidrug-resistant isolates. These drug-resistant types spread from Africa and the Middle East to Europe and Asia. Although S. Kentucky serovar is of potential human relevance, there is currently no standardized fingerprinting method for it, in Tunisia. In the present study, a collection of 57 Salmonella Kentucky isolates were analyzed using plasmid profiling, pulsed-field gel electrophoresis (PFGE), ribotyping, enterobacterial repetitive intergenic consensus (ERIC) fingerprinting, and Random Amplification of Polymorphic DNA. Plasmid profiling showed a discriminatory index (D) of 0.290, and only 9 out of 57 (16%) isolates carried plasmids, which represents a limitation of this technique. Fingerprinting of genomic DNA by PFGE and ribotyping produced 4 and 5 patterns, respectively. Distinct PFGE patterns (SX1, SX2, SX3, and SX4) were generated for only 28 strains out of 57 (49.1%) with a D value of 0.647. RAPD fingerprinting with primers RAPD1 and RAPD2 produced 4 and 20 patterns, respectively. ERIC fingerprinting revealed 14 different patterns with a high discriminatory index (D) of 0.903. When the methods were combined, the best combination of two methods was ERIC-2 with RAPD2. These results indicates that a single method cannot be relied upon for discriminating between S. Kentucky strains, and a combination of typing methods such ERIC2 and RAPD2 allows further discrimination.

摘要

肠炎沙门氏菌是世界范围内最常见的食源性感染原因之一。在过去的十年中,肠炎沙门氏菌血清型肯塔基州在世界不同地区的出现率有所增加,同时出现了多药耐药株。这些耐药类型从非洲和中东传播到欧洲和亚洲。尽管 S. Kentucky 血清型与人类有潜在相关性,但目前在突尼斯还没有针对它的标准化指纹图谱方法。在本研究中,使用质粒图谱分析、脉冲场凝胶电泳(PFGE)、核糖体分型、肠杆菌重复基因间一致性(ERIC)指纹图谱和随机扩增多态性 DNA 对 57 株肠炎沙门氏菌 Kentucky 分离株进行了分析。质粒图谱分析显示分辨指数(D)为 0.290,只有 57 株中的 9 株(16%)携带质粒,这是该技术的局限性。PFGE 和核糖体分型对基因组 DNA 的指纹图谱分析分别产生了 4 种和 5 种模式。只有 57 株中的 28 株(49.1%)产生了独特的 PFGE 模式(SX1、SX2、SX3 和 SX4),D 值为 0.647。引物 RAPD1 和 RAPD2 的 RAPD 指纹图谱分别产生了 4 种和 20 种模式。ERIC 指纹图谱显示了 14 种不同的模式,具有较高的分辨指数(D)为 0.903。当这些方法结合使用时,ERIC-2 和 RAPD2 这两种方法的最佳组合。这些结果表明,不能仅依靠单一方法来区分 S. Kentucky 菌株,需要结合 ERIC2 和 RAPD2 等多种分型方法进行进一步区分。

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