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通过分析prtF1基因的RD2区域确定细胞侵袭性耐红霉素和敏感A组链球菌的遗传多样性。

Genetic diversity of cell-invasive erythromycin-resistant and -susceptible group A streptococci determined by analysis of the RD2 region of the prtF1 gene.

作者信息

Spinaci Cinzia, Magi Gloria, Zampaloni Claudia, Vitali Luca A, Paoletti Claudia, Catania Maria R, Prenna Manuela, Ferrante Luigi, Ripa Sandro, Varaldo Pietro E, Facinelli Bruna

机构信息

Department of Microbiology and Biomedical Sciences, University of Ancona Medical School, 60131 Ancona, Italy.

出版信息

J Clin Microbiol. 2004 Feb;42(2):639-44. doi: 10.1128/JCM.42.2.639-644.2004.

Abstract

The RD2 region of the internalization-associated gene prtF1, which encodes the fibronectin-binding repeat domain type 2 of protein F1, plays a crucial role in the entry of group A streptococci (GAS) into epithelial cells. A molecular study of the variability of the RD2 region was carried out with 77 independent Italian GAS, 66 erythromycin resistant (ER) and 11 erythromycin susceptible (ES), which had previously been investigated for the association between erythromycin resistance and ability to enter human respiratory cells. The amplicons obtained from PCR analysis of the RD2 region were consistent with a number of RD2 repeats ranging from one to five, more frequently four (n = 30), three (n = 27), and one (n = 18). A new method to type cell-invasive GAS (RD2 typing) was developed by combining PCR analysis of the RD2 region and restriction analysis of PCR products with endonucleases HaeIII, DdeI, and HinfI. Overall, 10 RD2 types (a to j) were distinguished (all detected among the 66 ER isolates, four detected among the 11 ES isolates). Comparison and correlation of RD2 typing data with the genotype and phenotype of macrolide resistance and with data from PCR M typing and SmaI macrorestriction analysis allowed us to identify 41 different clones (31 among the 66 ER isolates and 10 among the 11 ES isolates). Three major clones accounted for 40% of the isolates (47% of ER strains). Some ES isolates appeared to be related to ER isolates with identical combinations of RD2 type and emm type. While simultaneous use of different typing methods is essential for a thorough investigation of GAS epidemiology, RD2 typing may be especially helpful in typing cell-invasive GAS.

摘要

内化相关基因prtF1的RD2区域编码蛋白F1的2型纤连蛋白结合重复结构域,在A组链球菌(GAS)进入上皮细胞的过程中起关键作用。对77株独立的意大利GAS进行了RD2区域变异性的分子研究,其中66株对红霉素耐药(ER),11株对红霉素敏感(ES),之前已对这些菌株进行过红霉素耐药性与进入人呼吸道细胞能力之间关联的研究。从RD2区域PCR分析获得的扩增子显示RD2重复次数为1至5次,其中4次(n = 30)最为常见,其次是3次(n = 27)和1次(n = 18)。通过结合RD2区域的PCR分析以及用限制性内切酶HaeIII、DdeI和HinfI对PCR产物进行限制性分析,开发了一种对细胞侵袭性GAS进行分型的新方法(RD2分型)。总体而言,区分出了10种RD2类型(a至j)(所有类型在66株ER分离株中均有检测到,4种类型在11株ES分离株中检测到)。将RD2分型数据与大环内酯耐药的基因型和表型以及PCR M分型和SmaI宏限制性分析的数据进行比较和关联,使我们能够鉴定出41个不同的克隆(66株ER分离株中有31个,11株ES分离株中有10个)。三个主要克隆占分离株的40%(ER菌株的47%)。一些ES分离株似乎与具有相同RD2类型和emm类型组合的ER分离株有关。虽然同时使用不同的分型方法对于全面研究GAS流行病学至关重要,但RD2分型在对细胞侵袭性GAS进行分型时可能特别有用。

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