Analysis of Integrons and Antimicrobial Resistances of Multidrug ResistantEscherichia coliIsolated in Korea

Q4 Immunology and Microbiology Journal of Bacteriology and Virology Pub Date : 2019-12-01 DOI:10.4167/jbv.2019.49.4.176
Yun-Yi Yang, M. Suh
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引用次数: 1

Abstract

©This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/ license/by-nc/3.0/). Antibacterial drugs are one of the most important therapeutic agents of bacterial infections but multidrug resistant Escherichia coli (MDREC) is an increasing problem worldwide. Major resistance mechanism of MDREC is horizontal gene transfer of R plasmids harboring integrons, which the integron integrase (IntI) catalyzes gene cassette insertion and excision through site specific recombination. In this study, resistance profiles of integron harboring E. coli isolated in Korea and the genetic environments of integron gene cassettes were analyzed by PCR and direct sequencing to clarify the mechanisms of spread of integron harboring E. coli. Resistance rates of integron harboring E. coli, including β-lactams, aminoglycosides, and fluoroquinolones and MDR frequencies were significantly higher than that of E. coli without integron (p<0.01). Majority (80%) of integron harboring E. coli showed resistance transfer by conjugation. Most (80%) of E. coli had dfrA17-aadA5 cassette array and PcH1 hybrid promoter; 16.7% of E. coli had dfrA12-orfF-aadA2 cassette array and PcW promoter. The higher prevalence of weak Pc variants among most (96.7%) of integron harboring MDREC suggests that a flexible cassette array is more important than enhanced expression. All the integrons had LexA binding motif suggests that SOS responses control the expression of these integrons. In conclusion, the genetic bases of integrons were diverse, and the spread and the expression of prevalent gene cassette arrays may be deeply related with strengths of Pc promoters in integrons. These informations will provide important knowledge to control the increase of integron harboring MDREC.
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韩国多药耐药大肠杆菌的整合子及耐药性分析
©这是一篇基于知识共享署名非商业许可协议(http://creativecommons.org/ License /by-nc/3.0/)的开放获取文章。抗菌药物是治疗细菌感染最重要的药物之一,但耐多药大肠杆菌(MDREC)是一个日益严重的世界性问题。MDREC的主要耐药机制是携带整合子的R质粒的水平基因转移,整合子整合酶(IntI)通过位点特异性重组催化基因盒的插入和切除。本研究采用PCR和直接测序的方法,分析了韩国分离的含整合子大肠杆菌的耐药谱和整合子基因盒的遗传环境,以阐明含整合子大肠杆菌的传播机制。含整合子的大肠杆菌对β-内酰胺类、氨基糖苷类、氟喹诺酮类药物的耐药率和耐多药频次均显著高于未含整合子的大肠杆菌(p<0.01)。大多数(80%)携带整合子的大肠杆菌通过偶联转移抗性。大多数(80%)大肠杆菌具有dfrA17-aadA5盒式阵列和PcH1杂交启动子;16.7%的大肠杆菌含有dfrA12-orfF-aadA2盒式阵列和PcW启动子。在大多数(96.7%)携带MDREC的整合子中,弱Pc变体的患病率较高,这表明灵活的盒式阵列比增强表达更重要。所有整合子都含有LexA结合基序,表明SOS应答控制了这些整合子的表达。综上所述,整合子的遗传基础是多样的,普遍基因盒阵列的传播和表达可能与整合子中Pc启动子的强度密切相关。这些信息将为控制携带MDREC的整合子的增加提供重要的知识。
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来源期刊
Journal of Bacteriology and Virology
Journal of Bacteriology and Virology Immunology and Microbiology-Immunology
CiteScore
0.80
自引率
0.00%
发文量
16
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