抗菌药物耐药性和碲酸钾(PT)在医院环境中的传播:碲酸钾的使用手段和插入序列的检测是否有助于预防和干预?

B. D. O. Fonseca, Verônica Dias Gonçalves, Gabriela Alves de Souza, Melissa Vianna Henriques, Renata de Meirelles Santos Pereira, A. Bello, J. Pereira
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引用次数: 0

摘要

多药耐药性是一个公共卫生问题。肠杆菌科菌株可能是抗菌和碲酸钾(PT)抗性基因的储存库,这是细菌逃逸到吞噬细胞内杀死机制的决定因素。抗性基因的迁移及其基因重排与这些基因的传播密切相关。整合子和转座子等移动遗传元件,以及IS26(被认为是主要的ISs之一),促进了质粒中抗性基因集的形成和动员,这些抗性和毒力决定因素能够水平转移。有证据表明,在质粒中,编码黏附素、毒素和抗菌素耐药性的基因存在关联,可能与PT耐药性有关。在目前的工作中,在巴西里约热内卢里约热内卢大学医院的不同单位(医院厨房、内科和外科诊所病房以及重症监护病房)收集了342份样本进行细菌培养:98份来自专业人员的手样本,85份来自食品处理人员的手样本,104份来自患者的粪便样本(直肠拭子)和55份食物样本。采用含有头孢菌素(32µg/mL)的选择性培养基分离27株肠杆菌科细菌。采用常规表型方法进行细菌鉴定。采用纸片扩散法进行抗菌药敏试验和广谱β -内酰胺酶(ESBLs)产生的表型试验。在25µg/mL和112µg/mL的培养基上直接播种,检测其PT抗性。质粒通过琼脂糖凝胶电泳对细菌DNA提取物进行可视化。此外,采用PCR法检测耐药基因和IS26。从27株分离的肠杆菌科菌株中,考虑到ESBLs产生的表型、对氨基糖苷类的耐药性以及高分子量和低分子量质粒的存在(来自食品处理人员的手、食物和住院患者的粪便),选择了8株肠杆菌科菌株。3株3/8(37.5%)同时对氨基糖苷类和头孢菌素耐药。4株4/8菌株(50.0%)产生ESBL表型试验阳性,6株6/8菌株(75.0%)产生PT抗性。对氨基糖苷类耐药和产生ESBL的菌株均有基因扩增产物。我们认为这些抗菌素耐药基因,也是对PT(细菌毒力因子)和IS26耐药的决定因素,可能有助于R质粒在不同环境中的可塑性和适应性,有利于相关致病菌株的循环。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Dissemination of antimicrobial resistance and Potassium Tellurite (PT) in the hospital environment: can the use of means with Tellurite and the detection of insertion sequences contribute to prevention and intervention?
Multidrug resistance is a public health problem. Enterobacteriaceae strains may be reservoirs of antimicrobial and potassium tellurite (PT) resistance genes, which is a determinant of bacterial escape to intraphagocytic killing mechanisms. The mobility of resistance genes and their genetic rearrangements are significantly involved in the dissemination of these genes. Mobile genetic elements such as integrons and transposons, as well as IS26 (considered among the predominant ISs), facilitate the formation and mobilization of sets of resistance genes in plasmids capable of transferring these determinants of resistance and virulence horizontally. There is evidence of associations, in plasmids, of genes encoding adhesins, toxins and antimicrobial resistance, possibly related to PT resistance. In the present work, 342 samples were collected for bacteriological culture in different units of a University Hospital in Rio de Janeiro, Brazil (Hospital Kitchen, Medical and Surgical Clinics Wards, and Intensive Care Unit): 98 samples from hands of professionals, 85 hand samples from food handlers, 104 stool samples (rectal swab) from patients and 55 food samples. We isolated 27 strains of Enterobacteriaceae through selective media containing cephalothin (32µg/mL). Bacterial identification was performed by conventional phenotypic methods. Antimicrobial susceptibility tests, as well as the phenotypic test for Extended-Spectrum Beta-lactamases (ESBLs) production, were performed by disk diffusion. PT resistance was also tested by direct seeding in media with 25µg/mL and 112 µg/mL of the compound. Plasmids were visualized by agarose gel electrophoresis of bacterial DNA extracts. Additionally, antimicrobial resistance genes and IS26 were detected by PCR assays. From a total of 27 strains of Enterobacteriaceae isolated, eight strains of Enterobacteriaceae were selected, considering phenotypes indicative of ESBLs production, resistance to aminoglycosides and presence of plasmids of high and low molecular weight (from the hands of food handlers, food and feces from hospitalized patients).  Three strains 3/8 (37.5%) were resistant to aminoglycosides and cephalosporins, concomitantly. Four 4/8 strains (50.0%) were positive for the phenotypic test for ESBL production and six 6/8 strains (75.0%) were resistant to PT. Strains with resistance to aminoglycosides and producing ESBL showed amplification product for the genes tested. We consider that these antimicrobial resistance genes, also the determinants for resistance to PT (as a bacterial virulence factor), as well as IS26, may contribute to the plasticity and fitness of R plasmids, in different environments, favoring the circulation of relevant pathogenic strains.
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