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耐碳青霉烯类肺炎克雷伯菌临床分离株中多粘菌素耐药机制的遗传多样性:一项中国的多中心研究

Genetic Diversity of Polymyxin-Resistance Mechanisms in Clinical Isolates of Carbapenem-Resistant Klebsiella pneumoniae: a Multicenter Study in China.

作者信息

Li Ziyao, Liu Xinmeng, Lei Zichen, Li Chen, Zhang Feilong, Wu Yongli, Yang Xinrui, Zhao Jiankang, Zhang Yulin, Hu Yanning, Shen Fangfang, Wang Pingbang, Yang Junwen, Liu Yulei, Lu Binghuai

机构信息

China-Japan Friendship Institute of Clinical Medical Sciences, Beijing, China.

Laboratory of Clinical Microbiology and Infectious Diseases, Department of Pulmonary and Critical Care Medicine, Center of Respiratory Medicine, National Clinical Research Center for Respiratory Diseases, National Center for Respiratory Medicine, China-Japan Friendship Hospital, Beijing, China.

出版信息

Microbiol Spectr. 2023 Feb 27;11(2):e0523122. doi: 10.1128/spectrum.05231-22.

Abstract

Polymyxin has been the last resort to treat multidrug-resistant Klebsiella pneumonia. However, recent studies have revealed that polymyxin-resistant carbapenem-resistant Klebsiella pneumonia (PR-CRKP) emerged due to the mutations in chromosomal genes or the plasmid-harboring gene, leading to lipopolysaccharide modification or efflux of polymyxin through pumps. Further surveillance was required. In the present study we collected PR-CRKP strains from 8 hospitals in 6 provinces/cities across China to identify the carbapenemase and polymyxin resistance genes and epidemiological features by whole-genome sequencing (WGS). The broth microdilution method (BMD) was performed to determine the MIC of polymyxin. Of 662 nonduplicate CRKP strains, 15.26% (101/662) were defined as PR-CRKP; 10 (9.90%) were confirmed as Klebsiella quasipneumoniae by WGS. The strains were further classified into 21 individual sequence types (STs) by using multilocus sequence typing (MLST), with ST11 being prevalent (68/101, 67.33%). Five carbapenemase types were identified among 92 CR-PRKP, (66.67%), (16.83%), (0.99%), (4.95%), and (0.99%). Notably, 2 PR-CRKP strains harbored both and . The inactivation of , associated significantly with high-level polymyxin resistance, was mainly caused by the insertion sequence (IS) insertion (62.96%, 17/27). Furthermore, was inserted coincidently by IS (67/101, 66.33%). The deletion or splicing mutations of were significantly associated with ST11 and KL47 (capsule locus types), and diverse mutations of the gene were identified. Only one strain carried the gene. In summary, the high IS-inserted inactivation, the close relationship between ST11 and the deletion or splicing mutations of the , and the specific features of PR- constituted notable features of our PR-CRKP strains in China. Polymyxin-resistant CRKP is a serious public health threat whose resistance mechanisms should be under continuous surveillance. Here, we collected 662 nonduplicate CRKP strains across China to identify the carbapenemase and polymyxin resistance genes and epidemiological features. Polymyxin resistance mechanism in 101 PR-CRKP strains in China were also investigated, 9.8% of which (10/101) were , as determined via WGS, and inactivation of remained the most crucial polymyxin resistance mechanism, significantly related to high-level resistance. Deletion or splicing mutations of were significantly associated with ST11 and KL47. Diverse mutations of the gene were identified. The plasmid complementation experiment and mRNA expression analysis further confirmed that the promoter and played a critical role in polymyxin resistance. This multicenter study contributed to the understanding of antibiotic resistance forms in China.

摘要

多粘菌素一直是治疗多重耐药肺炎克雷伯菌的最后手段。然而,最近的研究表明,由于染色体基因或携带质粒的基因突变,导致脂多糖修饰或多粘菌素通过泵流出,从而出现了对多粘菌素耐药的耐碳青霉烯类肺炎克雷伯菌(PR-CRKP)。需要进一步监测。在本研究中,我们从中国6个省/市的8家医院收集了PR-CRKP菌株,通过全基因组测序(WGS)来鉴定碳青霉烯酶和多粘菌素耐药基因以及流行病学特征。采用肉汤微量稀释法(BMD)测定多粘菌素的最低抑菌浓度(MIC)。在662株非重复的CRKP菌株中,15.26%(101/662)被定义为PR-CRKP;通过WGS确认10株(9.90%)为准肺炎克雷伯菌。使用多位点序列分型(MLST)将这些菌株进一步分为21个单倍型序列类型(STs),其中ST11最为常见(68/101,67.33%)。在92株CR-PRKP中鉴定出5种碳青霉烯酶类型,分别为(66.67%)、(16.83%)、(0.99%)、(4.95%)和(0.99%)。值得注意的是,2株PR-CRKP菌株同时携带和。与高水平多粘菌素耐药显著相关的的失活,主要是由插入序列(IS)插入引起的(62.96%,17/27)。此外,(67/101,66.33%)也被IS巧合插入。的缺失或剪接突变与ST11和KL47(荚膜位点类型)显著相关,并且鉴定出了基因的多种突变。只有1株携带基因。总之,高比例的IS插入导致失活、ST11与的缺失或剪接突变之间的密切关系以及PR-的特定特征构成了我国PR-CRKP菌株的显著特点。耐多粘菌素CRKP是一种严重的公共卫生威胁,其耐药机制应持续监测。在此,我们收集了全国662株非重复的CRKP菌株,以鉴定碳青霉烯酶和多粘菌素耐药基因以及流行病学特征。我们还研究了中国101株PR-CRKP菌株的多粘菌素耐药机制,通过WGS确定其中9.8%(10/101)为,并且的失活仍然是最关键的多粘菌素耐药机制,与高水平耐药显著相关。基因的缺失或剪接突变与ST11和KL47显著相关。鉴定出了基因的多种突变。质粒互补实验和mRNA表达分析进一步证实,启动子和在多粘菌素耐药中起关键作用。这项多中心研究有助于了解中国的抗生素耐药形式。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fffd/10100843/2025a9370d33/spectrum.05231-22-f001.jpg

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