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FosA13的特性鉴定,FosA13是在家禽分离株中鉴定出的一种新型磷霉素谷胱甘肽转移酶。

Characterization of FosA13, a novel fosfomycin glutathione transferase identified in a isolate from poultry.

作者信息

Zhang Runzhi, Yu Yan, Huang Lulu, Chen Susu, Hu Ruxi, Wang Xiuxiu, Huang Dawei, Song Chunhan, Lu Junwan, Bao Qiyu, Hu Yunliang, Jiang Pengfei, Pan Wei

机构信息

Institute of Molecular Virology and Immunology, Department of Microbiology and Immunology, School of Basic Medical Sciences, Wenzhou Medical University, Wenzhou, China.

Institute of Biomedical Informatics/School of Laboratory Medicine and Life Sciences, Wenzhou Medical University, Wenzhou, China.

出版信息

Front Cell Infect Microbiol. 2025 Mar 11;15:1534084. doi: 10.3389/fcimb.2025.1534084. eCollection 2025.

Abstract

BACKGROUND

is a species of the genus in the family . This species primarily causes infections of postoperative wounds and the urinary tract. Some isolates of exhibit resistance to multiple antibiotics due to multidrug resistance traits, complicating clinical treatment; thus, there is a growing need to elucidate the resistance mechanisms of this pathogen.

METHODS

A total of 658 bacterial strains were isolated from anal fecal swabs from poultry and livestock and from the surrounding environment in Wenzhou, China, via plate streaking. The full genome sequences of the bacteria were obtained via next-generation sequencing platforms. The standard agar dilution method was employed to determine the minimum inhibitory concentrations (MICs) of various antimicrobial agents. The resistance gene () of the isolate was identified using the Comprehensive Antibiotic Resistance Database (CARD) and confirmed via molecular cloning. The FosA13 protein encoded by the novel resistance gene was expressed with the vector pCold I, and its enzyme kinetics parameters were characterized. The genetic background and evolutionary process of the sequence of this novel resistance gene were analyzed by means of bioinformatics methods.

RESULTS

In this study, we identified a new chromosomally encoded fosfomycin resistance gene, designated , from the isolate DW0548, which was isolated from poultry on a farm in Wenzhou, China. Compared with the control strain (pUCP19/DH5α), the recombinant strain carrying (pUCP19-/DH5α) presented a fourfold increase in the MIC value for fosfomycin. The enzyme kinetics data of FosA13 revealed effective inactivation of fosfomycin, with a of (1.50 ± 0.02)×10 M·s. Among functionally characterized resistance proteins, FosA13 presented the highest amino acid (aa) homology (55.6%) with FosA. FosA13 also contained essential functional residues of FosA proteins. The isolate DW0548 presented high MIC values (≥ 8 μg/mL) for 5 classes of antimicrobials, namely, aminoglycosides, β-lactams, quinolones, tetracycline, and chloramphenicol, but only two functionally characteristic antimicrobial resistance genes (ARGs) have been identified in the complete genome: a β-lactam resistance gene ( ) and a phenol resistance gene (). These findings indicate that in addition to the novel resistance gene identified in this work, other uncharacterized resistance mechanisms might exist in DW0548.

CONCLUSION

A novel chromosomal fosfomycin resistance gene, , was identified in an animal isolate, and its enzymatic parameters were characterized. This protein shares the highest aa identity of 55.6% with the functionally characterized protein FosA and has all the essential functional residues of FosA proteins. Exploring more antimicrobial resistance mechanisms of this pathogen would help clinicians choose effective drugs to treat infectious diseases in animal husbandry and clinical practice and facilitate the development of methods to prevent the spread of resistance between bacteria of different species.

摘要

背景

[细菌名称]是[科名]中[属名]的一个物种。该物种主要引起术后伤口感染和尿路感染。由于多重耐药特性,[细菌名称]的一些分离株对多种抗生素表现出耐药性,使临床治疗复杂化;因此,越来越需要阐明这种病原体的耐药机制。

方法

通过平板划线法,从中国温州的家禽和家畜的肛门粪便拭子以及周围环境中总共分离出658株细菌菌株。通过下一代测序平台获得细菌的全基因组序列。采用标准琼脂稀释法测定各种抗菌剂的最低抑菌浓度(MIC)。使用综合抗生素抗性数据库(CARD)鉴定分离株的抗性基因([基因名称]),并通过分子克隆进行确认。由新抗性基因[基因名称]编码的FosA13蛋白用载体pCold I表达,并对其酶动力学参数进行表征。通过生物信息学方法分析该新抗性基因序列的遗传背景和进化过程。

结果

在本研究中,我们从中国温州一个农场的家禽中分离出的[细菌名称]分离株DW0548中鉴定出一个新的染色体编码的磷霉素抗性基因,命名为[基因名称]。与对照菌株(pUCP19/DH5α)相比,携带[基因名称]的重组菌株(pUCP19 - /DH5α)对磷霉素的MIC值增加了四倍。FosA13的酶动力学数据显示磷霉素有效失活,[催化常数]为(1.50±0.02)×10[单位]M·s。在功能表征的抗性蛋白中,FosA13与FosA的氨基酸(aa)同源性最高(55.6%)。FosA13还包含FosA蛋白的必需功能残基。分离株DW0548对5类抗菌剂,即氨基糖苷类、β-内酰胺类、喹诺酮类、四环素类和氯霉素,表现出高MIC值(≥8μg/mL),但在完整基因组中仅鉴定出两个功能特征性抗菌抗性基因(ARG):一个β-内酰胺抗性基因([基因名称])和一个苯酚抗性基因([基因名称])。这些发现表明,除了本研究中鉴定的新抗性基因外,DW0548中可能还存在其他未表征的抗性机制。

结论

在动物[细菌名称]分离株中鉴定出一个新的染色体磷霉素抗性基因[基因名称],并对其酶学参数进行了表征。该蛋白与功能表征的蛋白FosA的氨基酸同一性最高为55.6%,并具有FosA蛋白的所有必需功能残基。探索该病原体更多的抗菌抗性机制将有助于临床医生选择有效的药物来治疗畜牧业和临床实践中的传染病,并促进预防不同物种细菌之间抗性传播方法的开发。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/85fd/11933065/93a300c40b3f/fcimb-15-1534084-g001.jpg

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