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首页> 外文期刊>Acta Biochimica Polonica >Nucleotide substitutions in the Candida albicans ERG11 gene of azole-susceptible and azole-resistant clinical isolates
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Nucleotide substitutions in the Candida albicans ERG11 gene of azole-susceptible and azole-resistant clinical isolates

机译:唑敏感和耐唑临床分离株的白色念珠菌ERG11基因中的核苷酸取代

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One of the mechanisms of Candida albicans resistance to azole drugs used in antifungal therapy relies on increased expression and presence of point mutations in the ERG11 gene that encodes sterol 14α demethylase (14DM), an enzyme which is the primary target for the azole class of antifungals. The aim of the study was to analyze nucleotide substitutions in the Candida albicans ERG11 gene of azole-susceptible and azole-resistant clinical isolates. The Candida albicans isolates represented a collection of 122 strains selected from 658 strains isolated from different biological materials. Samples were obtained from hospitalized patients. Fluconazole susceptibility was tested in vitro using a microdilution assay. Candida albicans strains used in this study consisted of two groups: 61 of the isolates were susceptible to azoles and the 61 were resistant to azoles. Four overlapping regions of the ERG11 gene of the isolates of Candida albicans strains were amplified and sequenced. The MSSCP (multitemperature single strand conformation polymorphism) method was performed to select Candida albicans samples presenting genetic differences in the ERG11 gene fragments for subsequent sequence analysis. Based on the sequencing results we managed to detect 19 substitutions of nucleotides in the ERG11 gene fragments. Sequencing revealed 4 different alterations: T495A, A530C, G622A and A945C leading to changes in the corresponding amino acid sequence: D116E, K128T, V159I and E266D. The single nucleotide changes in the ERG11 gene did not affect the sensitivity of Candida albicans strains, whereas multiple nucleotide substitutions in the ERG11 gene fragments indicated a possible relation with the increase in resistance to azole drugs.
机译:白色念珠菌对用于抗真菌治疗的唑类药物具有抗药性的机制之一依赖于编码固醇14α脱甲基酶(14DM)的ERG11基因的表达增加和点突变的存在,该酶是唑类抗真菌剂的主要靶标。该研究的目的是分析对吡咯敏感和对吡咯耐药的临床分离株的白色念珠菌ERG11基因的核苷酸取代。白色念珠菌分离物代表122种菌株的集合,该菌株选自从不同生物材料中分离的658种菌株。样本来自住院患者。使用微量稀释测定法在体外测试氟康唑的药敏性。这项研究中使用的白色念珠菌菌株包括两组:其中的61株对唑类敏感,而61株对唑类有抗性。扩增了白色念珠菌菌株的ERG11基因的四个重叠区域并进行了测序。进行了MSSCP(多温度单链构象多态性)方法,以选择在ERG11基因片段中存在遗传差异的白色念珠菌样品,用于后续序列分析。根据测序结果,我们设法检测到ERG11基因片段中19个核苷酸的取代。测序揭示了4种不同的变化:T495A,A530C,G622A和A945C导致相应氨基酸序列的变化:D116E,K128T,V159I和E266D。 ERG11基因中的单个核苷酸变化不会影响白色念珠菌菌株的敏感性,而ERG11基因片段中的多个核苷酸取代表明与对唑类药物的耐药性增加可能相关。

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