首页> 外文OA文献 >Detection of gyrA and gyrB mutations in quinolone-resistant clinical isolates of Escherichia coli by single-strand conformational polymorphism analysis and determination of levels of resistance conferred by two different single gyrA mutations.
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Detection of gyrA and gyrB mutations in quinolone-resistant clinical isolates of Escherichia coli by single-strand conformational polymorphism analysis and determination of levels of resistance conferred by two different single gyrA mutations.

机译:通过单链构象多态性分析检测喹诺酮耐药的临床大肠杆菌中的gyrA和gyrB突变,并确定两个不同的单个gyrA突变赋予的耐药水平。

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摘要

Twelve quinolone-resistant clinical isolates of Escherichia coli (nalidixic acid MICs, 64 to 512 micrograms/ml; norfloxacin MICs, 0.25 to 8 micrograms/ml) were transformed with plasmid pJSW101 carrying the gyrA+ gene and with plasmid pJB11 carrying the gyrB+ gene to examine the proportion of gyrA and gyrB mutations. Transformation with pJSW101 resulted in complementation (nalidixic acid MICs, 4 to 32 micrograms/ml; norfloxacin MICs, 0.06 to 0.25 micrograms/ml). In contrast, no change in MICs were observed after transformation with pJB11. A 418-bp fragment of gyrA from the 12 strains was amplified by PCR. Direct DNA sequencing of that fragment identified the causes of quinolone resistance in eight strains as a single point mutation leading to a substitution of the serine at position 83 (Ser-83) to Leu and in four strains as a single point mutation leading to a substitution of Asp-87 to Gly. Exchange of the fragment from one of these strains with that of gyrA+ and transformation of resistance with the hybrid gyrA plasmid indicated the contribution of Gly-87 to resistance and the stabilities of mutants containing GyrA (Gly-87). Thus, gyrA gene mutations are probably encountered more often than gyrB gene mutations in clinical isolates of E. coli. In addition, the substitution of Asp-87 to Gly can be encountered in such strains. On the basis of the level of resistance found in the fragment exchange experiment, the quinolone resistance attributable to Gly-87 appears to be comparable to that attributable to Leu-83. The levels of resistance found in the clinical isolates shown to have a Gly-87 mutation (nalidixic acid MICs, 64 to 512 micrograms/ml; norfloxacin MICs, 0.5 to 4 micrograms/ml) suggest that the Gly-87 mutation causes resistance at the level of the nalidixic acid MIC (64 micrograms/ml) or the norfloxacin MIC (0.5 micrograms/ml or less) and that the additional increments in resistance seen in the other strains with higher levels of resistance may be attributable to additional mutations. The single-strand conformational polymorphism analysis with PCR products readily detected te Leu-83 and Gly-87 mutations.
机译:用携带gyrA +基因的质粒pJSW101和携带gyrB +基因的质粒pJB11转化12株对喹诺酮耐药的大肠杆菌临床菌株(纳西地酸MIC,64至512微克/毫升;诺氟沙星MIC,0.25至8微克/毫升)。 gyrA和gyrB突变的比例。用pJSW101进行转化可产生互补作用(萘啶酸MIC为4至32微克/毫升;诺氟沙星MIC为0.06至0.25微克/毫升)。相反,用pJB11转化后未观察到MIC变化。通过PCR扩增了来自12个菌株的gyrA的418bp的片段。该片段的直接DNA测序确定了八株菌株中喹诺酮耐药的原因是单点突变,导致将83位(Ser-83)的丝氨酸替换为Leu;四株菌株中,喹诺酮抗性是单点突变,导致了替换Asp-87转给Gly。这些菌株之一的片段与gyrA +的片段交换以及杂种gyrA质粒的抗性转化表明Gly-87对抗性的贡献以及含有GyrA的突变体(Gly-87)的稳定性。因此,在大肠杆菌的临床分离物中,gyrA基因突变可能比gyrB基因突变更常见。另外,在这种菌株中可以遇到Asp-87向Gly的取代。根据片段交换实验中发现的耐药水平,归因于Gly-87的喹诺酮耐药性似乎与归因于Leu-83的喹诺酮耐药性相当。在临床分离株中发现的抗性水平显示具有Gly-87突变(萘啶酸MIC,64至512微克/毫升;诺氟沙星MIC,0.5至4微克/毫升),表明Gly-87突变会引起Gly-87突变。萘啶酸MIC(64微克/毫升)或诺氟沙星MIC(0.5微克/毫升或更低)的水平,以及在其他具有较高抗性水平的菌株中发现的抗性额外增加可能归因于其他突变。用PCR产物进行的单链构象多态性分析很容易检测到Leu-83和Gly-87突变。

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