首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Rapid screening of point mutations of the Neisseria gonorrhoeae parC gene associated with resistance to quinolones.
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Rapid screening of point mutations of the Neisseria gonorrhoeae parC gene associated with resistance to quinolones.

机译:快速筛选淋病奈瑟氏球菌parC基因与喹诺酮类药物耐药相关的点突变。

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摘要

To detect quinolone resistance-associated mutations within the Asp-86, Ser-87, Ser-88, and Glu-91 codons of the Neisseria gonorrhoeae parC gene, we developed a rapid and simple assay based on amplification of the regions of the parC gene containing the mutations sites by PCR and digestion of the PCR products with restriction enzymes. By using the method of primer-specified restriction site modification, artificial SalI, PstI, EcoRI, and HinfI restriction sites were created in the regions containing the Asp-86, Ser-87, Ser-88, and Glu-91 codons, respectively. The mutations generating alterations at Asp-86, Ser-87, Ser-88, and Glu-91 were detected as failures of SalI, PstI, EcoRI, and HinfI to digest the respective PCR products. Fifty-five clinical strains of N. gonorrhoeae were examined for mutations in the parC gene by this assay. Appropriate mutations at either the Asp-86, Ser-87, Ser-88, or Glu-91 codon were detected in each of 11 strains in which a mutation had previously been observed by DNA sequencing. This rapid and simple assay could be a useful device for screening genetic alterations in the parC gene associated with resistance to quinolones in N. gonorrhoeae.
机译:为了检测淋病奈瑟氏球菌parC基因的Asp-86,Ser-87,Ser-88和Glu-91密码子中的喹诺酮抗性相关突变,我们基于parC基因区域的扩增,开发了一种快速简单的测定方法通过PCR含有突变位点,并用限制酶消化PCR产物。通过使用引物指定的限制性位点修饰方法,分别在包含Asp-86,Ser-87,Ser-88和Glu-91密码子的区域中创建了人工SalI,PstI,EcoRI和HinfI限制性位点。检测到在Asp-86,Ser-87,Ser-88和Glu-91处产生突变的突变是SalI,PstI,EcoRI和HinfI消化相应PCR产物的失败。通过该测定法检查了55个淋病奈瑟氏球菌临床菌株中parC基因的突变。在11株以前通过DNA测序已观察到突变的菌株中,均检测到Asp-86,Ser-87,Ser-88或Glu-91密码子的适当突变。这种快速,简单的测定方法可能是筛选parC基因中与淋病奈瑟菌对喹诺酮类药物耐药相关的遗传变化的有用装置。

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