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作 者:肖克林[1] 王中兴[2] 周天祥[2] 麦光兴[1] 王秦宁 孔繁荣[3]
机构地区:[1]深圳市宝安区妇幼保健院中心实验室,518133 [2]深圳市宝安区妇幼保健院检验科,518133 [3]悉尼大学Westmead医院感染性疾病和微生物中心
出 处:《中华传染病杂志》2016年第2期111-114,共4页Chinese Journal of Infectious Diseases
基 金:广东省科技计划项目公益研究与能力建设专项资金(2014A020212703);广东省医学科研基金(A2015142)
摘 要:目的建立艰难梭菌数字化PCR-核糖体分型方法及常见基因型的参考图谱。方法利用荧光毛细管电泳技术代替琼脂糖凝胶电泳检测艰难梭菌PCR-核糖体分型产物,建立数字化PCR-核糖体分型方法;利用40株分属于10种核糖体型(RT)的艰难梭菌参考菌株构建常见基因型的数字化参考图谱。结果荧光毛细管电泳技术准确地检测出40株艰难梭菌参考菌株的PCR-核糖体分型片段,并以数字化的形式呈现,10种核糖体型艰难梭菌的PCR-核糖体分型数字化图谱差异明显。同为RT027的21株菌株间、RT002的3株菌株间和RT015的2株菌株间的数字化分型结果相似性都非常高,而7株RT001菌株则可分为4种亚型,2株RT014分为2种亚型。结论成功建立艰难梭菌数字化PCR-核糖体分型方法,同时构建了艰难梭菌10种核糖体型的数字化PCR-核糖体分型参考数据库。Objective To develop a digital polymerase chain reaction (PCR)-rihotyping method and database for Clostridiurn difficile genotyping. Methods Sequencer based fluorescence capillary gel electrophoresis was used, instead of agarose gel electrophoresis, to establish the digital PCR-ribotyping of Clostridium difficile. Forty Clostridium difficile reference strains, consisting of 10 PCR-ribotypes (RT), were genotyped by the new digital PCR-rihotyping method to set-up the database. Results The sequencer based fluorescence capillary gel electrophoresis correctly detected PCR-ribotyping products of the 40 reference strains, and showed as digital figure; significant differences of these digital figures were found between the 10 RT. High similar digital figures were shown in twenty-one RT027 strains, three RT002 strains and two RT014 strains. However, seven RT001 strains were typed as four subtypes, and two RT014 strains as two subtypes, respectively. Conclusion A digital PCR-ribotyping, and a reference database consisting of 10 RT are successfully established.
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