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Identification and classification of Oxalobacter formigenes strains by using oligonucleotide probes and primers.

机译:通过使用寡核苷酸探针和引物鉴定和鉴定富氧草酸杆菌菌株。

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Genomic DNAs of various strains of Oxalobacter formigenes were subjected to restriction endonuclease fragment length polymorphism- and PCR-based amplification analyses with DNA probes and primers complementary to sequences within either the oxc gene, encoding oxalyl coenzyme A (oxalyl-CoA) decarboxylase, or the frc gene, encoding formyl-CoA transferase. Oligonucleotide probes based on nonconserved sequences of oxc or frc were able to divide O. formigenes strains into at least two groups, consistent with the current separation of O. formigenes strains into groups I and II on the basis of 16S rRNA sequence similarities and lipid content. In contrast, an oligonucleotide probe based on the conserved 5' end of oxc appeared to bind all group I and the majority of group II strains. PCR amplification of the oxc gene showed even greater sensitivity in detecting O. formigenes and provided support for further division of the strains into subgroups. In addition, these oligonucleotides failed to hybridize to or amplify PCR products from whole fecal DNA isolated from fresh stool samples from an individual not colonized with O. formigenes, indicating unique specificity. Thus, these DNA analyses permit both detection as well as classification of O. formigenes strains.
机译:用限制性内切核酸酶片段长度多态性和PCR扩增分析各种菌株的草酸变形杆菌基因组DNA,并使用与oxc基因内编码草酰辅酶A(oxalyl-CoA)脱羧酶的序列互补的DNA探针和引物frc基因,编码甲酰基-CoA转移酶。基于oxc或frc的非保守序列的寡核苷酸探针能够将O.formigenes菌株分为至少两组,这与当前基于16S rRNA序列相似性和脂质含量将O.formigenes菌株分为I组和II组一致。 。相比之下,基于oxc保守5'端的寡核苷酸探针似乎结合了所有I型菌株和大多数II型菌株。 oxc基因的PCR扩增显示了检测O. formigenes的更高灵敏度,并为进一步将菌株分为亚组提供了支持。另外,这些寡核苷酸不能与未从富集O.formigenes的个体新鲜粪便样品分离得到的整个粪便DNA杂交或扩增PCR产物,表明独特的特异性。因此,这些DNA分析既可以检测也可以鉴定产气荚膜曲霉菌株。

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