首页> 外文期刊>Archives of microbiology >Alteration of flagellar phenotype of Escherichia coli strain P12b, the standard type strain for flagellar antigen H17, possessing a new non-fliC flagellin gene flnA, and possible loss of original flagellar phenotype and genotype in the course of subculturing through semisolid media.
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Alteration of flagellar phenotype of Escherichia coli strain P12b, the standard type strain for flagellar antigen H17, possessing a new non-fliC flagellin gene flnA, and possible loss of original flagellar phenotype and genotype in the course of subculturing through semisolid media.

机译:大肠杆菌P12b鞭毛表型的改变,鞭毛抗原H17的标准型菌株,具有新的非fliC鞭毛蛋白基因flnA,并且在通过半固体培养基传代培养的过程中可能会失去原始鞭毛表型和基因型。

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摘要

A practically important phenomenon, resulting in the loss of the original flagellar phenotype (genotype) of bacteria, is described in the Escherichia coli H17 type strain P12b possessing two distinct genes for H17 and H4 flagellins, respectively. By PCR, sequencing, and phylogenetic investigation, the H17 gene (originally expressed) was considered a new non-fliC flagellin gene and assigned flnA, while the H4 gene (originally cryptic) was reaffirmed as fliC. H17 and H4 flagella differed morphologically. The phenomenon consisted in the replacement of H17 cells by H4 cells during subculturing through certain semisolid media and resulted from the excision of flnA (H17) entirely or in part. The substitution rate depended on the density and nutrient composition of media and reached 100% even after a single passage through 0.3% LB agar. Such phenomenon can lead to an unexpected loss of original H17 phenotype. Our review of the literature showed that the loss of the original flagellar genotype (phenotype) of P12b has occurred in some laboratories while the authors continued to consider their cultures H17. We showed how to distinguish these alternative flagellin genotypes using popular fliC primers. Attention was also paid to possible discrepancies between serological and molecular results in flagellar typing of E. coli.
机译:在大肠杆菌H17型菌株P12b中描述了一种实际上重要的现象,该现象导致细菌的原始鞭毛表型(基因型)丧失,该菌株分别具有两个针对H17和H4鞭毛蛋白的基因。通过PCR,测序和系统发育研究,H17基因(最初表达)被认为是新的非fliC鞭毛蛋白基因,并被分配为flnA,而H4基因(最初为隐性)被确认为fliC。 H17和H4鞭毛形态上有所不同。该现象包括在通过某些半固体培养基传代培养过程中,H4细胞替代了H17细胞,这是由于flnA(H17)的全部或部分切除所致。取代率取决于培养基的密度和营养成分,甚至在单次通过0.3%LB琼脂后仍达到100%。这种现象可能会导致原始H17表型的意外损失。我们对文献的回顾表明,在一些实验室中,P12b原始鞭毛基因型(表型)的丧失已经发生,而作者继续考虑他们的文化H17。我们展示了如何使用流行的fliC引物区分这些替代鞭毛蛋白基因型。还应注意大肠杆菌鞭毛分型中血清学和分子结果之间可能存在的差异。

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