首页> 美国政府科技报告 >Identification and Characterization of a Gene Cluster Mediating EnteroaggregativeEscherichia Coli Aggregative Adherence Fimbria I Biogenesis. (Reannouncement with New Availability Information)
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Identification and Characterization of a Gene Cluster Mediating EnteroaggregativeEscherichia Coli Aggregative Adherence Fimbria I Biogenesis. (Reannouncement with New Availability Information)

机译:鉴定和表征介导肠聚集性大肠杆菌聚集体粘附Fimbria I生物发生的基因簇。 (重新公布新的可用性信息)

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The aggregative pattern of adherence (AA) exhibited by enteroaggregativeEscherichia coli upon HEp-2 cells is a plasmid-associated property which correlates with aggregative adherence fimbria I (AAF/I) expression and human erythrocyte hemagglutination. By using cloning and mutagenesis strategies, two noncontinguous plasmid segments (designated regions 1 and 2) required for AA expression have previously been identified in enteroaggregative E. coli 17-2. TnphoA mutagenesis was performed on clones containing region 1, and 16 TnphoA mutants which were negative for the AA phenotype were analyzed. The TnphoA insertion site for each mutant was determined by junctional DNA sequencing. All 16 mutations occurred within a 4.6-kb span in region 1. Nucleotide sequence analysis of the region revealed four contiguous open reading frames, designated aggDCBA, in the same span. AA-negative TnphoA insertions into all open reading frames except aggB were obtained. On the basis of mutational analysis and protein homology data, it is inferred that aggA, aggC, and aggD are involved in biogenesis of AAF/I, encoding a major fimbrial subunit, outer membrane usher, and periplasmic fimbrial chaperone, respectively. By immunogold electron microscopy, polyclonal antiserum raised against the aggA gene product decorated AAF/I fimbriae, affirming that AggA encodes an AAF/I subunit.

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