首页> 外文OA文献 >Analysis of Involvement of the RecF Pathway in p44 Recombination in Anaplasma phagocytophilum and in Escherichia coli by Using a Plasmid Carrying the p44 Expression and p44 Donor Loci
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Analysis of Involvement of the RecF Pathway in p44 Recombination in Anaplasma phagocytophilum and in Escherichia coli by Using a Plasmid Carrying the p44 Expression and p44 Donor Loci

机译:使用携带p44表达和p44供体基因座的质粒分析recF途径参与噬菌体和大肠杆菌中p44重组的过程

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摘要

Anaplasma phagocytophilum, the etiologic agent of human granulocytic anaplasmosis, has a large paralog cluster (approximate 90 members) that encodes the 44-kDa major outer membrane proteins (P44s). Gene conversion at a single p44 expression locus leads to P44 antigenic variation. Homologs of genes for the RecA-dependent RecF pathway, but not the RecBCD or RecE pathways, of recombination were detected in the A. phagocytophilum genome. In the present study, we examined whether the RecF pathway is involved in p44 gene conversion. The recombination intermediate structure between a donor p44 and the p44 expression locus of A. phagocytophilum was detected in an HL-60 cell culture by Southern blot analysis followed by sequencing the band and in blood samples from infected SCID mice by PCR, followed by sequencing. The sequences were consistent with the RecF pathway recombination: a half-crossover structure, consisting of the donor p44 locus connected to the 3′ conserved region of the recipient p44 in the p44 expression locus in direct orientation. To determine whether the p44 recombination intermediate structure can be generated in a RecF-active Escherichia coli strain, we constructed a double-origin plasmid carrying the p44 expression locus and a donor p44 locus and introduced the plasmid into various E. coli strains. The recombination intermediate was recovered in an E. coli strain with active RecF recombination pathway but not in strains with deficient RecF pathway. Our results support the view that the p44 gene conversion in A. phagocytophilum occurs through the RecF pathway.
机译:吞噬细胞无浆膜,人类粒细胞无形体病的病原体,具有较大的旁系同源簇(约90个成员),编码44kDa主要外膜蛋白(P44s)。在单个p44表达位点的基因转换导致P44抗原变异。在噬菌嗜热链球菌基因组中检测到了RecA依赖的RecF途径的重组基因的同源物,但未检测到RecBCD或RecE途径的重组基因。在本研究中,我们检查了RecF途径是否参与p44基因转化。通过Southern印迹分析在HL-60细胞培养物中检测供体p44和嗜血曲霉p44表达基因座之间的重组中间结构,然后对该条带进行测序,并通过PCR对感染的SCID小鼠的血样进行测序,然后进行测序。该序列与RecF途径重组一致:半交叉结构,其由供体p44基因座直接连接至p44表达基因座中受体p44的3'保守区组成。为了确定是否可以在具有RecF活性的大肠杆菌菌株中产生p44重组中间结构,我们构建了一个带有p44表达基因座和供体p44基因座的双源质粒,并将该质粒引入到各种大肠杆菌菌株中。在具有有效RecF重组途径的大肠杆菌菌株中回收了重组中间体,但是在具有不足RecF途径的菌株中未回收到重组中间体。我们的结果支持这样的观点,即嗜血曲霉中的p44基因转化是通过RecF途径发生的。

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