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铜绿假单胞菌黏液样菌株的整合宿主因子(IHF)缺陷型突变体的分离及IHF在algD基因表达中作用的评估。

Isolation of an IHF-deficient mutant of a Pseudomonas aeruginosa mucoid isolate and evaluation of the role of IHF in algD gene expression.

作者信息

Delic-Attree I, Toussaint B, Froger A, Willison J C, Vignais P M

机构信息

CEA/Grenoble, Laboratoire de Biochimie Microbienne (CNRS URA 1130 alliée à l'INSERM), France.

出版信息

Microbiology (Reading). 1996 Oct;142 ( Pt 10):2785-93. doi: 10.1099/13500872-142-10-2785.

DOI:10.1099/13500872-142-10-2785
PMID:8885394
Abstract

The role of integration host factor (IHF) in the regulation of alginate synthesis was investigated in a mucoid strain of Pseudomonas aeruginosa (strain CHA) isolated from a cystic fibrosis patient. Escherichia coli strain BL21(DE3) was made IHF-deficient by inactivation of its chromosomal IHF genes, himA and himD, then used as host strain to overproduce P. aeruginosa IHF. The purified recombinant IHF protein was used to determine the affinity of IHF for the two IHF binding sites in the algD promoter. The Kd values were determined to be 130 nM for algD IHF site 2 and about 2 microM for algD IHF site 1. Two IHF-deficient mutants of P. aeruginosa strain CHA were constructed by insertional inactivation of the himA gene, and the activity of the algD promoter was determined using transcriptional fusion with xylE as reporter gene. The expression of algD, the structural gene for GDP-mannose dehydrogenase, was decreased three- to fourfold in the himA mutants under conditions of high salinity and nitrogen limitation. Assays of alginate production by cultures grown on agar plates indicated that the IHF-deficient mutants synthesized 50% less polymer than the mucoid parental strain. These results demonstrate clearly that although IHF is dispensable for alginate production, himA expression is required for full activation of algD expression.

摘要

在从一名囊性纤维化患者分离出的铜绿假单胞菌黏液样菌株(CHA菌株)中,研究了整合宿主因子(IHF)在藻酸盐合成调控中的作用。通过使其染色体IHF基因himA和himD失活,使大肠杆菌BL21(DE3)菌株缺乏IHF,然后用作宿主菌株过量表达铜绿假单胞菌IHF。纯化的重组IHF蛋白用于确定IHF对藻酸盐合成酶基因(algD)启动子中两个IHF结合位点的亲和力。确定algD IHF位点2的解离常数(Kd)值为130 nM,algD IHF位点1约为2 μM。通过himA基因的插入失活构建了铜绿假单胞菌CHA菌株的两个IHF缺陷突变体,并使用木糖操纵子(xylE)作为报告基因的转录融合来确定algD启动子的活性。在高盐度和氮限制条件下,GDP-甘露糖脱氢酶结构基因algD在himA突变体中的表达降低了三到四倍。在琼脂平板上培养的菌株的藻酸盐产量测定表明,IHF缺陷突变体合成的聚合物比黏液样亲本菌株少50%。这些结果清楚地表明,虽然IHF对于藻酸盐生产不是必需的,但himA的表达是algD表达完全激活所必需的。

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