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Genetic and biochemical diversity of ureases of Proteus Providencia and Morganella species isolated from urinary tract infection.

机译:从尿路感染中分离出来的变形杆菌普罗维登西亚和摩根氏菌尿素酶的遗传和生化多样性。

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摘要

Bacterial urease, particularly from Proteus mirabilis, has been implicated as a contributing factor in the formation of urinary and kidney stones, obstruction of urinary catheters, and pyelonephritis. Weekly urine specimens (n = 1,135) from 32 patients, residing at two chronic-care facilities, with urinary catheters in place for greater than or equal to 30 days yielded 5,088 phenotypically and serotypically diverse bacterial isolates at greater than or equal to 10(5) CFU/ml. A total of 86% of specimens contained at least one urease-positive species, and 46% of 3,939 gram-negative bacilli were urease positive. For investigation of genetic relatedness of urease determinants, whole-cell DNA from 50 urease-positive isolates each of Providencia stuartii, Providencia rettgeri, P. mirabilis, Proteus vulgaris, and Morganella morganii were hybridized with a urease gene probe derived from within the urease operon of Providencia stuartii BE2467. The percentage of strains hybridizing with the gene probe was 98 for Providencia stuartii, 100 for Providencia rettgeri, 70 for P. mirabilis, 2 for M. morganii, and 0 for P. vulgaris. Electrophoretic mobilities of ureases from representative isolates revealed nine different patterns among the five species. The urease gene probe hybridized with fragments of HindIII-digested chromosomal DNA from all isolates except M. morganii. Fragment sizes differed between species. Molecular sizes of the enzymes, determined by Sephacryl S-300 chromatography, were found to be 280 kilodaltons (kDa) (P. mirabilis), 323 to 337 kDa (Providencia stuartii, Providencia rettgeri, P. mirabilis, P. vulgaris), 620 kDa (providencia rettgeri), and greater than 700 kDa (M. morganii, Providencia rettgeri). Kms ranged from 0.7 mM urea for M. morganii to 60 mM urea for a P. mirabilis isolate. In general, P. mirabilis ureases demonstrated lower affinities for substrate but hydrolyzed urea at rates 6- to 25-fold faster than did enzymes from other species, which may explain the frequent association of this species with stone formation.
机译:细菌尿素酶,特别是来自变形杆菌的尿素酶,被认为是导致泌尿和肾结石形成,导尿管阻塞和肾盂肾炎的重要因素。来自32个患者的每周尿液标本(n = 1,135),位于两个慢性病护理机构中,并放置导尿管超过或等于30天,产生了5,088个表型和血清型多样的细菌分离株,均大于或等于10(5) )CFU /毫升。共有86%的标本包含至少一种脲酶阳性菌种,而3,939克阴性杆菌中有46%为脲酶阳性。为了研究尿素酶决定簇的遗传相关性,将来自普罗维登斯氏菌,普罗维登斯氏菌,米氏疟原虫,寻常变形杆菌和摩根氏摩根氏菌的50个尿素酶阳性分离株的全细胞DNA与衍生自尿素酶操纵子的尿素酶基因探针杂交。 Providencia stuartii BE2467的产品。与该基因探针杂交的菌株的百分率对于斯氏普罗维登斯氏菌为98,对于瑞氏普罗维登斯氏菌为100,对于奇异假单胞菌为70,摩根摩根氏菌为2,寻常型毕赤酵母为0。来自代表性分离物的脲酶的电泳迁移率揭示了这五个物种中的九种不同模式。尿素酶基因探针与除摩根支原体以外的所有分离物中HindIII消化的染色体DNA片段杂交。物种之间的片段大小不同。通过Sephacryl S-300色谱法测定的酶的分子大小为280道尔顿(kDa)(奇异假单胞菌),323至337 kDa(Providencia stuartii,Providencia rettgeri,P. mirabilis,P.vulgaris),620 kDa(providencia rettgeri)和大于700 kDa(M. Morganii,Providencia rettgeri)。 Kms的范围从用于摩根摩根氏菌的0.7 mM尿素到用于奇异疟原虫分离株的60 mM尿素。通常,奇异毕赤酵母脲酶对底物的亲和力较低,但水解尿素的速率比其他物种的酶快6至25倍,这可能解释了该物种与结石的频繁关联。

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