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小肠结肠炎耶尔森菌的磷脂酶A在小鼠模型中参与致病过程。

Phospholipase A of Yersinia enterocolitica contributes to pathogenesis in a mouse model.

作者信息

Schmiel D H, Wagar E, Karamanou L, Weeks D, Miller V L

机构信息

Department of Microbiology and Molecular Genetics, University of California, Los Angeles, CA 90095, USA.

出版信息

Infect Immun. 1998 Aug;66(8):3941-51. doi: 10.1128/IAI.66.8.3941-3951.1998.

Abstract

Some isolates of Yersinia enterocolitica exhibit phospholipase activity, which has been linked to lecithin-dependent hemolysis (M. Tsubokura, K. Otsoki, I. Shimohira, and H. Yamamoto, Infect. Immun. 25:939-942, 1979). A gene encoding Y. enterocolitica phospholipase was identified, and analysis of the nucleotide sequence revealed two tandemly transcribed open reading frames. The first, yplA, has 74% identity and 85% similarity to the phospholipase A found in Serratia liquefaciens. Though the other, yplB, was less similar to the downstream accessory protein found in S. liquefaciens, the organization in both species is similar. Subsequently, a yplA-null Y. enterocolitica strain, YEDS10, was constructed and demonstrated to be phospholipase negative by plate and spectrophotometric assays. To ascertain whether the phospholipase has a role in pathogenesis, YEDS10 was tested in the mouse model. In experiments with perorally infected BALB/c mice, fewer YEDS10 organisms were recovered from the mesenteric lymph nodes and Peyer's patches (PP) than the parental strain at 3 or 5 days postinfection. Furthermore, bowel tissue and PP infected with YEDS10 appeared to be less inflamed than those infected with the parental strain. When extremely high doses of both the parental and YEDS10 strains were given, similar numbers of viable bacteria were recovered from the PP and mesenteric lymph nodes on day 3. However, the numbers of foci and the extent of inflammation and necrosis within them were noticeably less for YEDS10 compared to the parental strain. Together these findings suggest that Y. enterocolitica produces a phospholipase A which has a role in pathogenesis.

摘要

一些小肠结肠炎耶尔森菌分离株表现出磷脂酶活性,这与卵磷脂依赖性溶血有关(M. Tsubokura、K. Otsoki、I. Shimohira和H. Yamamoto,《感染与免疫》25:939 - 942,1979年)。一个编码小肠结肠炎耶尔森菌磷脂酶的基因被鉴定出来,对核苷酸序列的分析揭示了两个串联转录的开放阅读框。第一个是yplA,与在液化沙雷氏菌中发现的磷脂酶A有74%的同一性和85%的相似性。虽然另一个yplB与液化沙雷氏菌中发现的下游辅助蛋白的相似性较低,但两个物种中的基因组织是相似的。随后,构建了一个yplA基因缺失的小肠结肠炎耶尔森菌菌株YEDS10,并通过平板和分光光度法测定证明其为磷脂酶阴性。为了确定磷脂酶在发病机制中是否起作用,在小鼠模型中对YEDS10进行了测试。在对经口感染的BALB/c小鼠进行的实验中,在感染后3天或5天,从肠系膜淋巴结和派尔集合淋巴结(PP)中回收的YEDS10菌株比亲代菌株少。此外,感染YEDS10的肠组织和PP似乎比感染亲代菌株的炎症轻。当给予极高剂量的亲代菌株和YEDS10菌株时,在第3天从PP和肠系膜淋巴结中回收的活菌数量相似。然而,与亲代菌株相比,YEDS10的病灶数量以及其中的炎症和坏死程度明显较少。这些发现共同表明,小肠结肠炎耶尔森菌产生一种在发病机制中起作用的磷脂酶A。

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