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Molecular cloning and sequence analysis of the gene encoding LipL41 a surface-exposed lipoprotein of pathogenic Leptospira species.

机译:编码LipL41(致病性钩端螺旋体物种的表面暴露的脂蛋白)的基因的分子克隆和序列分析。

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摘要

We report the cloning of the gene encoding a surface-exposed leptospiral lipoprotein, designated LipL41. In a previous study, a 41-kDa protein antigen was identified on the surface of Leptospira kirschneri (D. A. Haake, E. M. Walker, D. R. Blanco, C. A. Bolin, J. N. Miller, and M. A. Lovett, Infect. Immun. 59:1131-1140, 1991). We obtained the N-terminal amino acid sequence of a staphylococcal V8 proteolytic-digest fragment in order to design an oligonucleotide probe.A Lambda ZAP II library containing EcoRI fragments of L. kirschneri DNA was screened, and a 2.3-kb DNA fragment which contained the entire structural lipL41 gene was identified. The deduced amino acid sequence of LipL41 would encode a 355-amino-acid polypeptide with a 19-amino-acid signal peptide, followed by an L-X-Y-C lipoprotein signal peptidase cleavage site. A recombinant His6-LipL41 fusion protein was expressed in Escherichia coli in order to generate specific rabbit antiserum. LipL41 is solubilized by Triton X-114 extraction of L. kirschneri; phase separation results in partitioning of LipL41 exclusively into the detergent phase. At least eight proteins, including LipL41 and the other major Triton X-114 detergent phase proteins, are intrinsically labeled during incubation of L. kirschneri in media containing [3H] palmitate. Processing of LipL41 is inhibited by globomycin, a selective inhibitor of lipoprotein signal peptidase. Triton X-100 extracts of L. kirschneri contain immunoprecipitable OmpL1 (porin), LipL41, and another lipoprotein, LipL36. However, in contrast to LipL36, only LipL41 and OmpL1 were exposed on the surface of intact organisms. Immunoblot analysis of a panel of Leptospira species reveals that LipL41 expression is highly conserved among leptospiral pathogens.
机译:我们报告了编码表面暴露的钩端螺旋体脂蛋白命名为LipL41的基因的克隆。在先前的研究中,在克氏钩端螺旋体的表面鉴定出41 kDa的蛋白质抗原(DA Haake,EM Walker,DR Blanco,CA Bolin,JN Miller和MA Lovett,Infect。Immun。59:1131-1140,1991)。 )。为了设计寡核苷酸探针,我们获得了葡萄球菌V8蛋白水解消化片段的N末端氨基酸序列。一个Lambda ZAP II文库包含了柯氏乳酸杆菌DNA的EcoRI片段,并筛选了一个2.3kb的DNA片段。鉴定了完整的lipL41结构基因。 LipL41的推导氨基酸序列将编码一个具有19个氨基酸信号肽的355个氨基酸多肽,然后是L-X-Y-C脂蛋白信号肽酶切割位点。为了产生特异性的兔抗血清,重组His6-LipL41融合蛋白在大肠杆菌中表达。 LipTri41通过Triton X-114提取柯氏乳杆菌溶解。相分离导致LipL41仅分配到去污剂相中。在含有[3H]棕榈酸酯的培养基中培养柯氏乳杆菌期间,至少对8种蛋白质(包括LipL41和其他主要的Triton X-114去污剂相蛋白质)进行了内在标记。 LipL41的加工受到球蛋白(脂蛋白信号肽酶的选择性抑制剂)的抑制。 Kirschneri的Triton X-100提取物含有可免疫沉淀的OmpL1(孔蛋白),LipL41和另一种脂蛋白,LipL36。但是,与LipL36相比,只有LipL41和OmpL1暴露在完整生物的表面上。一组钩端螺旋体物种的免疫印迹分析表明,LipL41的表达在钩端螺旋体病原体中高度保守。

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