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Functional characterization of VC1929 of Vibrio cholerae El Tor: role in mannose-sensitive haemagglutination, virulence and utilization of sialic acid

机译:Vibrio Cholerae Elor VC1929的功能表征:在甘露糖敏感血凝中的作用,唾液酸的毒力和利用

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The nonadhesive mutant CD11 of Vibrio cholerae El Tor, defective in expression of mannose-sensitive haemagglutinin, lacks a protein when compared with its parent strain. Determination of the amino acid sequence revealed the identity of the protein as the product of VC1929, which is annotated to encode a protein, DctP, involved in the transport of C4-dicarboxylates. We cloned the dctP gene in pUC19 vector and expressed it in mutant CD11. Expression of DctP in the resulting complemented strain restored virulence, adhesive and colonizing capabilities, mannose-sensitive haemagglutination (MSHA) and ability to grow in medium containing sialic acid as a sole carbon source. The mutation in CD11 was caused by insertion of an adenine nucleotide in the reading frame of dctP. Recombinant purified DctP protein showed MSHA of human red blood cells, and protected rabbits against infection by V. cholerae. The protein was localized in membrane and cell wall fractions. The mutant, recombinant CD11 expressing DctP and parent strains were grown in M9 minimal medium in the presence of various carbohydrates (glucose, malate, fumarate, succinate or N-acetylneuraminic acid). The mutant was unable to grow in minimal medium containing N-acetylneuraminic acid (sialic acid) as the sole carbon source whereas the recombinant and parent strains utilized all the sugars tested. It is concluded that DctP is a mannose-sensitive haemagglutinin and a virulence factor and is involved in the utilization of sialic acid.
机译:与其亲本菌株相比,vibrio霍乱E11的vibrio choleraeL的突变体CD11缺乏缺乏蛋白质。氨基酸序列的测定揭示了蛋白质作为VC1929的产物的蛋白质,其注释为编码蛋白质,DCTP,涉及C4二羧酸酯的转运。我们克隆了PUC19载体中的DCTP基因,并在突变体CD11中表达。 DCTP在由此产生的互补菌株中的表达恢复了毒力,粘合剂和定植能力,甘露糖敏感性血凝(MSHA)和含唾液酸中培养基的能力作为唯一的碳源。 CD11中的突变是通过在DCTP的读数框中插入腺嘌呤核苷酸引起的。重组纯化的DCTP蛋白显示人红细胞MSHA,并受到V.Cholerae的影响免受感染的兔。蛋白质局部化为膜和细胞壁级分。在各种碳水化合物(葡萄糖,苹果酸盐,富马酸盐,琥珀酸盐或N-乙酰氨酸)存在下,在M9最小培养基中生长突变体,表达DCTP和亲本菌株的突变体,在M9最小培养基中生长。突变体不能在含有N-乙酰氨基葡萄酸(唾液酸)的最小培养基中,作为唯一的碳源,而重组和亲本菌株使用所有测试的糖。得出结论,DCTP是甘露糖敏感的血凝素和毒力因子,并且参与利用唾液酸。

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