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Isolation and biochemical and molecular analyses of a species-specific protein antigen from the gastric pathogen Helicobacter pylori.

机译:胃病原体幽门螺杆菌中物种特异性蛋白抗原的分离生化和分子分析。

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摘要

A protein of Mr 26,000 which was present in large quantities in extracts of cells of Helicobacter pylori was purified to homogeneity by ammonium sulfate precipitation followed by gel filtration and reversed-phase chromatography or anion-exchange chromatography. The protein appeared to be associated with the soluble fraction of the cell, and antibodies raised against the protein were reactive with whole-cell lysates of a variety of H. pylori strains in a simple immunodot blot assay. This reaction was species specific. Protein sequence determination of the amino terminus and internal cyanogen bromide fragments and amino acid composition analysis were performed. An oligonucleotide derived from these data was used to clone a fragment encoding most of the coding sequence. Expression in Escherichia coli was dependent on vector promoters. The DNA sequence of the fragment was determined. DNA probes derived from the cloned fragment hybridized to genomic DNA of all H. pylori strains tested, but not to DNAs of Helicobacter mustelae, Wolinella succinogenes, various Campylobacter species, and a panel of gram-negative enteric bacteria. The apparent uniqueness of this protein may be exploited for the development of species-specific diagnostics for this gastric pathogen.
机译:通过硫酸铵沉淀,凝胶过滤和反相色谱或阴离子交换色谱,将幽门螺杆菌细胞提取物中大量存在的26,000 Mr蛋白质纯化至均质。该蛋白质似乎与细胞的可溶性部分有关,并且在简单的免疫斑点印迹分析中,针对该蛋白质产生的抗体可与多种幽门螺杆菌菌株的全细胞裂解物反应。该反应是物种特异性的。进行了氨基末端和内部溴化氰片段的蛋白质序列测定以及氨基酸组成分析。从这些数据得到的寡核苷酸被用于克隆编码大部分编码序列的片段。在大肠杆菌中的表达取决于载体启动子。确定了片段的DNA序列。源自克隆片段的DNA探针与所有测试的幽门螺杆菌菌株的基因组DNA杂交,但不与芥酸幽门螺杆菌,琥珀酸沃林氏菌,各种弯曲杆菌属和一组革兰氏阴性肠杆菌的DNA杂交。这种蛋白质的表观独特性可用于开发这种胃病原体的物种特异性诊断。

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