首页> 美国卫生研究院文献>Journal of Bacteriology >Involvement of a Protein Tyrosine Kinase in Production of the Polymeric Bioemulsifier Emulsan from the Oil-Degrading Strain Acinetobacter lwoffii RAG-1
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Involvement of a Protein Tyrosine Kinase in Production of the Polymeric Bioemulsifier Emulsan from the Oil-Degrading Strain Acinetobacter lwoffii RAG-1

机译:蛋白质酪氨酸激酶参与产油降解菌株lwoffii RAG-1聚合生物乳化剂Emulsan的生产。

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摘要

The genes associated with the biosynthesis of the polymeric bioemulsifier emulsan, produced by the oil-degrading Acinetobacter lwoffii RAG-1 are clustered within a 27-kbp region termed the wee cluster. This report demonstrates the involvement of two genes of the wee cluster of RAG-1, wzb and wzc, in emulsan biosynthesis. The two gene products, Wzc and Wzb were overexpressed and purified. Wzc exhibited ATP-dependent autophosphorylating protein tyrosine kinase activity. Wzb was found to be a protein tyrosine phosphatase capable of dephosphorylating the phosphorylated Wzc. Using the synthetic substrate p-nitrophenyl phosphate (PNPP) Wzb exhibited a Vmax of 12 μmol of PNPP min−1 mg−1 and a Km of 8 mM PNPP at 30°C. The emulsifying activity of mutants lacking either wzb or wzc was 16 and 15% of RAG-1 activity, respectively, suggesting a role for the two enzymes in emulsan production. Phosphorylation of Wzc was found to occur within a cluster of five tyrosine residues at the C terminus. Colonies from a mutant in which these five tyrosine residues were replaced by five phenylalanine residues along with those of a second mutant, which also lacked Wzb, exhibited a highly viscous colony consistency. Emulsan activity of these mutants was 25 and 24% of that of RAG-1, respectively. Neither of these mutants contained cell-associated emulsan. However, they did produce an extracellular high-molecular-mass galactosamine-containing polysaccharide. A model is proposed in which subunit polymerization, translocation and release of emulsan are all associated and coregulated by tyrosine phosphorylation.
机译:由油降解的不动杆菌伊瓦菲RAG-1产生的与聚合生物乳化剂乳桑酸的生物合成相关的基因聚集在称为wee簇的27kbp区域内。该报告证明了RAG-1的wee簇的两个基因wzb和wzc参与了乳桑生物合成。 Wzc和Wzb这两个基因产物被过表达和纯化。 Wzc表现出ATP依赖的自磷酸化蛋白酪氨酸激酶活性。发现Wzb是一种能够使磷酸化的Wzc去磷酸化的蛋白质酪氨酸磷酸酶。使用合成的磷酸对硝基苯酯(PNPP),Wzb在30°时的Vmax为12μmolPNPP min -1 mg -1 ,Km为8 mM PNPP C。缺乏wzb或wzc的突变体的乳化活性分别为RAG-1活性的16%和15%,表明这两种酶在乳油生产中的作用。发现Wzc的磷酸化发生在C端的五个酪氨酸残基簇中。来自其中五个酪氨酸残基被五个苯丙氨酸残基替换的突变体的菌落,以及同样缺乏Wzb的第二个突变体的菌落,显示出高粘性的菌落稠度。这些突变体的Emulsan活性分别是RAG-1的25%和24%。这些突变体均不包含细胞相关的乳胶。但是,它们确实产生了细胞外的含半乳糖胺的高分子多糖。提出了一个模型,其中酪氨酸磷酸化使亚单位的聚合,易位和释放均与乳化有关。

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