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花生根瘤菌类菌体氢酶的分离提纯及特性
引用本文:黄南仲,许良树,张凤章,龙敏南.花生根瘤菌类菌体氢酶的分离提纯及特性[J].植物生理与分子生物学学报,1995(1).
作者姓名:黄南仲  许良树  张凤章  龙敏南
作者单位:厦门大学生物学系
摘    要:花生根瘤菌类菌体经超声波破碎,TritonX-100溶解,正已烷-硫酸铵处理后,再经DEAE-纤维素和Sephacryl凝胶柱层析等纯化步骤,获得凝胶电泳纯的膜结合态氢酶,比活为71.4μmolH2mg-1Protmin-1,为类菌体吸H2活性的211倍。纯化的氢酶分子量为110kD。经SDS-PAGE后,呈现两个蛋白带,分子量分利为65kD和35kD。纯酶的Ni含量为0.62molNi/mol氢酶。在磷酸缓冲液中其活性的最适pH为6.5。DCIP、亚甲蓝、铁氰化钾、细胞色素C均可作为氢酶的电子受体,其中以DCIP为最适。

关 键 词:花生,类菌体,氨酶,提纯,特性

Purification and Some Properties of the Membrane-Bound Hydrogenase from the Bacteroids of Peanut Root Nodules
HUANG Nan-Zhong, XU Liang-Shu,ZHANG Feng-Zhang and LONG Min-Nan.Purification and Some Properties of the Membrane-Bound Hydrogenase from the Bacteroids of Peanut Root Nodules[J].Journal Of Plant Physiology and Molecular Biology,1995(1).
Authors:HUANG Nan-Zhong  XU Liang-Shu  ZHANG Feng-Zhang and LONG Min-Nan
Abstract:The H2-uptake hydrogenase fromthe bacteroids of peanut nodules hasbeen purified and characterized. Bacteroids were prepared, then broken bysonication. The membrane-bound hydrogenase was solubilized by treatmentwith Triton X-100 and followed byammonium sulfate-he-cane extractionto remove lipids and detergent.. Thehydrogenase was further purified byDEAE-cellulars column chromatography, eluted with Tris-HCl buffer containing NaCl 0. 3 mol/L and GenapolX-080 0. 2%. The enzyme was purified to homogeneity by runningSephacryl H200 column chromatogtaphy twice. The specific activity was71. 4 pmol H2 oxidiZed Per mg proteinper mid and was incrsased 211 foldsrelative to that in hacteroids. Themolecular weisht of native enzyme wasabout 1 10 kD as determined by PAGEin undenatured form. SDS-PAGEShowed two bands with molecularweight of 65 kD and 35 kD, indicatingthat the membrane-bound hydsogenasewas an a, 6 dimer. The nickel contentof purified hydrogenase was found tobe 0. 62 mole Ni/mol hydrogenase.The optimum PH for the activity of thepurified enzyme was found to be near6. 5 in potassium phosphate buffer.Suitable electron acceptors are DCIP,methylene blue, ferricyanide and CytC. The best one is DCIP. Benzyl viologen, methyl viologen and NAD werealmost not reduced.
Keywords:penut  bacteroid  hydrogenase  purification  properties  
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