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从以乙酸盐为生长底物的嗜热嗜甲烷菌中分离出一种含有类咕啉和镍且具有一氧化碳脱氢酶活性的酶复合物。

Isolation of an enzyme complex with carbon monoxide dehydrogenase activity containing corrinoid and nickel from acetate-grown Methanosarcina thermophila.

作者信息

Terlesky K C, Nelson M J, Ferry J G

出版信息

J Bacteriol. 1986 Dec;168(3):1053-8. doi: 10.1128/jb.168.3.1053-1058.1986.

Abstract

Fast protein liquid chromatography of cell extract from methanol- or acetate-grown Methanosarcina thermophila resolved two peaks of CO dehydrogenase activity. The activity of one of the CO dehydrogenases was sixfold greater in acetate-grown compared with methanol-grown cells. This CO dehydrogenase was purified to apparent homogeneity (70 mumol of methyl viologen reduced per min per mg of protein) and made up greater than 10% of the cellular protein of acetate-grown cells. The native enzyme (Mr 250,000) formed aggregates with an Mr of approximately 1,000,000. The enzyme contained five subunits (Mrs 89,000, 71,000, 60,000, 58,000, and 19,000), suggesting a multifunctional enzyme complex. Nickel, iron, cobalt, zinc, inorganic sulfide, and a corrinoid were present in the complex. The UV-visible spectrum suggested the presence of iron-sulfur centers. The electron paramagnetic resonance spectrum contained g values of 2.073, 2.049, and 2.028; these features were broadened in enzyme that was purified from cells grown in the presence of medium enriched with 61Ni, indicating the involvement of this metal in the spectrum. The pattern of potassium cyanide inhibition indicated that cyanide binds at or near the CO binding site. The properties of the enzyme imply an involvement in the dissimilation of acetate to methane, possibly by cleavage of acetate or activated acetate.

摘要

对嗜热甲烷八叠球菌甲醇或乙酸盐培养物的细胞提取物进行快速蛋白质液相色谱分析,分离出两个一氧化碳脱氢酶活性峰。与甲醇培养的细胞相比,乙酸盐培养的细胞中一种一氧化碳脱氢酶的活性高6倍。这种一氧化碳脱氢酶被纯化至表观均一(每毫克蛋白质每分钟还原70微摩尔甲基紫精),在乙酸盐培养的细胞中占细胞蛋白质的10%以上。天然酶(Mr 250,000)形成了Mr约为1,000,000的聚集体。该酶含有五个亚基(Mr分别为89,000、71,000、60,000、58,000和19,000),表明是一种多功能酶复合物。该复合物中存在镍、铁、钴、锌、无机硫化物和类咕啉。紫外可见光谱表明存在铁硫中心。电子顺磁共振光谱的g值为2.073、2.049和2.028;在从富含61Ni的培养基中生长的细胞中纯化的酶中,这些特征变宽,表明这种金属参与了光谱。氰化钾抑制模式表明氰化物在一氧化碳结合位点或其附近结合。该酶的特性表明它可能参与乙酸盐向甲烷的异化作用,可能是通过乙酸盐或活化乙酸盐的裂解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c53f/213601/2d352c43c455/jbacter00205-0015-a.jpg

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