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酿酒酵母中粪卟啉原氧化酶的纯化及性质

Purification and properties of coproporphyrinogen oxidase from the yeast Saccharomyces cerevisiae.

作者信息

Camadro J M, Chambon H, Jolles J, Labbe P

出版信息

Eur J Biochem. 1986 May 2;156(3):579-87. doi: 10.1111/j.1432-1033.1986.tb09617.x.

Abstract

Coproporphyrinogen oxidase has been located in the cytosol of yeast cells. The enzyme was purified to homogeneity from a heme mutant strain exhibiting a high specific activity (15-20 enzyme units/mg soluble protein compared to 1-2 enzyme units/mg soluble protein of by the wild-type strain). The final preparation was homogeneous as judged by sodium dodecyl sulfate/polyacrylamide gel electrophoresis (Mr = 35,000) and isoelectrofocusing (pI = 6.2). Gel filtration on AcA 44 gave a relative molecular mass of 70,000. N-terminal amino-acid sequence analysis revealed a single polypeptide chain. Thus the enzyme appears to be a dimer with identical subunits. Two iron atoms/molecule of native protein were detected; they could not be removed by exhaustive dialysis or gel filtration on Sephadex G-25. However the involvement of the iron atoms in the oxidative catalytic activity of the enzyme was not demonstrated. The Km value for coproporphyrinogen was 0.05 microM. The enzyme was active only when molecular oxygen was used as electron acceptor; no anaerobic activity could be detected. Thiol-directed reagents partially inhibited the enzyme, indicating that an SH group is required for activity. Yeast coproporphyrinogen oxidase was activated by phospholipids or neutral detergents as described for the bovine liver enzyme.

摘要

粪卟啉原氧化酶定位于酵母细胞的胞质溶胶中。该酶从一个表现出高比活性的血红素突变株中纯化至同质(野生型菌株的比活性为1 - 2酶单位/毫克可溶性蛋白,而该突变株为15 - 20酶单位/毫克可溶性蛋白)。通过十二烷基硫酸钠/聚丙烯酰胺凝胶电泳(Mr = 35,000)和等电聚焦(pI = 6.2)判断,最终制剂是同质的。在AcA 44上进行凝胶过滤得到的相对分子质量为70,000。N端氨基酸序列分析显示为单条多肽链。因此,该酶似乎是由相同亚基组成的二聚体。检测到天然蛋白质分子中有两个铁原子;通过彻底透析或在Sephadex G - 25上进行凝胶过滤都无法去除它们。然而,尚未证明铁原子参与该酶的氧化催化活性。粪卟啉原的Km值为0.05微摩尔。该酶仅在以分子氧作为电子受体时才有活性;未检测到厌氧活性。硫醇导向试剂部分抑制该酶,表明活性需要一个SH基团。如对牛肝酶所描述的那样,酵母粪卟啉原氧化酶被磷脂或中性去污剂激活。

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