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从嗜热栖热放线菌中分离和重组含铁和锰的超氧化物歧化酶。

Isolation and reconstitution of iron- and manganese-containing superoxide dismutases from Bacteroides thetaiotaomicron.

作者信息

Pennington C D, Gregory E M

出版信息

J Bacteriol. 1986 May;166(2):528-32. doi: 10.1128/jb.166.2.528-532.1986.

Abstract

Superoxide dismutase (SOD) from extracts of anaerobically maintained Bacteroides thetaiotaomicron was a dimer of equally sized 23,000-molecular-weight monomers joined noncovalently. A preparation with a specific activity of 1,200 U/mg contained 1.1 g-atom of Fe, 0.6 g-atom of Zn, and less than 0.05 g-atom of Mn per mol of dimer. The apoprotein, prepared by dialysis of iron-SOD in 5 M guanidinium chloride-20 mM 8-hydroxyquinoline, had no superoxide-scavenging activity when renatured without exogenous metal. Enzymatic activity was restored to the denatured apoprotein by dialysis against either 1 mM Fe(NH4)2 or 1 mM MnCl2 in 20 mM Tris (pH 7.0). The Fe-reconstituted enzyme and the native enzyme were inhibited approximately 50% by 0.2 mM NaN3, whereas the Mn-reconstituted enzyme was inhibited 60% by 10 mM NaN3. Aeration of the anaerobic cells resulted in a fourfold induction of an azide-resistant SOD. The enzyme (43,000 molecular weight) isolated from aerated cells was a dimer of equally sized subunits. The metal content was 1.0 g-atom of Mn, 0.55 g-atom of Fe, and 0.3 g-atom of Zn per mol of dimer. Enzymatic activity of the denatured apoprotein from this enzyme was also restored on addition of either iron or manganese. The constitutive Fe-SOD and the O2-induced Mn-SOD, tested alone and in combination, migrated identically on acrylamide gels, had similar amino acid compositions, and had alanine as the sole N-terminal amino acid. These data are consistent with the synthesis of a single apoprotein in either anaerobically maintained or oxygenated cells. We have observed a similar phenomenon with SOD from Bacteroides fragilis (E. M. Gregory, Arch. Biochem. Biophys. 238:83-89, 1985).

摘要

在厌氧条件下培养的多形拟杆菌提取物中的超氧化物歧化酶(SOD)是由两个分子量均为23,000的单体通过非共价键结合而成的二聚体。每摩尔二聚体中,比活性为1200 U/mg的制剂含有1.1克原子的铁、0.6克原子的锌和少于0.05克原子的锰。通过在5 M氯化胍 - 20 mM 8 - 羟基喹啉中对铁 - SOD进行透析制备的脱辅基蛋白,在没有外源金属的情况下复性时没有超氧化物清除活性。通过在20 mM Tris(pH 7.0)中用1 mM Fe(NH4)2或1 mM MnCl2进行透析,可使变性的脱辅基蛋白恢复酶活性。铁重构酶和天然酶被0.2 mM叠氮化钠抑制约50%,而锰重构酶被10 mM叠氮化钠抑制60%。对厌氧细胞进行通气导致一种抗叠氮化物SOD的四倍诱导。从通气细胞中分离出的酶(分子量43,000)是由大小相同的亚基组成的二聚体。每摩尔二聚体的金属含量为1.0克原子的锰、0.55克原子的铁和0.3克原子的锌。加入铁或锰后,该酶变性脱辅基蛋白的酶活性也得以恢复。单独测试和联合测试时,组成型铁 - SOD和氧气诱导的锰 - SOD在丙烯酰胺凝胶上迁移情况相同,氨基酸组成相似,且唯一的N端氨基酸均为丙氨酸。这些数据与在厌氧培养或充氧细胞中合成单一脱辅基蛋白一致。我们在脆弱拟杆菌的SOD中也观察到了类似现象(E. M. Gregory,《生物化学与生物物理学报》238:83 - 89,1985)。

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