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亚基相互作用增强了通过His标签重组蛋白方法纯化的甘薯胞质铜/锌超氧化物歧化酶的酶活性和稳定性。

Subunit interaction enhances enzyme activity and stability of sweet potato cytosolic Cu/Zn-superoxide dismutase purified by a His-tagged recombinant protein method.

作者信息

Lin C T, Lin M T, Chen Y T, Shaw J F

机构信息

Institute of Marine Biotechnology, National Taiwan Ocean University, Keelung.

出版信息

Plant Mol Biol. 1995 May;28(2):303-11. doi: 10.1007/BF00020249.

DOI:10.1007/BF00020249
PMID:7599315
Abstract

The coding region of copper/zinc-superoxide dismutase (Cu/Zn-SOD) cDNA from sweet potato, Ipomoea batatas (L.) Lam. cv. Tainong 57, was introduced into an expression vector, pET-20b(+). The Cu/Zn-SOD purified by His-tagged technique showed two active forms (dimer and monomer). The amount of proteins of dimer and monomer appeared to be equal, but the activity of dimeric form was seven times higher than that of monomeric form. The enzyme was dissociated into monomer by imidazole buffer above 1.0 M, acidic pH (below 3.0), or SDS (above 1%). The enzyme is quite stable. The enzyme activity is not affected at 85 degrees C for 20 min, in alkali pH 11.2, or in 0.1 M EDTA and also quite resistant to proteolytic attack. Dimer is more stable than monomer. The thermal inactivation rate constant kd calculated for the monomer at 85 degrees C was 0.029 min-1 and the half-life for inactivation was about 28 min. In contrast, there is no significant change of dimer activity after 40 min at 85 degrees C. The enzyme dimer and monomer retained 83% and 58% of original activity, respectively, after 3 h incubation with trypsin at 37 degrees C, while those retained 100% and 31% of original activity with chymotrypsin under the same condition. These results suggest subunit interaction might change the enzyme conformation and greatly improve the catalytic activity and stability of the enzyme. It is also possible that the intersubunit contacts stabilize a particular optimal conformation of the protein or the dimeric structure enhances catalytic activity by increasing the electrostatic steering of substrate into the active site.

摘要

将甘薯(Ipomoea batatas (L.) Lam. cv. Tainong 57)铜/锌超氧化物歧化酶(Cu/Zn-SOD)cDNA的编码区导入表达载体pET-20b(+)。通过His标签技术纯化的Cu/Zn-SOD呈现出两种活性形式(二聚体和单体)。二聚体和单体的蛋白量似乎相等,但二聚体形式的活性比单体形式高7倍。该酶在1.0 M以上的咪唑缓冲液、酸性pH(低于3.0)或SDS(高于1%)作用下会解离成单体。该酶相当稳定。在85℃下20分钟、碱性pH 11.2或0.1 M EDTA条件下,酶活性不受影响,并且对蛋白水解攻击也相当抗性。二聚体比单体更稳定。在85℃下计算得到的单体热失活速率常数kd为0.029 min-1,失活半衰期约为28分钟。相比之下,二聚体在85℃下40分钟后活性没有显著变化。在37℃下与胰蛋白酶孵育3小时后,酶二聚体和单体分别保留了83%和58%的原始活性,而在相同条件下与胰凝乳蛋白酶孵育时,它们分别保留了100%和31%的原始活性。这些结果表明亚基相互作用可能会改变酶的构象并极大地提高酶的催化活性和稳定性。也有可能亚基间的接触稳定了蛋白质的特定最佳构象,或者二聚体结构通过增加底物向活性位点的静电导向来增强催化活性。

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