首页> 美国卫生研究院文献>Biochemical Journal >Regulation of aortic CuZn-superoxide dismutase with copper. Caeruloplasmin and albumin re-activate and transfer copper to the enzyme in culture.
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Regulation of aortic CuZn-superoxide dismutase with copper. Caeruloplasmin and albumin re-activate and transfer copper to the enzyme in culture.

机译:用铜调节主动脉CuZn-超氧化物歧化酶。铜蓝蛋白和白蛋白重新活化并将铜转移到培养物中的酶中。

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摘要

Caeruloplasmin and albumin were compared as potential donors of copper to Cu2Zn2-superoxide dismutase (CuZn-SOD) in culture. Aortas from 15-day copper-deficient chicks were suspended in oxygenated, serum-free, Waymouth medium (752/1) for 24 h. SOD activity was restored when the medium was supplemented with CuCl2, a copper-albumin complex or caeruloplasmin, all present at a level equivalent to 5 microM-copper. Activation did not occur at 4 degrees C or with Cu-EDTA as the supplement. Mn2+ and Zn2+, alone or in combination, did not activate nor enhance the activation achieved by CuCl2. The activation with CuCl2 was not inhibited by cycloheximide or cordycepin. [67Cu]Caeruloplasmin and albumin when added to the medium transferred radioactive copper to at least three cytosolic protein fractions, one of which was determined by immunoprecipitation to be CuZn-SOD. The transfer of 67Cu from caeruloplasmin was inhibited by increasing amounts of unlabelled caeruloplasmin; disodium EDTA (1.0 mM) had no effect on the transfer of copper from caeruloplasmin. These data show that aortic SOD activity, suppressed in copper deficiency, can be restored by incubating the aortas in culture medium supplemented with copper salts. In this system, caeruloplasmin and Cu-albumin appear equally capable of activating aortic CuZn-SOD. Moreover, the transfer of copper into the enzyme structure appears to be the primary event restoring catalytic activity to the enzyme.
机译:比较了铜绿蛋白和白蛋白作为铜在培养物中对Cu2Zn2-超氧化物歧化酶(CuZn-SOD)的潜在供体。将来自15天缺铜小鸡的主动脉悬浮在无氧,氧化的Waymouth培养基(752/1)中24小时。当向培养基中添加CuCl2,铜-白蛋白复合物或铜蓝蛋白时,其SOD活性得以恢复,它们的含量均相当于5 microM-铜。在4摄氏度或使用Cu-EDTA作为补充剂时未发生活化。单独或组合使用的Mn2 +和Zn2 +不会激活也不会增强CuCl2所实现的激活。 CuCl 2的活化不受环己酰亚胺或虫草素的抑制。 [67Cu] Caeruloplasmin和白蛋白添加到培养基中时,会将放射性铜转移到至少三个胞质蛋白组分中,其中之一通过免疫沉淀法确定为CuZn-SOD。通过增加未标记的铜蓝蛋白的量抑制了67Cu从铜蓝蛋白的转移。 EDTA钠(1.0 mM)对铜从铜蓝蛋白的转移没有影响。这些数据表明,通过在添加了铜盐的培养基中培养主动脉,可以恢复被铜缺乏抑制的主动脉SOD活性。在该系统中,铜蓝蛋白和铜白蛋白似乎同样具有激活主动脉CuZn-SOD的能力。此外,铜向酶结构的转移似乎是恢复对酶的催化活性的主要事件。

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