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大鼠睾丸磷酸二酯酶激活蛋白与兔骨骼肌肌钙蛋白-C的生物学交叉反应性。

Biological cross-reactivity of rat testis phosphodiesterase activator protein and rabbit skeletal muscle troponin-C.

作者信息

Dedman J R, Potter J D, Means A R

出版信息

J Biol Chem. 1977 Apr 10;252(7):2437-40.

PMID:191460
Abstract

Phosphodiesterase activator protein and troponin-C have been purified from rat testis and rabbit skeletal muscle, respectively. The two proteins appear to be structurally distinct since the activator protein migrates faster than troponin-C on sodium dodecyl sulfate-polyacrylamide gels. Each of the calcium-binding proteins will, however, substitute for the other in their respective biological systems. Testis activator protein forms a complex with rabbit muscle troponin subunits TnI and TnT soluble in low salt. This hybrid complex (AIT) can regulate rabbit skeletal muscle actomyosin ATPase activity. AIT regulation, although influenced by free Aa2+ levels, is distinct from that of native troponin. Likewise, muscle troponin-C can substitute for activator protein in the stimulation of cyclic nucleotide phosphodiesterase. Troponin-C will fully stimulate phosphodiesterase although its affinity is 600-fold lower than that of activator protein. Ca2+ regulation studies demonstrate that both proteins require micormolar levels of free Ca2+ to induce phosphodiesterase activation. Activator protein requires 1.2 x 10(6) M and troponin-C, 1.9 X 10(6) M free Ca2+ for half-maximal stimulation of phosphodiesterase. The biological cross-reactivity of these proteins supports the sequence homology recently reported by Watterson et al. (Watterson, D.M., Harrelson, W.G., Keller, P.M., Sharief, F., and Vanaman, T.C. (1976) J.Biol. Chem. 251, 4501-4513). In addition, this preliminary study suggests that this nonmuscle troponin-C-like protein potentially may function in other Ca2+-regulated cellular events in addition to its moculation of cyclic nucleotide levels.

摘要

磷酸二酯酶激活蛋白和肌钙蛋白C分别从大鼠睾丸和兔骨骼肌中纯化得到。这两种蛋白质在结构上似乎不同,因为在十二烷基硫酸钠-聚丙烯酰胺凝胶上,激活蛋白的迁移速度比肌钙蛋白C快。然而,每种钙结合蛋白在其各自的生物系统中都可以相互替代。睾丸激活蛋白与兔肌肉肌钙蛋白亚基TnI和TnT形成一种可溶于低盐的复合物。这种杂交复合物(AIT)可以调节兔骨骼肌肌动球蛋白ATP酶的活性。AIT的调节虽然受游离Ca2+水平的影响,但与天然肌钙蛋白的调节不同。同样,肌肉肌钙蛋白C可以替代激活蛋白来刺激环核苷酸磷酸二酯酶。肌钙蛋白C虽然其亲和力比激活蛋白低600倍,但仍能完全刺激磷酸二酯酶。Ca2+调节研究表明,这两种蛋白质都需要微摩尔水平的游离Ca2+来诱导磷酸二酯酶的激活。激活蛋白需要1.2×10(-6)M,肌钙蛋白C需要1.9×10(-6)M游离Ca2+才能对磷酸二酯酶进行半最大刺激。这些蛋白质的生物交叉反应性支持了Watterson等人最近报道的序列同源性(Watterson, D.M., Harrelson, W.G., Keller, P.M., Sharief, F., and Vanaman, T.C. (1976) J.Biol. Chem. 251, 4501-4513)。此外,这项初步研究表明,这种非肌肉肌钙蛋白C样蛋白除了调节环核苷酸水平外,还可能在其他Ca2+调节的细胞事件中发挥作用。

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J Biol Chem. 1977 Apr 10;252(7):2437-40.
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