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通过连接到肌动蛋白半胱氨酸上的荧光探针在偏振光下进行脉冲荧光测定法研究肌动蛋白及其与重酶解肌球蛋白和调节蛋白的相互作用。

Study of actin and its interactions with heavy meromyosin and the regulatory proteins by the pulse fluorimetry in polarized light of a fluorescent probe attached to an actin cysteine.

作者信息

Tawada K, Wahl P, Auchet J C

出版信息

Eur J Biochem. 1978 Aug 1;88(2):411-9. doi: 10.1111/j.1432-1033.1978.tb12463.x.

Abstract

The decay of anisotropy of the N-iodoacetyl-N'-(5-sulfo-1-naphthyl)-ethylenediamine fluorescence attached to cysteine-373 of actin can be characterized by two correlation times theta1 and theta2. theta1 has a value of several nanoseconds and is thought to represent some local protein motion. theta2 is of the order of several hundreds of nanoseconds. Its value increases with actin concentration. It represents an average of the G and F actin correlation times. When actin interacts with heavy meromyosin, theta2 increases and becomes infinite at a molar ratio of one heavy meromyosin molecule per four actin protomers. It is concluded that a definite complex is then formed between F actin and heavy meromyosin. In the same time, G actin concentration becomes equal to zero. Finally, when F actin forms a complex with the regulatory proteins tropomyosin and troponin, the value of theta2 is greater in the absence than in the presence of Ca2+. This result indicates that micromolar concentrations of Ca2+ induces a conformation change of the complex of F actin with the regulatory proteins.

摘要

与肌动蛋白半胱氨酸-373相连的N-碘乙酰基-N'-(5-磺基-1-萘基)-乙二胺荧光各向异性的衰减可用两个相关时间θ1和θ2来表征。θ1的值为几纳秒,被认为代表了蛋白质的一些局部运动。θ2约为几百纳秒。其值随肌动蛋白浓度增加。它代表了G-肌动蛋白和F-肌动蛋白相关时间的平均值。当肌动蛋白与重酶解肌球蛋白相互作用时,θ2增加,在每四个肌动蛋白原纤维对应一个重酶解肌球蛋白分子的摩尔比时变为无穷大。可以得出结论,此时F-肌动蛋白和重酶解肌球蛋白之间形成了确定的复合物。同时,G-肌动蛋白浓度变为零。最后,当F-肌动蛋白与调节蛋白原肌球蛋白和肌钙蛋白形成复合物时,在无Ca2+时θ2的值大于有Ca2+时。这一结果表明,微摩尔浓度的Ca2+会诱导F-肌动蛋白与调节蛋白复合物的构象变化。

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