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一个能刺激光感受器中G蛋白GTP酶的效应位点。

An effector site that stimulates G-protein GTPase in photoreceptors.

作者信息

Slepak V Z, Artemyev N O, Zhu Y, Dumke C L, Sabacan L, Sondek J, Hamm H E, Bownds M D, Arshavsky V Y

机构信息

Division of Biology, California Institute of Technology, Pasadena 91125, USA.

出版信息

J Biol Chem. 1995 Jun 16;270(24):14319-24. doi: 10.1074/jbc.270.24.14319.

DOI:10.1074/jbc.270.24.14319
PMID:7782290
Abstract

Heterotrimeric G-proteins mediate between receptors and effectors, acting as molecular clocks. G-protein interactions with activated receptors catalyze the replacement of GDP bound to the alpha-subunit with GTP. alpha-Subunits then modulate the activity of downstream effectors until the bound GTP is hydrolyzed. In several signal transduction pathways, including the cGMP cascade of photoreceptor cells, the relatively slow GTPase activity of heterotrimeric G-proteins can be significantly accelerated when they are complexed with corresponding effectors. In the phototransduction cascade the GTPase activity of photoreceptor G-protein, transducin, is substantially accelerated in a complex with its effector, cGMP phosphodiesterase. Here we characterize the stimulation of transducin GTPase by a set of 23 mutant phosphodiesterase gamma-subunits (PDE gamma) containing single alanine substitutions within a stretch of the 25 C-terminal amino acid residues known to be primarily responsible for the GTPase regulation. The substitution of tryptophan at position 70 completely abolished the acceleration of GTP hydrolysis by transducin in a complex with this mutant. This mutation also resulted in a reduction of PDE gamma affinity for transducin, but did not affect PDE gamma interactions with the phosphodiesterase catalytic subunits. Single substitutions of 7 other hydrophobic amino acids resulted in a 50-70% reduction in the ability of PDE gamma to stimulate transducin GTPase, while substitutions of charged and polar amino acids had little or no effect. These observations suggest that the role of PDE gamma in activation of the transducin GTPase rate may be based on multiple hydrophobic interactions between these molecules.

摘要

异源三聚体G蛋白作为分子时钟,在受体和效应器之间起介导作用。G蛋白与活化受体的相互作用催化与α亚基结合的GDP被GTP取代。然后α亚基调节下游效应器的活性,直到结合的GTP被水解。在包括光感受器细胞的cGMP级联反应在内的几种信号转导途径中,当异源三聚体G蛋白与相应效应器形成复合物时,其相对较慢的GTP酶活性可被显著加速。在光转导级联反应中,光感受器G蛋白转导素的GTP酶活性在与其效应器cGMP磷酸二酯酶形成的复合物中被大幅加速。在此,我们对一组23个突变的磷酸二酯酶γ亚基(PDEγ)刺激转导素GTP酶的情况进行了表征,这些突变体在已知主要负责GTP酶调节的25个C末端氨基酸残基区域内含有单个丙氨酸取代。在该突变体中,第70位色氨酸的取代完全消除了与转导素形成复合物时转导素对GTP水解的加速作用。该突变还导致PDEγ对转导素的亲和力降低,但不影响PDEγ与磷酸二酯酶催化亚基的相互作用。其他7个疏水氨基酸的单取代导致PDEγ刺激转导素GTP酶的能力降低50 - 70%,而带电荷和极性氨基酸的取代几乎没有影响。这些观察结果表明,PDEγ在激活转导素GTP酶速率中的作用可能基于这些分子之间的多种疏水相互作用。

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