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效应酶通过增加转导素与RGS蛋白之间的亲和力来调节脊椎动物光感受器中G蛋白信号传导的持续时间。

The effector enzyme regulates the duration of G protein signaling in vertebrate photoreceptors by increasing the affinity between transducin and RGS protein.

作者信息

Skiba N P, Hopp J A, Arshavsky V Y

机构信息

Department of Ophthalmology, Harvard Medical School, Massachusetts Eye and Ear Infirmary, Boston Massachusetts 02114, USA.

出版信息

J Biol Chem. 2000 Oct 20;275(42):32716-20. doi: 10.1074/jbc.C000413200.

DOI:10.1074/jbc.C000413200
PMID:10973941
Abstract

The photoreceptor-specific G protein transducin acts as a molecular switch, stimulating the activity of its downstream effector in its GTP-bound form and inactivating the effector upon GTP hydrolysis. This activity makes the rate of transducin GTPase an essential factor in determining the duration of photoresponse in vertebrate rods and cones. In photoreceptors, the slow intrinsic rate of transducin GTPase is accelerated by the complex of the ninth member of the regulators of G protein signaling family with the long splice variant of type 5 G protein beta subunit (RGS9.Gbeta5L). However, physiologically rapid GTPase is observed only when transducin forms a complex with its effector, the gamma subunit of cGMP phosphodiesterase (PDEgamma). In this study, we addressed the mechanism by which PDEgamma regulates the rate of transducin GTPase. We found that RGS9.Gbeta5L alone has a significant ability to activate transducin GTPase, but its affinity for transducin is low. PDEgamma acts by enhancing the affinity between activated transducin and RGS9.Gbeta5L by more than 15-fold, which is evident both from kinetic measurements of transducin GTPase rate and from protein binding assays with immobilized transducin. Furthermore, our data indicate that a single RGS9.Gbeta5L molecule is capable of accelerating the GTPase activity of approximately 100 transducin molecules/s. This rate is faster than the rates reported previously for any RGS protein and is sufficient for timely photoreceptor recovery in both rod and cone photoreceptors.

摘要

光感受器特异性G蛋白转导素作为一种分子开关,以其结合GTP的形式刺激其下游效应器的活性,并在GTP水解后使效应器失活。这种活性使得转导素GTP酶的速率成为决定脊椎动物视杆细胞和视锥细胞光反应持续时间的一个重要因素。在光感受器中,转导素GTP酶的缓慢内在速率通过G蛋白信号调节家族的第九个成员与5型G蛋白β亚基的长剪接变体(RGS9.Gβ5L)的复合物而加速。然而,只有当转导素与其效应器cGMP磷酸二酯酶的γ亚基(PDEγ)形成复合物时,才会观察到生理上快速的GTP酶活性。在本研究中,我们探讨了PDEγ调节转导素GTP酶速率的机制。我们发现,单独的RGS9.Gβ5L具有显著激活转导素GTP酶的能力,但其对转导素的亲和力较低。PDEγ通过将活化的转导素与RGS9.Gβ5L之间的亲和力提高15倍以上来发挥作用,这在转导素GTP酶速率的动力学测量以及与固定化转导素的蛋白质结合试验中都很明显。此外,我们的数据表明,单个RGS9.Gβ5L分子能够加速约100个转导素分子/秒的GTP酶活性。这个速率比之前报道的任何RGS蛋白的速率都要快,足以使视杆细胞和视锥细胞光感受器及时恢复。

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