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蛙视网膜视杆细胞中光激发视紫红质与外周酶之间的相互作用。对视紫红质II衰变后阶段及视紫红质磷酸化速率的影响。

Interaction between photoexcited rhodopsin and peripheral enzymes in frog retinal rods. Influence on the postmetarhodopsin II decay and phosphorylation rate of rhodopsin.

作者信息

Pfister C, Kühn H, Chabre M

出版信息

Eur J Biochem. 1983 Nov 15;136(3):489-99. doi: 10.1111/j.1432-1033.1983.tb07767.x.

DOI:10.1111/j.1432-1033.1983.tb07767.x
PMID:6315431
Abstract

The major peripheral and soluble proteins in frog rod outer segment preparations, and their interactions with photoexcited rhodopsin, have been compared to those in cattle rod outer segments and found to be similar in both systems. In particular the GTP-binding protein (G) has the same subunit composition, the same abundance relative to rhodopsin (1/10) and it undergoes the same light and nucleotide-dependent interactions with rhodopsin in both preparations. Previous work on cattle rod outer segments has shown that photoexcited rhodopsin (R*), in a state identified with metarhodopsin II, associates with the G protein as a first step to the light-activated GDP/GTP exchange on G. The complex R*-G is stable in absence of GTP, but is rapidly dissociated by GTP owing to the GDP/GTP exchange reaction. Low bleaching extents (less than 10% R*) in absence of GTP therefore create predominantly R*-G complexes, whereas bleaching in presence of GTP creates free R*. We report here that, under conditions of complexed R*, two reactions of R* in frog rod outer segments are highly perturbed as compared to free R*: (a) the spectral decay of metarhodopsin II (MII) into later photoproducts, and (b) the phosphorylation of R* by an ATP-dependent protein kinase. a) The spectral measurements have been performed using linear dichroism on oriented frog rod outer segments; this technique allows discrimination between MII and later photoproducts absorbing at the same wavelength. Association of R* with G leads to a strong reduction of the amount of MIII formed and to an acceleration of the decay of MIII. Furthermore, MII is significantly stabilized, in agreement with the hypothesis that MII is the intermediate which binds to G. b) The phosphorylation of R* is strongly inhibited under conditions of R*-G complex formation as compared to free R*. Interferences between reactions at the three sites involved in R* are discussed: the retinal binding site in the hydrophobic core is sensitive to the presence of GTP-binding protein at its binding site on the cytoplasmic surface of R*; the kinase and the GTP-binding protein compete for access to their respective binding sites, both located on the surface of R*. We also observed a slow and nucleotide-dependent light-induced binding of a protein of molecular weight 50 000, which we consider as the equivalent of the 48 000 Mr light-dependent protein previously identified in cattle rod outer segments.

摘要

已将蛙视杆外段制剂中的主要外周蛋白和可溶性蛋白及其与光激发视紫红质的相互作用,与牛视杆外段中的相应成分进行了比较,发现这两个系统中的情况相似。特别是,鸟苷三磷酸结合蛋白(G)具有相同的亚基组成,相对于视紫红质的丰度相同(1/10),并且在两种制剂中它与视紫红质发生相同的光和核苷酸依赖性相互作用。先前对牛视杆外段的研究表明,处于与变视紫红质II相同状态的光激发视紫红质(R*),作为G上光激活的GDP/GTP交换的第一步,与G蛋白结合。在没有GTP的情况下,复合物R*-G是稳定的,但由于GDP/GTP交换反应,它会被GTP迅速解离。因此,在没有GTP的情况下低漂白程度(小于10%R*)主要产生R*-G复合物,而在有GTP的情况下漂白则产生游离的R*。我们在此报告,在R复合的条件下,与游离R相比,蛙视杆外段中R的两个反应受到高度干扰:(a)变视紫红质II(MII)向后续光产物的光谱衰减,以及(b)R被ATP依赖性蛋白激酶磷酸化。a)使用线性二色性对取向的蛙视杆外段进行了光谱测量;该技术允许区分在相同波长下吸收的MII和后续光产物。R与G的结合导致形成的MIII量大幅减少,并加速MIII的衰减。此外,MII显著稳定,这与MII是与G结合的中间体这一假设一致。b)与游离R相比,在R*-G复合物形成的条件下,R的磷酸化受到强烈抑制。讨论了R中涉及的三个位点处反应之间的干扰:疏水核心中的视黄醛结合位点对其在R细胞质表面的结合位点上存在鸟苷三磷酸结合蛋白敏感;激酶和鸟苷三磷酸结合蛋白竞争进入它们各自位于R表面的结合位点。我们还观察到一种分子量为50000的蛋白质的缓慢且核苷酸依赖性的光诱导结合,我们认为它相当于先前在牛视杆外段中鉴定出的48000Mr光依赖性蛋白。

相似文献

1
Interaction between photoexcited rhodopsin and peripheral enzymes in frog retinal rods. Influence on the postmetarhodopsin II decay and phosphorylation rate of rhodopsin.蛙视网膜视杆细胞中光激发视紫红质与外周酶之间的相互作用。对视紫红质II衰变后阶段及视紫红质磷酸化速率的影响。
Eur J Biochem. 1983 Nov 15;136(3):489-99. doi: 10.1111/j.1432-1033.1983.tb07767.x.
2
Interactions between photoexcited rhodopsin and GTP-binding protein: kinetic and stoichiometric analyses from light-scattering changes.光激发视紫红质与GTP结合蛋白之间的相互作用:基于光散射变化的动力学和化学计量分析
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The G-protein of retinal rod outer segments (transducin). Mechanism of interaction with rhodopsin and nucleotides.视网膜杆状细胞外段的G蛋白(转导素)。与视紫红质和核苷酸相互作用的机制。
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Light-induced interaction between rhodopsin and the GTP-binding protein. Metarhodopsin II is the major photoproduct involved.视紫红质与GTP结合蛋白之间的光诱导相互作用。主要的光产物是变视紫红质II。
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Phosphodiesterase activation by photoexcited rhodopsin is quenched when rhodopsin is phosphorylated and binds the intrinsic 48-kDa protein of rod outer segments.当视紫红质被磷酸化并结合视杆外段的内在48 kDa蛋白时,光激发视紫红质引起的磷酸二酯酶激活被淬灭。
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Light-induced interaction between rhodopsin and GTP-binding protein leads to the hydrolysis of GTP in the rod outer segment.视紫红质与GTP结合蛋白之间的光诱导相互作用导致视杆外段中GTP的水解。
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引用本文的文献

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Toward a unified model of vertebrate rod phototransduction.迈向脊椎动物视杆光转导的统一模型。
Vis Neurosci. 2005 Jul-Aug;22(4):417-36. doi: 10.1017/S0952523805224045.
2
Multiple steps of phosphorylation of activated rhodopsin can account for the reproducibility of vertebrate rod single-photon responses.活化视紫红质的多步磷酸化可解释脊椎动物视杆单光子反应的可重复性。
J Gen Physiol. 2003 Oct;122(4):419-44. doi: 10.1085/jgp.200308832. Epub 2003 Sep 15.
3
Function of the farnesyl moiety in visual signalling.法尼基部分在视觉信号传导中的作用。
Biochem J. 2000 Apr 1;347 Pt 1(Pt 1):163-71.
4
Light and GTP dependence of transducin solubility in retinal rods. Further analysis by near infra-red light scattering.视网膜视杆细胞中传导素溶解性的光和GTP依赖性。通过近红外光散射进行的进一步分析。
Eur Biophys J. 1988;16(4):207-18. doi: 10.1007/BF00261263.
5
The transducin cascade is involved in the light-induced structural changes observed by neutron diffraction on retinal rod outer segments.转导素级联反应参与了通过中子衍射在视网膜视杆外段观察到的光诱导结构变化。
Biophys J. 1987 Oct;52(4):587-94. doi: 10.1016/S0006-3495(87)83248-4.
6
Aluminofluoride action on G-proteins of the adenylate cyclase system is not different from that on transducin.铝氟化物对腺苷酸环化酶系统G蛋白的作用与对转导素的作用并无差异。
Biochem J. 1989 Mar 15;258(3):931-2. doi: 10.1042/bj2580931.
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The role of G proteins in transmembrane signalling.G蛋白在跨膜信号传导中的作用。
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