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通过使用光反应性法尼基类似物分析转导素的法尼基部分的分子相互作用。

Analysis of the molecular interaction of the farnesyl moiety of transducin through the use of a photoreactive farnesyl analogue.

作者信息

Hagiwara Ken'ichi, Wada Akimori, Katadae Maiko, Ito Masayoshi, Ohya Yoshikazu, Casey Patrick J, Fukada Yoshitaka

机构信息

Department of Biophysics and Biochemistry, Graduate School of Science, The University of Tokyo, Hongo, Bunkyo-ku, Tokyo 113-0032, Japan.

出版信息

Biochemistry. 2004 Jan 20;43(2):300-9. doi: 10.1021/bi0351514.

Abstract

Farnesylation of the gamma-subunit of the retinal G-protein, transducin (Talpha/Tbetagamma), is indispensable for light-initiated signaling in photoreceptor cells. However, the farnesyl-mediated molecular interactions important for signaling are not well understood. To explore this issue, we created a functional Tbetagamma analogue in which the farnesyl group was replaced with a (3-azidophenoxy)geranyl (POG) group, a novel farnesyl analogue with a distal photoreactive azido group. In the presence of lipid membranes and/or Talpha-GDP, UV irradiation of POG-modified Tbetagamma (POG-Tbetagamma) invariably yielded a cross-linked product Tgamma-Tbeta, reflecting a constitutive interaction of the Tgamma C-terminal lipid with Tbeta. In addition to the Tgamma-Tbeta adduct, a Tgamma-Talpha cross-link was detected in the aqueous fraction. Reconstitution of POG-Tbetagamma with Talpha and light-activated rhodopsin (Rh) in photoreceptor membranes resulted in cross-linking of Tgamma with a glycerophospholipid, indicating molecular interaction of the farnesyl group with cellular membranes. The Tgamma-phospholipid cross-link was observed only in the presence of both Talpha-GDP and Rh, and was abolished by the addition of GTPgammaS or by replacing Rh with opsin. These findings suggest a transient farnesyl-membrane interaction occurs only in a signaling state formed in a transducin-Rh ternary complex. On the other hand, UV irradiation of POG-Tbetagamma in a soluble complex with phosducin, a negative regulator of G-protein, yielded a Tgamma-phosducin adduct in addition to the Tgamma-Tbeta cross-link. These results illustrate that, rather than being a static membrane anchor, the farnesyl moiety plays an active role in the dynamics of protein-protein and protein-membrane interactions at defined steps in the signal transduction process.

摘要

视网膜G蛋白转导素(Tα/Tβγ)的γ亚基的法尼基化对于光感受器细胞中的光启动信号传导必不可少。然而,对于信号传导重要的法尼基介导的分子相互作用尚未得到充分理解。为了探讨这个问题,我们创建了一种功能性Tβγ类似物,其中法尼基基团被(3-叠氮苯氧基)香叶基(POG)基团取代,这是一种带有远端光反应性叠氮基团的新型法尼基类似物。在脂质膜和/或Tα-GDP存在的情况下,紫外线照射POG修饰的Tβγ(POG-Tβγ)总是产生交联产物Tγ-Tβ,这反映了Tγ C末端脂质与Tβ的组成性相互作用。除了Tγ-Tβ加合物外,在水相中还检测到Tγ-Tα交联。POG-Tβγ与Tα和光感受器膜中的光激活视紫红质(Rh)重组导致Tγ与甘油磷脂交联,表明法尼基基团与细胞膜的分子相互作用。仅在Tα-GDP和Rh同时存在的情况下观察到Tγ-磷脂交联,并且通过添加GTPγS或用视蛋白取代Rh而消除。这些发现表明瞬时法尼基-膜相互作用仅发生在转导素-Rh三元复合物形成的信号传导状态中。另一方面,在与G蛋白负调节剂磷转导蛋白的可溶性复合物中紫外线照射POG-Tβγ,除了Tγ-Tβ交联外,还产生了Tγ-磷转导蛋白加合物。这些结果表明,法尼基部分不是静态的膜锚,而是在信号转导过程中特定步骤的蛋白质-蛋白质和蛋白质-膜相互作用的动力学中发挥积极作用。

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