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共振能量转移作为GTP结合蛋白-效应器相互作用的直接监测手段:活化的α-转导蛋白与牛视觉转导级联反应中的cGMP磷酸二酯酶结合。

Resonance energy transfer as a direct monitor of GTP-binding protein-effector interactions: activated alpha-transducin binding to the cGMP phosphodiesterase in the bovine phototransduction cascade.

作者信息

Erickson J W, Cerione R A

机构信息

Department of Pharmacology, New York State College of Veterinary Medicine, Cornell University, Ithaca 14853-6401.

出版信息

Biochemistry. 1991 Jul 23;30(29):7112-8. doi: 10.1021/bi00243a011.

DOI:10.1021/bi00243a011
PMID:1713060
Abstract

Resonance energy-transfer approaches have been used to directly monitor the interactions of the GTP gamma S-bound alpha subunit of transducin (alpha T GTP gamma S) with the retinal cyclic GMP phosphodiesterase (PDE). The PDE was labeled with 5-(iodoacetamido) fluorescein (IAF-PDE) and served as the fluorescence donor in these experiments while the alpha T GTP gamma S was labeled with eosin-5-isothiocyanate (EITC-alpha T GTP gamma S) and served as the energy acceptor. The EITC-alpha T GTP gamma S species was able to quench a significant percentage of the IAF-PDE fluorescence (typically greater than or equal to 30%) due to resonance energy transfer between the IAF and EITC moieties. The quenching by the EITC-alpha T GTP gamma S species was dose-dependent, saturable (Kd = 21 nM), and specific for the GTP gamma S-bound form of the alpha T subunit. Limited trypsin treatment of the IAF-PDE, which selectively removes a fluorescein-labeled gamma subunit (gamma PDE), completely eliminates the quenching of the IAF fluorescence by the EITC-alpha T GTP gamma S complex. Although the EITC-alpha T GTP gamma S complex competes with the unlabeled alpha T GTP gamma S for a binding site on the IAF-PDE, as well as for a site on the native PDE, it is not able to stimulate PDE activity. Thus, the modification of a single EITC-reactive residue on the alpha T GTP gamma S complex prevents this subunit from eliciting a key activation event within the retinal effector enzyme.

摘要

共振能量转移方法已被用于直接监测转导素的GTPγS结合α亚基(αT GTPγS)与视网膜环鸟苷酸磷酸二酯酶(PDE)之间的相互作用。在这些实验中,PDE用5-(碘乙酰胺基)荧光素(IAF-PDE)标记,并作为荧光供体,而αT GTPγS用异硫氰酸酯-5-曙红(EITC-αT GTPγS)标记,并作为能量受体。由于IAF和EITC部分之间的共振能量转移,EITC-αT GTPγS能够淬灭相当比例的IAF-PDE荧光(通常大于或等于30%)。EITC-αT GTPγS的淬灭是剂量依赖性的、可饱和的(Kd = 21 nM),并且对αT亚基的GTPγS结合形式具有特异性。对IAF-PDE进行有限的胰蛋白酶处理,选择性地去除荧光素标记的γ亚基(γPDE),完全消除了EITC-αT GTPγS复合物对IAF荧光的淬灭。尽管EITC-αT GTPγS复合物与未标记的αT GTPγS竞争IAF-PDE上的结合位点以及天然PDE上的位点,但它不能刺激PDE活性。因此,αT GTPγS复合物上单个EITC反应性残基的修饰阻止了该亚基引发视网膜效应酶内的关键激活事件。

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