Cerione R A, Kroll S, Rajaram R, Unson C, Goldsmith P, Spiegel A M
Department of Pharmacology, New York State College of Veterinary Medicine, Cornell University, Ithaca 14853-6401.
J Biol Chem. 1988 Jul 5;263(19):9345-52.
An antibody (AS/7) prepared against the carboxyl-terminal decapeptide of the alpha subunit of transducin (alpha T) has been used in various reconstitution studies aimed at characterizing the role of the carboxyl-terminal domain in the different functional activities of transducin. The peptide-specific antibody is a potent inhibitor of the rhodopsin-stimulated GTPase activity in phospholipid vesicle systems containing pure rhodopsin and pure holo-transducin, or rhodopsin and the purified alpha T and beta/gamma (beta gamma T) subunit components, with the highest levels of inhibition (80-95%) occurring under conditions where the molar ratio of holo-transducin (or alpha T) to AS/7 approximately equal to 1. The inhibition of the receptor-stimulated GTPase does not represent an interference in the interactions between the alpha T subunit and the beta gamma T complex, since essentially identical levels of inhibition are observed when AS/7 is preincubated with either free alpha T, holo-transducin, or alpha T in the presence of excess beta gamma T, prior to assay. The AS/7-induced inhibition also does not appear to reflect an alteration in the ability of alpha T to bind or hydrolyze GTP and, in fact, the incubation of alpha T with AS/7 results in a stimulation of the intrinsic GTPase activity for alpha T alone (i.e. in the absence of rhodopsin). Thus, we conclude that the inhibition of the rhodopsin-stimulated GTPase activity by AS/7 is due to the direct blocking (by the antibody) of rhodopsin-alpha T interactions. While AS/7 is capable of uncoupling rhodopsin-transducin interactions, it appears to promote the stimulation of the cyclic GMP phosphodiesterase (PDE) by an activated alpha T subunit. Specifically, when the pure alpha T-guanosine 5-O-(3-thiotriphosphate) (alpha TGTP gamma S) species is preincubated with AS/7 prior to its addition to an assay solution containing PDE, there is at least a 4-fold increase in the resultant cyclic GMP hydrolysis relative to the activities measured with alpha TGTP gamma S, alone, or with alpha TGTP gamma S preincubated with nonimmune (control) rabbit IgG. The AS/7-induced promotion is specific for the active form of alpha T; the inactive alpha TGDP species does not stimulate PDE activity either in the presence or absence of the antibody. The different effects by AS/7 on the various activities of the alpha T subunit highlight the existence of distinct functional domains on alpha T.(ABSTRACT TRUNCATED AT 400 WORDS)
一种针对转导素(αT)α亚基羧基末端十肽制备的抗体(AS/7)已用于各种重组研究,旨在确定羧基末端结构域在转导素不同功能活性中的作用。这种肽特异性抗体是含纯视紫红质和纯全转导素的磷脂囊泡系统中视紫红质刺激的GTP酶活性的有效抑制剂,在含视紫红质与纯化的αT和β/γ(βγT)亚基成分的系统中也有抑制作用,在全转导素(或αT)与AS/7的摩尔比约等于1的条件下抑制水平最高(80 - 95%)。受体刺激的GTP酶的抑制并不代表对αT亚基与βγT复合物之间相互作用的干扰,因为在测定前将AS/7与游离αT、全转导素或存在过量βγT时的αT预孵育,观察到的抑制水平基本相同。AS/7诱导的抑制似乎也不反映αT结合或水解GTP能力的改变,实际上,αT与AS/7孵育会导致单独的αT(即不存在视紫红质时)的内在GTP酶活性受到刺激。因此,我们得出结论,AS/7对视紫红质刺激的GTP酶活性的抑制是由于抗体直接阻断了视紫红质 - αT的相互作用。虽然AS/7能够解开视紫红质 - 转导素的相互作用,但它似乎能促进活化的αT亚基对环鸟苷酸磷酸二酯酶(PDE)的刺激。具体而言,当纯αT - 鸟苷5 - O -(3 - 硫代三磷酸)(αTGTPγS)在加入含有PDE的测定溶液之前与AS/7预孵育时,相对于单独用αTGTPγS或与非免疫(对照)兔IgG预孵育的αTGTPγS所测得的活性,产生的环鸟苷酸水解至少增加4倍。AS/7诱导的促进作用对αT的活性形式具有特异性;无活性的αTGDP形式在有或没有抗体的情况下均不刺激PDE活性。AS/7对αT亚基各种活性的不同影响突出了αT上不同功能结构域的存在。(摘要截断于400字)
