Gβγ对人磷脂酶C-η2的激活作用
Activation of human phospholipase C-eta2 by Gbetagamma.
作者信息
Zhou Yixing, Sondek John, Harden T Kendall
机构信息
Department of Pharmacology, University of North Carolina School of Medicine, Chapel Hill, North Carolina 27599, USA.
出版信息
Biochemistry. 2008 Apr 15;47(15):4410-7. doi: 10.1021/bi800044n. Epub 2008 Mar 25.
Phospholipase C-eta2 (PLC-eta2) was recently identified as a novel broadly expressed phosphoinositide-hydrolyzing isozyme [Zhou, Y., et al. (2005) Biochem. J. 391, 667-676; Nakahara, M., et al. (2005) J. Biol. Chem. 280, 29128-29134]. In this study, we investigated the direct regulation of PLC-eta2 by Gbetagamma subunits of heterotrimeric G proteins. Coexpression of PLC-eta2 with Gbeta 1gamma 2, as well as with certain other Gbetagamma dimers, in COS-7 cells resulted in increases in inositol phosphate accumulation. Gbeta 1gamma 2-dependent increases in phosphoinositide hydrolysis also were observed with a truncation mutant of PLC-eta2 that lacks the long alternatively spliced carboxy-terminal domain of the isozyme. To begin to define the enzymatic properties of PLC-eta2 and its potential direct activation by Gbetagamma, a construct of PLC-eta2 encompassing the canonical domains conserved in all PLCs (PH domain through C2 domain) was purified to homogeneity after expression from a baculovirus in insect cells. Enzyme activity of purified PLC-eta2 was quantified after reconstitution with PtdIns(4,5)P 2-containing phospholipid vesicles, and values for K m (14.4 microM) and V max [12.6 micromol min (-1) (mg of protein) (-1)] were similar to activities previously observed with purified PLC-beta or PLC-epsilon isozymes. Moreover, purified Gbeta 1gamma 2 stimulated the activity of purified PLC-eta2 in a concentration-dependent manner similar to that observed with purified PLC-beta2. Activation was dependent on the presence of free Gbeta 1gamma 2 since its sequestration in the presence of Galpha i1 or GRK2-ct reversed Gbeta 1gamma 2-promoted activation. The PH domain of PLC-eta2 is not required for Gbeta 1gamma 2-mediated regulation since a purified fragment encompassing the EF-hand through C2 domains but lacking the PH domain nonetheless was activated by Gbeta 1gamma 2. Taken together, these studies illustrate that PLC-eta2 is a direct downstream effector of Gbetagamma and, therefore, of receptor-activated heterotrimeric G proteins.
磷脂酶C-η2(PLC-η2)最近被鉴定为一种新的广泛表达的磷酸肌醇水解同工酶[周,Y.等人(2005年)《生物化学杂志》391卷,667 - 676页;中原,M.等人(2005年)《生物化学杂志》280卷,29128 - 29134页]。在本研究中,我们研究了异源三聚体G蛋白的Gβγ亚基对PLC-η2的直接调控。在COS-7细胞中,PLC-η2与Gβ1γ2以及某些其他Gβγ二聚体共表达导致肌醇磷酸积累增加。对于缺乏该同工酶长的可变剪接羧基末端结构域的PLC-η2截短突变体,也观察到了Gβ1γ2依赖性的磷酸肌醇水解增加。为了开始确定PLC-η2的酶学性质及其被Gβγ直接激活的可能性,在昆虫细胞中通过杆状病毒表达后,将包含所有PLC中保守的典型结构域(从PH结构域到C2结构域)的PLC-η构建体纯化至同质。用含磷脂酰肌醇(4,5)二磷酸(PtdIns(4,5)P₂) 的磷脂囊泡重构后,对纯化的PLC-η2的酶活性进行了定量,其米氏常数(Kₘ)(14.4微摩尔)和最大反应速度(Vₘₐₓ)[12.6微摩尔·分钟⁻¹·(毫克蛋白)⁻¹]与先前用纯化的PLC-β或PLC-ε同工酶观察到的活性相似。此外,纯化的Gβ1γ2以浓度依赖性方式刺激纯化的PLC-η2的活性,这与用纯化的PLC-β2观察到的情况相似。激活依赖于游离Gβ1γ2的存在,因为在存在Gαi1或GRK2-ct的情况下将其隔离会逆转Gβ1γ2促进的激活。PLC-η2的PH结构域对于Gβ1γ2介导的调控不是必需的,因为一个包含从EF手结构域到C2结构域但缺乏PH结构域的纯化片段仍然被Gβ1γ2激活。综上所述,这些研究表明PLC-η2是Gβγ的直接下游效应物,因此也是受体激活的异源三聚体G蛋白的直接下游效应物。
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