Wildman D E, Tamir H, Leberer E, Northup J K, Dennis M
Department of Pharmacology, Yale University School of Medicine, New Haven, CT 06510.
Proc Natl Acad Sci U S A. 1993 Feb 1;90(3):794-8. doi: 10.1073/pnas.90.3.794.
Guanine nucleotide-binding regulatory protein (G protein) beta gamma dimers that were active in reconstitution assays were produced in insect cells using the baculovirus/Sf9 insect cell expression system. Sf9 cells were infected either singly or in combination with recombinant baculoviruses containing a human G-protein beta 1 gene or a bovine G-protein gamma 2 gene. It was possible to express the beta 1 and gamma 2 gene products independently of each other in this system, as determined by using immunological and metabolic labeling techniques. Further, the ability of recombinant beta and/or gamma chains to function in defined biochemical assays of beta gamma activity was assessed for membrane extracts and supernatant fractions from infected Sf9 cells. Extracts of cells expressing beta or gamma chain alone were inactive in these assays, whereas those from cells coinfected with beta 1 and gamma 2 did display activity. These assays were used to identify recombinant beta gamma dimer migration during chromatographic purification, and the recombinant dimers were purified to near homogeneity. Both the membrane-associated and soluble beta gamma dimers facilitated rhodopsin-catalyzed guanosine 5'-[gamma-thio]triphosphate binding to Gt alpha, the GTP-binding subunit of the retinal G protein transducin (K0.5 of 13 +/- 2 and 36 +/- 5 nM, respectively). Both recombinant beta gamma dimers also facilitated the pertussis toxin-catalyzed ADP-ribosylation of Gt alpha with equal potency (K0.5 of 9 +/- 1 and 10 +/- 3 nM for membrane and soluble dimers, respectively). [3H]Mevalonolactone labeling showed that the gamma 2 subunits of membrane-associated beta gamma dimers incorporated radiolabel, whereas in the soluble form they did not. Thus, prenyl modification of gamma 2 directs the membrane association of the beta 1 gamma 2 dimer and increases its apparent affinity for receptor, but it is not required for the functional interaction(s) of the dimer.
利用杆状病毒/Sf9昆虫细胞表达系统在昆虫细胞中产生了在重组实验中具有活性的鸟嘌呤核苷酸结合调节蛋白(G蛋白)βγ二聚体。Sf9细胞单独感染或与含有人类G蛋白β1基因或牛G蛋白γ2基因的重组杆状病毒联合感染。通过免疫和代谢标记技术确定,在该系统中β1和γ2基因产物能够彼此独立表达。此外,针对感染的Sf9细胞的膜提取物和上清液组分,评估了重组β链和/或γ链在βγ活性的特定生化实验中发挥功能的能力。单独表达β链或γ链的细胞提取物在这些实验中无活性,而同时感染β1和γ2的细胞提取物则表现出活性。这些实验用于鉴定色谱纯化过程中重组βγ二聚体的迁移情况,并且将重组二聚体纯化至接近均一状态。膜相关的和可溶性的βγ二聚体均促进视紫红质催化鸟苷5'-[γ-硫代]三磷酸与Gtα结合,Gtα是视网膜G蛋白转导素的GTP结合亚基(K0.5分别为13±2和36±5 nM)。两种重组βγ二聚体还以相同效力促进百日咳毒素催化的Gtα的ADP核糖基化(膜二聚体和可溶性二聚体的K0.5分别为9±1和10±3 nM)。[3H]甲羟戊酸内酯标记显示,膜相关βγ二聚体的γ2亚基掺入放射性标记,而可溶性形式的则未掺入。因此,γ2的异戊二烯化修饰指导β1γ2二聚体的膜结合并增加其对受体 的表观亲和力,但对于二聚体的功能相互作用并非必需。
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