Bourova Lenka, Kostrnova Alexandra, Hejnova Lucie, Moravcova Zuzana, Moon Hyo-Eun, Novotny Jiri, Milligan Graeme, Svoboda Petr
Institute of Physiology, Academy of Sciences of the Czech Republic, Prague, Czech Republic.
J Neurochem. 2003 Apr;85(1):34-49. doi: 10.1046/j.1471-4159.2003.01667.x.
Low-density membrane fragments (domains) were separated from the bulk of plasma membranes of human embryonic kidney (HEK)293 cells expressing a delta-opioid (DOP) receptor-Gi1alpha fusion protein by drastic homogenization and flotation on equilibrium sucrose density gradients. The functional activity of trimeric G proteins and capacity of the DOP receptor to stimulate both the fusion protein-linked Gi1alpha and endogenous pertussis-toxin sensitive G proteins was measured as d-Ala2, d-Leu5-enkephalin stimulated high-affinity GTPase or guanosine-5'-[gamma-35S]triphosphate ([35S]GTPgammaS) binding. The maximum d-Ala2-d-Leu5 enkephalin (DADLE)-stimulated GTPase was two times higher in low-density membrane fragments than in bulk of plasma membranes; 58 and 27 pmol/mg/min, respectively. The same difference was obtained for [35S]GTPgammaS binding. Contrarily, the low-density domains contained no more than half the DOP receptor binding sites (Bmax = 6.6 pmol/mg versus 13.6 pmol/mg). Thus, when corrected for expression levels of the receptor, low-density domains exhibited four times higher agonist-stimulated GTPase and [35S]GTPgammaS binding than the bulk plasma membranes. The regulator of G protein signaling RGS1, enhanced further the G protein functional activity but did not remove the difference between domain-bound and plasma membrane pools of G protein. The potency of the agonist in functional studies and the affinity of specific [3H]DADLE binding to the receptor were, however, the same in both types of membranes - EC50 = 4.5 +/- 0.1 x 10(-8) and 3.2 +/- 1.4 x 10(-8) m for GTPase; Kd = 1.2 +/- 0.1 and 1.3 +/- 0.1 nm for [3H]DADLE radioligand binding assay. Similar results were obtained when sodium bicarbonate was used for alkaline isolation of membrane domains. By contrast, detergent-insensitive membrane domains isolated following treatment of cells with Triton X100 exhibited no DADLE-stimulated GTPase or GTPgammaS binding. Functional coupling between the DOP receptor and cognate G proteins was also blocked by high-energy ultrasound and repeated freezing-thawing. Our data indicate, for the first time, that membrane domains isolated using 'detergent-free' procedures exhibit higher efficiency of coupling between a G protein-coupled receptor and its corresponding G protein(s) than bulk plasma membranes. Detergent-extraction diminishes these interactions, even when the receptor and G proteins are physically tethered together.
通过剧烈匀浆和在平衡蔗糖密度梯度上进行浮选,从表达δ-阿片受体(DOP)-Gi1α融合蛋白的人胚肾(HEK)293细胞的大部分质膜中分离出低密度膜片段(结构域)。三聚体G蛋白的功能活性以及DOP受体刺激融合蛋白连接的Gi1α和内源性百日咳毒素敏感G蛋白的能力,通过d-Ala2、d-Leu5-脑啡肽刺激的高亲和力GTP酶或鸟苷-5'-[γ-35S]三磷酸([35S]GTPγS)结合来测定。在低密度膜片段中,d-Ala2-d-Leu5脑啡肽(DADLE)刺激的最大GTP酶活性比质膜的大部分高两倍;分别为58和27 pmol/mg/min。[35S]GTPγS结合也得到了相同的差异。相反,低密度结构域所含的DOP受体结合位点不超过一半(Bmax = 6.6 pmol/mg,而质膜为13.6 pmol/mg)。因此,校正受体表达水平后,低密度结构域中激动剂刺激的GTP酶活性和[35S]GTPγS结合比质膜高四倍。G蛋白信号调节因子RGS1进一步增强了G蛋白的功能活性,但并未消除结构域结合的G蛋白与质膜池之间的差异。然而,在两种类型的膜中,激动剂在功能研究中的效力以及特异性[3H]DADLE与受体结合的亲和力是相同的——GTP酶活性的EC50 = 4.5 +/- 0.1 x 10(-8)和3.2 +/- 1.4 x 10(-8) m;[3H]DADLE放射性配体结合测定的Kd = 1.2 +/- 0.1和1.3 +/- 0.1 nm。当使用碳酸氢钠进行膜结构域的碱性分离时,也得到了类似的结果。相比之下,用Triton X100处理细胞后分离的去污剂不敏感膜结构域未表现出DADLE刺激的GTP酶活性或GTPγS结合。DOP受体与同源G蛋白之间的功能偶联也被高能超声和反复冻融所阻断。我们的数据首次表明,使用“无去污剂”方法分离的膜结构域,与质膜相比,在G蛋白偶联受体与其相应G蛋白之间表现出更高的偶联效率。去污剂提取会减少这些相互作用,即使受体和G蛋白在物理上拴在一起。
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