人类组胺H(4)受体的高组成活性和不依赖G蛋白的高亲和力状态。
High constitutive activity and a G-protein-independent high-affinity state of the human histamine H(4)-receptor.
作者信息
Schneider Erich H, Schnell David, Papa Dan, Seifert Roland
机构信息
Department of Pharmacology and Toxicology, University of Regensburg, Universitatsstrasse 31, D-93040 Regensburg, Germany.
出版信息
Biochemistry. 2009 Feb 17;48(6):1424-38. doi: 10.1021/bi802050d.
The human histamine H(4)-receptor (hH(4)R) is expressed in mast cells and eosinophils and mediates histamine (HA)-induced chemotaxis via G(i)-proteins. For a detailed investigation of hH(4)R/G(i)-protein interaction, we coexpressed the hH(4)R with Galpha(i2) and Gbeta(1)gamma(2) as well as an hH(4)R-Galpha(i2) fusion protein with Gbeta(1)gamma(2) in Sf9 insect cells. The agonist radioligand [(3)H]HA showed a K(D) value of approximately 10 nM at hH(4)R and hH(4)R-Galpha(i2). The high-affinity states of hH(4)R and hH(4)R-Galpha(i2) were insensitive to guanosine 5'-[gamma-thio]triphosphate (GTPgammaS). The affinity of [(3)H]HA for hH(4)R was retained in the absence of mammalian G(i)-proteins. In steady-state GTPase- and [(35)S]GTPgammaS-binding assays, hH(4)R exhibited high constitutive activity and uncommon insensitivity to Na(+). Thioperamide (THIO) was only a partial inverse agonist. Addition of HA or THIO to baculovirus-infected (hH(4)R + Galpha(i2) + Gbeta(1)gamma(2)) Sf9 cells increased the B(max) in [(3)H]HA binding, but not in immunoblots, suggesting conformational instability and ligand-induced stabilization of membrane-integrated hH(4)R. No effect was observed on hH(4)R-Galpha(i2) expression, neither in [(3)H]HA binding nor in immunoblot. However, the expression level of hH(4)R-Galpha(i2) was consistently higher compared to hH(4)R, suggesting chaperone-like or stabilizing effects of Galpha(i2) on hH(4)R. In 37 degrees C stability assays, HA stabilized hH(4)R, and THIO even restored misfolded [(3)H]HA binding sites. Inhibition of hH(4)R glycosylation by tunicamycin reduced the [(3)H]HA binding B(max) value. In conclusion, (i) hH(4)R shows high constitutive activity and structural instability; (ii) hH(4)R shows a G-protein-independent high-affinity state; (iii) hH(4)R conformation is stabilized by agonists, inverse agonists and G-proteins; (iv) hH(4)R glycosylation is essential for cell-surface expression of intact hH(4)R.
人组胺H(4)受体(hH(4)R)在肥大细胞和嗜酸性粒细胞中表达,并通过G(i)蛋白介导组胺(HA)诱导的趋化作用。为了详细研究hH(4)R/G(i)蛋白相互作用,我们在Sf9昆虫细胞中共表达了hH(4)R与Gα(i2)和Gβ(1)γ(2),以及hH(4)R-Gα(i2)融合蛋白与Gβ(1)γ(2)。激动剂放射性配体[(3)H]HA在hH(4)R和hH(4)R-Gα(i2)上的K(D)值约为10 nM。hH(4)R和hH(4)R-Gα(i2)的高亲和力状态对鸟苷5'-[γ-硫代]三磷酸(GTPγS)不敏感。在没有哺乳动物G(i)蛋白的情况下,[(3)H]HA对hH(4)R的亲和力得以保留。在稳态GTP酶和[(35)S]GTPγS结合试验中,hH(4)R表现出高组成性活性且对Na(+)不常见的不敏感性。硫代哌啶(THIO)只是部分反向激动剂。向杆状病毒感染的(hH(4)R + Gα(i2) + Gβ(1)γ(2))Sf9细胞中添加HA或THIO会增加[(3)H]HA结合的B(max)值,但在免疫印迹中没有增加,这表明膜整合hH(4)R的构象不稳定以及配体诱导的稳定作用。在[(3)H]HA结合或免疫印迹中,对hH(4)R-Gα(i2)表达均未观察到影响。然而,与hH(4)R相比,hH(4)R-Gα(i2)的表达水平始终较高,这表明Gα(i2)对hH(4)R具有伴侣样或稳定作用。在37℃稳定性试验中,HA稳定了hH(4)R,而THIO甚至恢复了错误折叠的[(3)H]HA结合位点。衣霉素抑制hH(4)R糖基化会降低[(3)H]HA结合的B(max)值。总之,(i)hH(4)R表现出高组成性活性和结构不稳定性;(ii)hH(4)R表现出与G蛋白无关的高亲和力状态;(iii)hH(4)R构象通过激动剂、反向激动剂和G蛋白得以稳定;(iv)hH(4)R糖基化对于完整hH(4)R的细胞表面表达至关重要。
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