Waldo Gary L, Harden T Kendall
Department of Pharmacology, University of North Carolina School of Medicine, Chapel Hill, North Carolina 27599-7365, USA.
Mol Pharmacol. 2004 Feb;65(2):426-36. doi: 10.1124/mol.65.2.426.
The human P2Y1 receptor (P2Y1-R) was purified after high-level expression from a recombinant baculovirus in Sf9 insect cells. Quantification by protein staining and with a radioligand binding assay using the high-affinity P2Y1-R antagonist [3H]MRS2279 ([3H]2-chloro-N6-methyl-(N)-methanocarba-2'-deoxyadenosine 3',5'-bis-phosphate) indicated a nearly homogenous preparation of receptor protein. Ki values determined in [3H]MRS2279 binding assays for antagonists with the purified P2Y1-R were in good agreement with the Ki and KB values determined for these molecules in membrane binding and activity assays, respectively. Availability of P2Y1-R in purified form allowed direct determination of nucleotide agonist affinities under conditions not compromised by nucleotide metabolism/interconversion, and an order of affinities of 2-methylthio-ADP (2MeSADP) > ADP = 2-methylthioATP = adenosine-5'-O-(3-thio)triphosphate = adenosine-5'-O(2-thiodiphosphate) >> ATP was obtained. The signaling activity of the purified P2Y1-R was quantified after reconstitution in proteoliposomes with heterotrimeric G proteins. Steady-state GTP hydrolysis in vesicles reconstituted with P2Y1-R and Galpha(q)beta(1)gamma(2) was stimulated by the addition of either 2MeADP or RGS4 alone and was increased by up to 50-fold in their combined presence. EC50 values of agonists for activation of the purified P2Y1-R were similar to their respective Ki values determined in radioligand binding experiments with the purified receptor. Moreover, ATP exhibited 20-fold higher EC50 and Ki values than did ADP and was a partial agonist relative to ADP and 2MeSADP under conditions in which no metabolism of the nucleotide occurred. Both RGS4 and PLC-beta1 were potent and efficacious GTPase-activating proteins for Galphaq and Galpha11 in P2Y1-R-containing vesicles. These results illustrate that the binding and signaling properties of the human P2Y1-R can be studied with purified proteins under conditions that circumvent the complications that occur in vivo.
人P2Y1受体(P2Y1-R)在杆状病毒重组体在Sf9昆虫细胞中高水平表达后被纯化。通过蛋白质染色以及使用高亲和力P2Y1-R拮抗剂[3H]MRS2279([3H]2-氯-N6-甲基-(N)-甲硫基-2'-脱氧腺苷3',5'-双磷酸)的放射性配体结合试验进行定量,结果表明受体蛋白的制备几乎是纯的。在[3H]MRS2279结合试验中,用纯化的P2Y1-R测定的拮抗剂的Ki值,分别与在膜结合试验和活性试验中为这些分子测定的Ki和KB值高度一致。纯化形式的P2Y1-R的可得性使得能够在不受核苷酸代谢/相互转化影响的条件下直接测定核苷酸激动剂的亲和力,并且得到的亲和力顺序为2-甲硫基-ADP(2MeSADP)>ADP = 2-甲硫基ATP =腺苷-5'-O-(3-硫代)三磷酸=腺苷-5'-O(2-硫代二磷酸)>>ATP。在用异源三聚体G蛋白重构到蛋白脂质体中后,对纯化的P2Y1-R的信号活性进行了定量。单独添加2MeADP或RGS4均可刺激用P2Y1-R和Gα(q)β(1)γ(2)重构的囊泡中的稳态GTP水解,并且在它们同时存在时水解增加高达50倍。激动剂激活纯化的P2Y1-R的EC50值与其在使用纯化受体的放射性配体结合实验中测定的各自的Ki值相似。此外,在核苷酸不发生代谢的条件下,ATP的EC50和Ki值比ADP高20倍,并且相对于ADP和2MeSADP是部分激动剂。RGS4和PLC-β1都是含P2Y1-R的囊泡中Gαq和Gα11的有效且高效的GTP酶激活蛋白。这些结果表明,在规避体内出现的复杂情况的条件下,可以用纯化的蛋白质研究人P2Y1-R的结合和信号特性。
Zotero 插件