Chen Yongli, Banerjee Anamitro, Hess George P
Department of Molecular Biology and Genetics, 216 Biotechnology Building, Cornell University, Ithaca, New York 14853-2703, USA.
Biochemistry. 2004 Aug 10;43(31):10149-56. doi: 10.1021/bi049590u.
The nicotinic acetylcholine receptor (nAChR) belongs to a group of five structurally related membrane proteins that play a major role in the communication between approximately 10(12) cells of the mammalian nervous system. The receptor is inhibited by both abused drugs and therapeutic agents. During the past two decades, many attempts have been made to find compounds that prevent cocaine inhibition of this protein. The use of newly developed transient kinetic techniques in investigations of the inhibition of the receptor by cocaine and MK-801 led to an inhibition mechanism not previously proposed. It was observed that the receptor contains two inhibitory sites: one that equilibrates with the tested noncompetitive inhibitors within approximately 50 ms, and a second site that equilibrates with inhibitors within approximately 1 s. The mechanism of inhibition of the rapidly equilibrating inhibitory site has been investigated, and based on that mechanism, the first evidence that small organic molecules exist that prevent inhibition of the rapidly equilibrating inhibitory site was obtained. These compounds did not prevent the inhibition due to the slowly equilibrating inhibitory site. Here, we present the first evidence that a compound (3-acetoxy ecgonine methyl ester) exists that prevents inhibition of the slowly equilibrating inhibitory site and that the mechanism of inhibition of this site differs from that of the rapidly equilibrating site. BC3H1 cells containing a fetal mouse muscle-type nAChR were used, and the receptor was activated by carbamoylcholine. The resulting whole-cell current due to the nondesensitized nAChR was determined. Because the nAChR desensitizes rapidly, the measurements required the use of a transient kinetic technique with a time resolution of 10 ms; the cell-flow technique was used. Inhibitors and compounds that alleviate inhibition were tested by determining their effects on the whole-cell current due to activation of the nAChR by carbamoylcholine.
烟碱型乙酰胆碱受体(nAChR)属于一组结构相关的五种膜蛋白,在哺乳动物神经系统约10¹²个细胞之间的通讯中起主要作用。该受体受到滥用药物和治疗药物的抑制。在过去二十年中,人们进行了许多尝试来寻找能够阻止可卡因对该蛋白抑制作用的化合物。在研究可卡因和MK - 801对该受体的抑制作用时,使用新开发的瞬态动力学技术得出了一个以前未提出的抑制机制。据观察,该受体含有两个抑制位点:一个在约50毫秒内与测试的非竞争性抑制剂达到平衡,另一个位点在约1秒内与抑制剂达到平衡。对快速平衡抑制位点的抑制机制进行了研究,并基于该机制,获得了首个证据,即存在能够阻止快速平衡抑制位点被抑制的小分子有机化合物。这些化合物并未阻止由于缓慢平衡抑制位点导致的抑制作用。在此,我们首次证明存在一种化合物(3 - 乙酰氧基芽子碱甲酯),它能够阻止缓慢平衡抑制位点的抑制作用,并且该位点的抑制机制与快速平衡位点不同。使用含有胎儿小鼠肌肉型nAChR的BC3H1细胞,并用氨甲酰胆碱激活该受体。测定了由于未脱敏的nAChR产生的全细胞电流。由于nAChR快速脱敏,测量需要使用时间分辨率为10毫秒的瞬态动力学技术;采用了细胞流动技术。通过测定抑制剂和减轻抑制作用的化合物对氨甲酰胆碱激活nAChR所产生的全细胞电流的影响来进行测试。