A CYSTEINE RESIDUE IN THE 3RD MEMBRANE-SPANNING SEGMENT OF THE HUMAN D-2-DOPAMINE RECEPTOR IS EXPOSED IN THE BINDING-SITE CREVICE

被引:128
作者
JAVITCH, JA
LI, XC
KABACK, J
KARLIN, A
机构
[1] COLUMBIA UNIV,DEPT PSYCHIAT,NEW YORK,NY 10032
[2] COLUMBIA UNIV,DEPT BIOCHEM & MOLEC BIOPHYS,NEW YORK,NY 10032
[3] COLUMBIA UNIV,DEPT NEUROL,NEW YORK,NY 10032
[4] COLUMBIA UNIV,DEPT PHYSIOL & CELLULAR BIOPHYS,NEW YORK,NY 10032
[5] NEW YORK STATE PSYCHIAT INST & HOSP,NEW YORK,NY 10032
关键词
SURFACE MAPPING; MUTAGENESIS; SULFHYDRYL; METHANETHIOSULFONATE; CATECHOLAMINE RECEPTOR;
D O I
10.1073/pnas.91.22.10355
中图分类号
O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];
学科分类号
07 ; 0710 ; 09 ;
摘要
The binding site in G-protein-Linked neurotransmitter receptors is formed among their membrane-spanning segments. Because the binding site is in the plane of the bilayer and is accessible to charged, water-soluble agonists, it must lie in a crevice open to the extracellular, aqueous medium. Information about the structure of these receptors can be obtained by identifying the residues in the membrane-spanning segments which face this water-filled crevice. Human D-2 dopamine receptor was expressed in human embryonic kidney 293 cells. Small, charged, sulfhydryl-specific methanethiosulfonate (MTS) derivatives irreversibly inhibited the binding of the D-2-specific antagonist [H-3]YM-09151-2 to these cells. The highly polar MTS derivatives should react with cysteine sulfhydryl groups only at the water-accessible surface of the receptor, which includes the surface of the binding-site crevice. In contrast, these reagents will have little access to sulfhydryls facing the lipid bilayer or buried in the protein interior. Positively charged MTS reagents irreversibly inhibited binding several hundredfold faster than a negatively charged MTS reagent, consistent with the affinity of-the binding site for positively charged dopamine agonists and antagonists. Furthermore, both agonists and antagonists of the D-2 receptor protected against irreversible inhibition by the MTS reagents. To identify the susceptible cysteine, we mutated, one at a time, five transmembrane and two extracellular cysteine residues to serine. Only the mutation of Cys(118) to serine decreased the susceptibility of antagonist binding to irreversible inhibition by the MTS reagents. Thus, Cys(118), a residue in the middle of the third membrane-spanning segment, is exposed in the D-2 receptor binding-site crevice.
引用
收藏
页码:10355 / 10359
页数:5
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