Mutation of the highly conserved Arg(165) and Glu(168) residues of human Gs alpha disrupts the alpha D-alpha E loop and enhances basal GDP/GTP exchange rate

Hinrichs, MV; Montecino, M.; Bunster, M; Olate, J

Abstract

G protein signalling regulates a wide range of cellular processes such as motility, differentiation, secretion, neurotransmission, and cell division. G proteins consist of three subunits organized as a G? monomer associated with a G?? heterodimer. Structural studies have shown that G? subunits are constituted by two domains: a Ras-like domain, also called the GTPase domain (GTPaseD), and an helical domain (HD), which is unique to heterotrimeric G-proteins. The HD display significantly higher primary structure diversity than the GTPaseD. Regardless of this diversity, there are small regions of the HD which show high degree of identity with residues that are 100% conserved. One of such regions is the ? helixD-? helixE loop (?D-?E) in the HD, which contains the consensus aminoacid sequence R*-[RSA]-[RSAN]-E*-[YF]-[QH]-L in all mammalian G? subunits. Interestingly, the highly conserved arginine (R*) and glutamic acid (E*) residues form a salt bridge that stabilizes the ?D-?E loop, that is localized in the top of the cleft formed between the GTPaseD and HD. Because the guanine nucleotide binding site is deeply buried in this cleft and those interdomain interactions are playing an important role in regulating the basal GDP/GTP nucleotide exchange rate of G? subunits, we studied the role of these highly conserved R and E residues in G? function. In the present study, we mutated the human Gs? R165 and E 168 residues to alanine (A), thus generating the R165 ? A, E168 ? A, and R165/E168 ? A mutants. We expressed these human Gs? (hGs?) mutants in bacteria as histidine tagged proteins, purified them by niquel-agarose chromatography and studied their nucleotide exchange properties. We show that the double R 165/E168 ? A mutant exhibited a fivefold increased GTP binding kinetics, a higher GDP dissociation rate, and an augmented capacity to activate adenylyl cyclase. Structure analysis showed that disruption of the salt bridge between R165 and E168 by the introduced mutations, caused important structural changes in the HD at the ?D-?E loop (residues 160-175) and in the GTPaseD at a region required for Gs? activation by the receptor (residues 308-315). In addition, other two GTPaseD regions that surround the GTP binding site were also affected. © 2004 Wiley-Liss, Inc.

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Título según WOS: Mutation of the highly conserved Arg(165) and Glu(168) residues of human Gs alpha disrupts the alpha D-alpha E loop and enhances basal GDP/GTP exchange rate
Título según SCOPUS: Mutation of the highly conserved Arg165 and Glu168 residues of human Gs? disrupts the ?D-?E loop and enhances basal GDP/GTP exchange rate
Título de la Revista: JOURNAL OF CELLULAR BIOCHEMISTRY
Volumen: 93
Número: 2
Editorial: Wiley
Fecha de publicación: 2004
Página de inicio: 409
Página final: 417
Idioma: English
URL: http://doi.wiley.com/10.1002/jcb.20193
DOI:

10.1002/jcb.20193

Notas: ISI, SCOPUS