Асосий контентга ўтиш
AkademIndex

Маҳсулотлар

Ишлаб чиқувчилар учун

AkademBaseЭкотизим учун очиқ API
Мақола

Thiol Modification of Cysteine 327 in the Eighth Transmembrane Domain of the Light Subunit xCT of the Heteromeric Cystine/Glutamate Antiporter Suggests Close Proximity to the Substrate Binding Site/Permeation Pathway

Maite Jiménez-VidalDepartment of Biochemistry and Molecular Biology, Faculty of Biology, University of Barcelona, E-08028 Barcelona, SpainEmma GasolDepartment of Biochemistry and Molecular Biology, Faculty of Biology, and the Barcelona Science Park, University of Barcelona, E-08028 Barcelona, SpainAntónio ZorzanoDepartment of Biochemistry and Molecular Biology, Faculty of Biology, and the Barcelona Science Park, University of Barcelona, E-08028 Barcelona, SpainVirginia NunesMedical and Molecular Genetics Center, Institut de Recerca Oncològica, L'Hospitalet de Llobregat, E-08028 Barcelona, SpainManuel Palacı́nDepartment of Biochemistry and Molecular Biology, Faculty of Biology, and the Barcelona Science Park, University of Barcelona, E-08028 Barcelona, SpainJosep ChillarónDepartment of Biochemistry and Molecular Biology, Faculty of Biology, and the Barcelona Science Park, University of Barcelona, E-08028 Barcelona, Spain
2004en
ABI

Аннотация

We measured sensitivity to thiol modification of the heteromeric glutamate/cystine transporter 4F2hc-xCT expressed in Xenopus oocytes. p-Chloromercuribenzoate (pCMB) and p-chloromercuribenzenesulfonate (pCMBS) rapidly blocked transport activity. Cys(327), located in the middle of the eighth transmembrane domain of the light subunit (xCT), was found to be the main target of inactivation. Cysteine, an impermeant reducing reagent, reversed pCMB and pCMBS effects only when applied from the extracellular medium. l-Glutamate and l-cystine, but not l-arginine, protected from the inactivation with an IC(50) similar to the K(m). Protection was not temperature-dependent, suggesting that it did not depend on large substrate-induced conformational changes. Mutation of Cys(327) to Ala and Ser slightly modified the K(m) and a C327L mutant abolished transport function without compromising transporter expression at the plasma membrane. The results indicate that Cys(327) is a functionally important residue accessible to the aqueous extracellular environment and is structurally linked to the permeation pathway and/or the substrate binding site.

Ҳали таржима қилинмаган

Идентификаторлар

Иқтибослар ва манбалар

2 та иқтибос0 та фойдаланилган манба