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Phosphorylation of S955 at the Protein Kinase A Consensus Promotes Maturation of the α Subunit of the Colonic H+,K+-ATPase
Author(s) -
Juan Codina,
Jingfang Liu,
Anthony J. Bleyer,
Raymond B. Penn,
Thomas D. DuBose
Publication year - 2006
Publication title -
journal of the american society of nephrology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 4.451
H-Index - 279
eISSN - 1533-3450
pISSN - 1046-6673
DOI - 10.1681/asn.2006010032
Subject(s) - protein subunit , g alpha subunit , atpase , transmembrane domain , phosphorylation , protein kinase a , cystic fibrosis transmembrane conductance regulator , biology , transmembrane protein , aspartic acid , amino acid , biochemistry , microbiology and biotechnology , enzyme , receptor , gene
All the alpha subunits of the Na+,K+ -ATPases and H+,K+ -ATPases have a protein kinase A (PKA) consensus sequence near or in the ninth transmembrane domain. The role of this domain in influencing alpha subunit synthesis/degradation, plasma membrane localization, and 86Rb+ uptake has not been established for the alpha subunit of the colonic H+,K+ -ATPase. This study examined the effect of mutating S955 (within the PKA consensus site of the alpha subunit of the colonic H+,K+ -ATPase [HKalpha2]) to alanine (S955/A) or aspartic acid (S955/D) on alpha subunit expression and function. The results demonstrate that a negatively charged amino acid at position 955 of HKalpha2 promotes higher expression levels of both whole-cell and plasma membrane-localized HKalpha2. Moreover, inhibition of PKA reduced expression of wild-type HKalpha2 and associated 86Rb+ uptake. Last, the activity of the HKalpha2 S955/A was rescued by treatment with 4-phenylbutyric acid, a compound that was shown previously to restore function to the cystic fibrosis transmembrane conductance regulator.

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