| Literature DB >> 16891312 |
Margaret A Owegi1, Donald L Pappas, Mark W Finch, Sarah A Bilbo, Cruz A Resendiz, Lori J Jacquemin, Aswathy Warrier, John D Trombley, Kathryn M McCulloch, Katrina L M Margalef, Melissa J Mertz, Jason M Storms, Craig A Damin, Karlett J Parra.
Abstract
Vacuolar proton-translocating ATPase pumps consist of two domains, V(1) and V(o). Subunit d is a component of V(o) located in a central stalk that rotates during catalysis. By generating mutations, we showed that subunit d couples ATP hydrolysis and proton transport. The mutation F94A strongly uncoupled the enzyme, preventing proton transport but not ATPase activity. C-terminal mutations changed coupling as well; ATPase activity was decreased by 59-72%, whereas proton transport was not measurable (E328A) or was moderately reduced (E317A and C329A). Except for W325A, which had low levels of V(1)V(o), mutations allowed wild-type assembly regardless of the fact that subunits E and d were reduced at the membrane. N- and C-terminal deletions of various lengths were inhibitory and gradually destabilized subunit d, limiting V(1)V(o) formation. Both N and C terminus were required for V(o) assembly. The N-terminal truncation 2-19Delta prevented V(1)V(o) formation, although subunit d was available. The C terminus was required for retention of subunits E and d at the membrane. In addition, the C terminus of its bacterial homolog (subunit C from T. thermophilus) stabilized the yeast subunit d mutant 310-345Delta and allowed assembly of the rotor structure with subunits A and B. Structural features conserved between bacterial and eukaryotic subunit d and the significance of domain 3 for vacuolar proton-translocating ATPase function are discussed.Entities:
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Year: 2006 PMID: 16891312 DOI: 10.1074/jbc.M605006200
Source DB: PubMed Journal: J Biol Chem ISSN: 0021-9258 Impact factor: 5.157