Structure of V-ATPase from the mammalian brain | Zendy

Y.M. Abbas | Zendy; Di Wu | Zendy; Stephanie A. Bueler | Zendy; Carol V. Robinson | Zendy; John L. Rubinstein | Zendy

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Structure of V-ATPase from the mammalian brain

Author(s) -

Y.M. Abbas,

Di Wu,

Stephanie A. Bueler,

Carol V. Robinson,

John L. Rubinstein

Publication year - 2020

Publication title -

science

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 12.556

H-Index - 1186

eISSN - 1095-9203

pISSN - 0036-8075

DOI - 10.1126/science.aaz2924

Subject(s) - protein subunit , transmembrane protein , v atpase , synaptic vesicle , microbiology and biotechnology , biology , atpase , gene isoform , membrane protein , transmembrane domain , chemistry , biochemistry , membrane , vesicle , enzyme , receptor , gene

In neurons, the loading of neurotransmitters into synaptic vesicles uses energy from proton-pumping vesicular- or vacuolar-type adenosine triphosphatases (V-ATPases). These membrane protein complexes possess numerous subunit isoforms, which complicates their analysis. We isolated homogeneous rat brain V-ATPase through its interaction with SidK, a Legionella pneumophila effector protein. Cryo-electron microscopy allowed the construction of an atomic model, defining the enzyme's ATP:proton ratio as 3:10 and revealing a homolog of yeast subunit f in the membrane region, which we tentatively identify as RNAseK. The c ring encloses the transmembrane anchors for cleaved ATP6AP1/Ac45 and ATP6AP2/PRR, the latter of which is the (pro)renin receptor that, in other contexts, is involved in both Wnt signaling and the renin-angiotensin system that regulates blood pressure. This structure shows how ATP6AP1/Ac45 and ATP6AP2/PRR enable assembly of the enzyme's catalytic and membrane regions.

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