http://www.cnr.it/ontology/cnr/individuo/prodotto/ID12669
Structures and interactions of proteins involved in the coupling function of the protonmotive FoF1-ATP Synthase (Articolo in rivista)
- Type
- Label
- Structures and interactions of proteins involved in the coupling function of the protonmotive FoF1-ATP Synthase (Articolo in rivista) (literal)
- Anno
- 2002-01-01T00:00:00+01:00 (literal)
- Alternative label
- Http://www.cnr.it/ontology/cnr/pubblicazioni.owl#autori
- Gaballo A., Zanotti F., Papa S. (literal)
- Pagina inizio
- Pagina fine
- Http://www.cnr.it/ontology/cnr/pubblicazioni.owl#numeroVolume
- Note
- ISI Web of Science (WOS) (literal)
- Titolo
- Structures and interactions of proteins involved in the coupling function of the protonmotive FoF1-ATP Synthase (literal)
- Abstract
- The mitochondrial F1Fo ATP synthase complex has a key role in cellular
energy metabolism. It can either synthesize or hydrolyze ATP, depending on
the presence or absence of an electrochemical proton gradient. The general
architecture of the enzyme is conserved among species and consists of a
globular catalytic moiety F1, protruding out of the membrane, a membrane
integral proton translocating moiety Fo, and a stalk connecting F1 to Fo.
The X ray crystallographic analysis of the structure of the bovine
mitochondrial F1 ATPase has provided a structural basis for the binding
change rotary mechanism of the catalytic process in F1, in which the g
subunit rotates in the central cavity of the F1 a3/b3 hexamer. Rotation of
g and e subunits in the E. coli enzyme, g and d subunits in the
mitochondrial enzyme, is driven, during ATP synthesis, by proton motive
rotation of an oligomer of c subunits (10-12) within the Fo basepiece.
Average analysis of electron microscopy images and cross-linking results
have revealed that, in addition to a central stalk, contributed by g and d/
e subunits, there is a second lateral one connecting the peripheries of Fo
and F1.
To gain deeper insight into the mechanism of coupling between proton
translocation and catalytic activity (ATP synthesis and hydrolysis),
studies have been undertaken on the role of F1 and Fo subunits which
contribute to the structural and functional connection between the
catalytic sector F1 and the proton translocating moiety Fo. These studies,
which employed limited proteolysis, chemical cross-linking and functional
analysis of the native and reconstituted F1Fo complex, as well as
isolated F1, have shown that the N-terminus of a subunits, located at the
top of the F1 hexamer, as indicated in the X ray crystallographic
structural analysis of F1, is essential for the energy coupling of F1 to
Fo. Moreover, the a N-terminus domain appears to be connected to Fo by
OSCP (Fo subunit conferring sensitivity of the complex to oligomycin).
OSCP contacts, in turn, FoI-PVP(b) and d subunits, with which it
constitutes a structure, which surrounds the central g and d rotary shaft.
Cross-linking of FoI-PVP(b) and g subunits causes a dramatic enhancement
of downhill proton translocation decoupled from ATP synthesis but is
without effect on ATP driven uphill proton transport. This would be
consistent with the existence of different rate-limiting steps in the two
directions of proton translocation through Fo.
In mitochondria, futile ATP hydrolysis by the F1Fo complex is specifically
inhibited by the water soluble ATPase inhibitor protein (IF1) which
reversibly binds at one side of the F1Fo connection. The trans-membrane D
pH component of the respiratory Dp displaces IF1 from the complex; in
particular, the matrix pH is the critical factor for IF1 association and
its related inhibitory activity. The 42L-58K segment of the IF1 has been
shown to be the most active segment of the protein; it interacts with the
surface of one a/b pairs of F1 thus inhibiting, with the same pH
dependence as the natural IF1, the conformational interconversions of the
catalytic sites involved in ATP hydrolysis.
IF1 has a relevant physiopathological role for the conservation of the
cellular ATP pool in ischemic tissues.Under these conditions IF1, which
seems to be over expressed, prevents dissipation of the ATP provided by
glycolysis.
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