The membrane-bound ATP synthase (F1Fo) from mitochondria, chloroplasts and
bacteria plays a crucial role in energy-transducing reactions. In the case
of Escherichia coli, the reversible, proton-translocating ATPase complex co
nsists of two different entities, F-1 and F-o. The water-soluble F-1 part c
arries the catalytic sites for ATP synthesis and hydrolysis, It is associat
ed with the membrane-embedded F-o complex, which functions as a proton chan
nel and consists of subunits a, b and c present in a stoichiometry of 1:2:1
2.
Subunit b was isolated by preparative gel electrophoresis, acetone-precipit
ated and renatured in a cholate-containing buffer. Reconstituted subunit b
together with purified ac subcomplex is active in proton translocation and
F-1 binding, thereby demonstrating that subunit b had recovered its native
conformation. Circular dichroism spectroscopy of subunit b reconstituted in
to liposomes revealed a rather high degree of alpha-helical conformation of
80%.
After addition of a His(6)-tag to the N terminus of subunit a, a stable ab(
2) subcomplex was purified instead of a single subunit a, arguing in favour
of a direct interaction between these subunits, After addition of subunit
c and reconstitution into phospholipid vesicles, an F-o complex was obtaine
d exhibiting rates of proton translocation and F-1 binding comparable with
those of wild-type F-o.
The epitopes of monoclonal antibodies against subunit c are located in the
hydrophilic loop region (cL31-Q42) as mapped by enzyme-linked immunosorbent
assay using overlapping synthetic heptapeptides. Binding studies revealed
that all monoclonal antibodies (mAbs) bind to everted membrane vesicles irr
espective of the presence or absence of F-1. Although the hydrophilic regio
n of subunit c, and especially the highly conserved residues cA40, cR41, cQ
42 and cP43, are known to interact with subunits gamma and epsilon Of the F
-1 part, the mAb molecules have no effect on the function of F-o, either in
proton translocation or in F-1 binding, However, the F-1 part and the mAb
molecule(s) are hound simultaneously to the F-o complex, suggesting that no
t all c subunits are involved in the interaction with F-1.