- Email: [email protected]
Immunochemical evidence that the FITC-labeling site on Na+,K+-ATPase is not the ATP binding site
Vol. 140,No. October
BIOCHEMICAL
1, 1987
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS Pages 246-253
14, 1987
Imnunochemical
Evidence
Na+,K+-ATPase
W.J.
Department
that
is
Ball
the
Not the
, Jr.
and M.L.
Cincinnati,
Site
Biophysics,
College
Ohio
on
Friedman
and Cell
of Cincinnati
Site
ATP Binding
of Pharmacology
University
FITC-labeling
of Medicine,
45267-0575
Received August 25, 1987 The covalent labeling of the a subunit of lamb fluorescein 5'-isothiocyanate at Lys-501 has generally at the ATP binding site. We have found that 496HLLVMKGAPER506 serves as the antigenic determinant M&Pl-A3: This antibody binds to both native and while this epitope undergoes ligand-induced changes involved in either enzyme function or the El * E2 monitored by FITC-fluorescence intensity. 0 1987 Academic
Na+,K+-ATPase
is
nit
(-100,DDO
and
the
maintenance
Mr) of
class
of ATP-driven
whose
functioning
ferent
conformations.
(FITC)
has been
has been fic
found
lysine
among
thought
and
to
monoclonal antibody
B subunit
(-50,000
Na+ levels
in
the
of the
The
cycling fluorescent
extensively
inactivate
to the
in a region
antibody
of the
pumps.
ATP blocks
Because FITC
of
the
M&Pl-A3
binds
function
and
enzyme
enzyme's
ATP to
0 I987
by Academic
of reproduction
in any
Press, form
Inc. reserved.
the
246
site
region
a subu-
function belongs
is to a
as ElE2 a series
pumps, of dif-
changes. by labeling is
a 1:l of
the
5'-isothiocyanate
which with
site
ligand-induced
between
activity
reacts
binding
(1)
ligand-induced
100 KD protein
this
enzyme
fluorescein
ATPase
labeling,
This
enzymes
these
FITC
primary
by Racker
probe study
Inc.
whose
cell.
involves
0006-291X/87$1.50 Copyright All rights
the
Press,
of two subunits,
Mr),
designated
be a portion
on
composed
transporters,
ElEp-ATPase
ATP binding
enzyme,
ion
used to
the
K+ and
residue
the
a membrane
kidney Na+,K+-ATPase by been assumed to occur the peptide sequence for monoclonal antibody FITC-labeled enzyme and these changes are not conformational changes
a speci-
highly
conserved
stoichiometry
labeling
is
(2).
We have
of a.
The effect
conformational
FITC
to
generally found
that
of
bound
changes
has
Vol. 148,No.
been
8lOCHEMlCALAND8lOPHYSlCALRESEARCH
1, 1987 The
investigated.
Na+,K+-ATPase
have also
EXPERIMENTAL
PROCEDURES
effects
of
these
ligands
COMMUNICATIONS
on
antibody
binding
to
been determined.
Enzyme preparation and assays. The Na+,K+-ATPase was prepared from frozen lamb kidneys as previously described by Lane et al (3). The Na+,K+-ATPase activity at 37'C was measured at 340 nm using the spectrophotometric, linked enzyme assay system of Schwartz et al (4) while the Kt-dependent p-nitrophenylphosphatase activity was determined by continuous measurement at 410 nm (5). [3H]-ouabain binding to the enzyme was determined at 37'C essentially as The labeling of Na+,K+-ATPase with described by Wallick and Schwartz (6). FITC (Molecular Probes, Inc.) has been described in our previous work (5), measurements were measured at 520 nm as while the fluorescence intensity described by Hegyvary and Jorgensen (7). Antibody M8-Pl-A3 preparation and binding determinations. This antibody was raised against the lamb kidney Na+,K+-ATPase and its isolation, purification and initial characterization was reported previously by Ball et al. (8). The indirect solid-surface adsorption (ELISA) assay used to quantitate antibody binding has been described in detail (8) but we have modified the proceIn this procedure antibody and enzyme were combined for l-2 h dure somewhat. and then the enzyme and any antibody-enzyme complex formed were removed from The unbound M8-Pl-A3 (in solution by centrifugation at 150,000 x g for 1 h. the supernatant) was then exposed to either untreated microtiter plates (Cooke flexible plates), plates previously coated with enzyme (+ 0.1% SDS), or synthetic peptide-BSA conjugates. M8-Pl-A3 binding to these plates was then quantitated using a B-galactosidase sheep anti-mouse IgG F(ab')2 conjugate as Solution phase binding of M8-Pl-A3 to the enzyme under second antibody. (Na +; Kt; Mg2+; Mg2+Pi and Mg2+ATP, all at 5 mM) was various ligand conditions also examined. RESULTS A collection Na+,K+-ATPase synthetic portions
of (9)
peptides
were
This
sequence
has
been
isolated,
(2,ll).
site
of
holoenzyme nM antibody, was about
Figure peptide
this the 2 6-BSA
respectively. 12-fold
lower
residues
a soluble
tryptic
and
to
shows
of
was achieved affinity
enzyme, 247
(Fig.
this
of the
the maximum
the
region
binding at
of
labeling of
levels
for
further
M8-Pl-A3
for of
a that
ATP binding
approximately antibody
peptide
site
was
of
of
sequence
1,
fragment
a portion
kidney
various
to the
(BSA)
covalent
to
lamb
a series
to bind
half-maximal
conjugate
for
be the
the
representing
digestion
M8-Pl-A3
that
the
length)
albumin
may comprise
binding
to recognize
was found
serum
region
to
in
M8-Pl-A3,
shown
raised
ability
bovine
While than
their
acid
to
sequenced
Na+,K+-ATPase,
and
amino
represents
antibodies
for
One antibody,
Because
characterized.
tested
conjugated
6).
FITC
monoclonal
(11-15
of a (10).
4g6HLLVMKGAPER506
five
to
7 and 85 the
bound
peptide antibody
BIOCHEMICAL
Vol. 148, No. 1, 1987
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
I.07
cE
.8 -
: E T B 0 2 0 Li 0
.6 -
.4 -
.2 -
rl 123456709 PEPTIDE
NUMBER
Determination of Monoclonal Antibody M8-Pl-A3 Binding to Synthetic ps. ntibody binding to peptide-BSA conjugates was determined using the solidsurface adsorption assay and a B-galactosidase sheep anti-mouse IgG F(ab')p conjugate as second antibody. Monoclonal antibody concentration was 1 uM. The sequence regions for each of the a peptides were: (1) 1-12; (2) 16-30; (3) 111-122; (4) 303-314; (5) 366-377; (6) 496-506; (7) 823-833; (8) 932-943; and (9) 1,003-1,013. achieved
were
that
antibody
body
binding
Competition
similar. binding to both
to
holoenzyme
plate-adsorbed
binding "in
studies solution"
enzyme
ANTl6ODY
[M8-P
(Fig. effectively
and peptide
1 -A3)
3) then
6-BSA
demonstrated
prevented conjugate.
antiThese
nk&
Determination of M8-Pl-A3 Binding to Antigen as a Function of iii&&Y Concentration. bpen circles (0) and closed circles (0) represent antibody binding to Na+,K+-ATPase and peptide 6-BSA conjugate, respectively. All values are given as the percentage of antibody binding relative to the maxlmum amount bound to Antibody binding to antlgen was detected using a each particular antigen. solid-surface adsorption assay. Antigen was adsorbed to the plates at 50 pg/well (Na+,K+-ATPase) and 5 uglwell (peptide 6-BSA conjugate) and bound antibody quantitated using B-galactosidase sheep anti-mouse IgG F(ab')2 conjugate. 248
Vol. 148, No. 1, 1987
8lOCHEMlCALAND8lOPHYSlCALRESEARCH
200
COMMUNICATIONS
400
[N~+.K+-ATPw~J
pglml
;ig. 3.1 Competition Binding Study. pen c rcles (0) and closed circles (9) show decrease in M8-Pl-A3 binding to plate adsorbed Na+,K+-ATPase and peptide 6-BSA conjugate, respectively, after exposure to varying concentrations of Na+,K+-ATPase. Antibody concentration was 10 nM. Plate adsorbed antigen concentrations were 50 pg/well, Na+,K+-ATPase and 5 ug/Well, peptide 6-BSA conjugate. Binding of antibody to Na+,K+-ATPase in solution phase occurred before exposing antibody to either solid-surface bound peptide 6-BSA conjugate or Na+,K+-ATPase.
results this
showed binding
gens.
Having
dies
a
high
(pNPPase) binding
data In
binding
addition,
its
effects studies
FITC-modified
of
> native
ligand
to both were
enzyme
(9)
antibody
M8-Pl-A3
various not
data
and
holoenzyme.
also
plate-adsorbed
native
enzyme
determined.
(>50:1)
was;
was
no
conditions
that anti-
and
peptide
In these
stu-
because
our
curves
plate-adsorbed Excess
showed
isolated
antibody
was
a >
found
to
p-nitrophenylphosphatase
effect
(Mg2+;
used
binding
Kt-dependent had
and
the
competition
affinity
or
Na+,K+-ATPase
of
function
to
Na+,K+-ATPase
activity. under
Mg'+Pi,
FITC,
on
on enzyme
titer
holoenzyme effect
binding
antibody
order
plate-adsorbed no
of
"native"
recognition
antibody
binding
relative
recognized
to antibody
effects
ratio or
the
antibody
established
antibody
"affinity"
have
the
corresponded
conjugate,
that
that
on
the
Mgz+ATP;
rate
of
ouabain
K+Na+Mgz+ATP;
and
shown). since
the
on FITC were enzyme
done,
antibody
was binding
fluorescence
were
as before,
exactly
as
which it
249
did
to
the
investigated. showed
that
to
unlabeled
same region First, M8-Pl-A3
of a as
competition bound
enzyme.
to the Next,
Vol. 148,No. fluorescence enzyme
spectroscopy
(in
bound
BIOCHEMICAL
1.1987
Tris-HCl
measurements
buffer)
Further,
probe. fluorescence
intensity
bound
antibody.
These
enzyme
moiety not
of
and
(since
epitope
and
on the
it
by
clear
Na+ were that
environment
to
addition
of
the
of
of the in
effected
by
was the
regulatory
the
decreases
not
M8-Pl-A3
the
to
intensity
dependent
perturbing
responses
binding
fluorescence
reversal
made
nor
antibody
and Mg*+* ouabain
their
results
its
it
for
is antibody
mational
changes.
antibody
and enzyme
ligands
ditions the
where
and
of
little
state
neither
fluorescent ligands
(data
that
centration
bound
the
different
binding
in
the
changes.
shows
of enzyme
presence than
Mg*+Pi
20X,
was
M8-Pl-A3
the
not
4 clearly in
free
conditions, Mg*+Pi
was required
that
binding
solution
the
we found
that
Nat
as
a reduction
data
from this the
the
absence
conforenzyme
by
binding
sen-
concentration
of
To achieve a
in
demonstrated
enzyme's
illustrates
increased.
if
the
displaced
had
contrast,
caused
to
required
in the
we found
These
antibody is
bound,
addition, Mg*+ATP
addition con-
In
sensitive
was
Figure
of
to
respectively.
enzyme
the
Using
antibody.
and
conforin which
was determined.
to antibody
Mg*+,
decrease ligand
the
prior
region
enzyme's
or after
was enzyme
bound
the
exposed
of experiments
before
antibody
of
be an in
by a series
or Mg*+ATP
level
to
involved
of M8-PI-A3
18 and to
not
1 h either
Mg*+Pi
on the
conformational It
Mg*+,
but
but
for
70-753
35,
is
of unbound
effect
binding
under
level
combined
M8-Pl-A3
sitivity.
combined
K+,
appeared
was tested
were
75% to
enzyme,
concept
the
from
mational these
that
no effect
Kt had
that
accessible)
were
Na+,
and ligands
binding
therefore,
approximately
addition
enzyme
M8-Pl-A3,
This
and then
essentially
body
Mg*+Pi
that
shown). The
of
K+,
function,
FITC
showed
had no effect
the
FITC
altering
AND BiOPHYSlCALRESEARCHCOMMUNlCATlONS
four-fold of added
50% antihigher
con-
ligands.
DISCUSSION These represents ligand-induced
data
demonstrate
the
epitope conformational
that for
the
monoclonal or
tertiary 250
sequence
region
antibody structural
496-506
M8-Pl-A3,
of
a,
undergoes
rearrangements
which some which
Vol. 148,No.
1. 1987
8lOCHEMlCALAND8IOPHYSlCALRESEARCHCOMMUNICATlONS
Effect of ligands on antibody binding to Na+,K+-ATPase. w e ecreasing curves show the ability of Na+,K+-ATPase under various ligand conditions to compete for MB-Pl-A3 binding to plate adsorbed (SDS-treated) enzyme. Open circles (0) show Na+,K+-ATPase concentrations in Tris-HCl buffer only; Open triangles (A) buffer plus Mg2+; Open squares (Cl) buffer plus Mgz+ATP; and Closed triangles (A) buffer plus Mg2+Pi. Antibody (1.5 pg/ml) and enzyme binding was done for 1 hr at 4OC before the centrifugation step was done.
alter
M8-Pl-A3
binding.
bound
antibody.
displace effect
on either
the
M8-Pl-A3
but not with enzymes
the
are
for
are
of
native
rat in
not.
are
or
the
this
that
(9).
The
these
rat
we
to
has
which
kidney
acid
their
two
antibody
Further,
amino
while
however,
changes
denatured
region,
bound
FITC.
with
Nevertheless,
sufficient,
ligand-induced
enzyme-linked
enzyme
not
we find
cross-reacts
identical
figurations
function,
intensity
that
changes
In addition,
enzyme
fluorescence
interest
These
no
alter
find
it
of
Na+,K+-ATPase
sequences of these
apparent
enzymes
have
is
involved
tertiary
similar
con-
affinities
ATP (12). We therefore
binding the
or
hydrolysis.
Lys-501
(and
fluorescein
appears
to the
group. fluorescein
must site)
group result
of from
ATP-binding This
this
region
given
the
in
the
proximity
order
for
it
to serve
FITC.
The
region
rather also
is
fixing
is
than
consistent
a competitive
inhibitor 251
the
in
either
adenine-binding
site
reactive
site
of
ATPase
activity
the
in
the
a position modification
with
the with
ATP
ATP and FITC,
as the
FITC from
between
of
inactivation
irreversibly
not
interactions
reside in
hypothesis
derivative,
that
However,
residue
thiocyanate
block
conclude
fact respect
for
then
to
sterically
of
the
that
the
lysine
eosin,
to ATP,
and it
a
Vol. 148,No. inhibits
ATPase
seems
likely
emission This
that
to
-SH groups
(14).
of
effected
by the in
important
regions
shift the
using
is
is
the but
not
Lys-719 actual
sequence
at
These
difference
5'iodoacetamido-
with
intensity
higher
several
to
con-
different
changes
results
not.
and the
a 20-fold
reacts
does
this
the
least
techniques
regions
two ATP analogues distant
a
(18).
portions
of
require
from
It
eosin's
repositioned
results to
yet
FITC
by ATP and enzyme
(15,16).
involved
have been
from
the
ATP
shown
analogous
activity
identify
to
is
emphasize
not
the
dif-
functionally
The
ATP binding
be any
site
they
but
alkylating
(FSBA)
may not
have
at amino
(ClRATP)
adenosine regions
binding
to react
benzylamide-ATP
These the
in
Lys-501.
5'-(p-fluorosulfonyl)benzoyl of
is
(13).
of a,
while
FITC
clearly
blocked
enzyme
same region
contrast
requires
modification
the
binding,
fluorescence
y[4-(N-2-chlorethyl-N-methylamino)] and
in
COMMUNiCATlONS
of proteins.
considerably
(17)
upon
and
labeling
chemical
the
effects
which
shows
labeling
at
Lys residue
This
it
modifying
functional
Na+,K+-ATPase
covalent
Currently established
a red
derivative
its
ficulties
bind
labeling
Though
FITC,
chemically
locations.
label
AND BIOPHYSICALRESEARCH
probes
two probes'
(5'-IAF)
centration
dues
upon
specific
fluorescein
two
undergoes
in the
their
without
these
spectra
suggests
those
activity
that
differences in
BIOCHEMICAL
1, 1987
are
acid
ATP reacts
at
more
not
analogue
Cys-656 to
additional
resi-
at Asp-710
the
likely
been
and
represent
regions
that
investigation.
ACKNOWLEDGEMENTS We thank
Purabi
assistance.
This
ROl-HL-32214
(WJB).
Dey
work
was
WJB is
and
Chuck
Loftice
supported
by
an Established
for NIH
grants
Investigator
their
excellent T32-HL-07382 of
the
technical (MLF)
American
Heart
Association.
REFERENCES 1.
Racker, E. (1985) Reconstitutions Pathological St!
of Transporters
252
and Receptors,
and
and
Vol. 148, No. 1, 1987
2. 3. 4. 5. 6. 7. 8. 9.
10. 11. 12. 13. 14. 15. 16. 17.
18.
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
Farley, R.A., Tran, C.M., Carilli, C.T., Hawke, D, and Shively, J.E. (1984) J. Biol. Chem. 259, 9532-9535. Lane, L.K., Potter, J.D, and Collins, J.H. (1979) Prep. Biochem. 9, 157-170. Schwartz, A., Allen, J.C. and Harigaya, S. (1969) J. Pharmacol. Exp. Ther. 168, 31-41. Ball, W.J. (1986) Biochemistry 25, 7155-7162. Wallick, E.T. and Schwartz, A. (1974) J. Biol. Chem. 249, 5141-5147. Hegyvary, C. and Jorgensen, P.L. (1981) J. Biol. Chem. 256, 62966303. Ball, W.J., Schwartz, A. and Lessard, J.L. (1982) Biochim. Biophys. Acta 719, 413-423. Bal1,W.J. and Lane, L.K. (1986) Biochim. Biophys. Acta 873, 79-87. Ball, W.J. and Loftice, C.D. (1987) In press. Kirley, T.L., Wang, T., Wallick, E.T. and Lane, L.K. (1985) Biochem. Biophys. Res. Comnun. 130, 732-738. Periyasamy, S.M., Huang, W.H. and Askari, A. (1983) Comp. Biochem. Physiol. 76B(3), 449-454. Skou, J.C. and Esmann, M. (1981) Biochim. Biophys. Acta 647, 232-240. Steinberg, M. and Kirley, T. Unpublished results. Kapakos, J.G. and Steinberg, M. (1986) J. Biol. Chem. 261, 2084-2089. Kapakos, J.G. and Steinberg, M. (1986) J. Biol. Chem. 261, 2090-2095. Ovchinnikov, Yu.A., Dzhandzugazyan, K.N., Lutsenko, S.V., Mustayev, A.A. and Modyanov, N.N. (1987) FEBS Letters 217, 111-116. Ohta, T., Nagano, K. and Yoshida, M. (1986) Proc. Nat'1 Acad. Sci. USA 83, 2071-2075.
253
BIOCHEMICAL
1, 1987
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS Pages 246-253
14, 1987
Imnunochemical
Evidence
Na+,K+-ATPase
W.J.
Department
that
is
Ball
the
Not the
, Jr.
and M.L.
Cincinnati,
Site
Biophysics,
College
Ohio
on
Friedman
and Cell
of Cincinnati
Site
ATP Binding
of Pharmacology
University
FITC-labeling
of Medicine,
45267-0575
Received August 25, 1987 The covalent labeling of the a subunit of lamb fluorescein 5'-isothiocyanate at Lys-501 has generally at the ATP binding site. We have found that 496HLLVMKGAPER506 serves as the antigenic determinant M&Pl-A3: This antibody binds to both native and while this epitope undergoes ligand-induced changes involved in either enzyme function or the El * E2 monitored by FITC-fluorescence intensity. 0 1987 Academic
Na+,K+-ATPase
is
nit
(-100,DDO
and
the
maintenance
Mr) of
class
of ATP-driven
whose
functioning
ferent
conformations.
(FITC)
has been
has been fic
found
lysine
among
thought
and
to
monoclonal antibody
B subunit
(-50,000
Na+ levels
in
the
of the
The
cycling fluorescent
extensively
inactivate
to the
in a region
antibody
of the
pumps.
ATP blocks
Because FITC
of
the
M&Pl-A3
binds
function
and
enzyme
enzyme's
ATP to
0 I987
by Academic
of reproduction
in any
Press, form
Inc. reserved.
the
246
site
region
a subu-
function belongs
is to a
as ElE2 a series
pumps, of dif-
changes. by labeling is
a 1:l of
the
5'-isothiocyanate
which with
site
ligand-induced
between
activity
reacts
binding
(1)
ligand-induced
100 KD protein
this
enzyme
fluorescein
ATPase
labeling,
This
enzymes
these
FITC
primary
by Racker
probe study
Inc.
whose
cell.
involves
0006-291X/87$1.50 Copyright All rights
the
Press,
of two subunits,
Mr),
designated
be a portion
on
composed
transporters,
ElEp-ATPase
ATP binding
enzyme,
ion
used to
the
K+ and
residue
the
a membrane
kidney Na+,K+-ATPase by been assumed to occur the peptide sequence for monoclonal antibody FITC-labeled enzyme and these changes are not conformational changes
a speci-
highly
conserved
stoichiometry
labeling
is
(2).
We have
of a.
The effect
conformational
FITC
to
generally found
that
of
bound
changes
has
Vol. 148,No.
been
8lOCHEMlCALAND8lOPHYSlCALRESEARCH
1, 1987 The
investigated.
Na+,K+-ATPase
have also
EXPERIMENTAL
PROCEDURES
effects
of
these
ligands
COMMUNICATIONS
on
antibody
binding
to
been determined.
Enzyme preparation and assays. The Na+,K+-ATPase was prepared from frozen lamb kidneys as previously described by Lane et al (3). The Na+,K+-ATPase activity at 37'C was measured at 340 nm using the spectrophotometric, linked enzyme assay system of Schwartz et al (4) while the Kt-dependent p-nitrophenylphosphatase activity was determined by continuous measurement at 410 nm (5). [3H]-ouabain binding to the enzyme was determined at 37'C essentially as The labeling of Na+,K+-ATPase with described by Wallick and Schwartz (6). FITC (Molecular Probes, Inc.) has been described in our previous work (5), measurements were measured at 520 nm as while the fluorescence intensity described by Hegyvary and Jorgensen (7). Antibody M8-Pl-A3 preparation and binding determinations. This antibody was raised against the lamb kidney Na+,K+-ATPase and its isolation, purification and initial characterization was reported previously by Ball et al. (8). The indirect solid-surface adsorption (ELISA) assay used to quantitate antibody binding has been described in detail (8) but we have modified the proceIn this procedure antibody and enzyme were combined for l-2 h dure somewhat. and then the enzyme and any antibody-enzyme complex formed were removed from The unbound M8-Pl-A3 (in solution by centrifugation at 150,000 x g for 1 h. the supernatant) was then exposed to either untreated microtiter plates (Cooke flexible plates), plates previously coated with enzyme (+ 0.1% SDS), or synthetic peptide-BSA conjugates. M8-Pl-A3 binding to these plates was then quantitated using a B-galactosidase sheep anti-mouse IgG F(ab')2 conjugate as Solution phase binding of M8-Pl-A3 to the enzyme under second antibody. (Na +; Kt; Mg2+; Mg2+Pi and Mg2+ATP, all at 5 mM) was various ligand conditions also examined. RESULTS A collection Na+,K+-ATPase synthetic portions
of (9)
peptides
were
This
sequence
has
been
isolated,
(2,ll).
site
of
holoenzyme nM antibody, was about
Figure peptide
this the 2 6-BSA
respectively. 12-fold
lower
residues
a soluble
tryptic
and
to
shows
of
was achieved affinity
enzyme, 247
(Fig.
this
of the
the maximum
the
region
binding at
of
labeling of
levels
for
further
M8-Pl-A3
for of
a that
ATP binding
approximately antibody
peptide
site
was
of
of
sequence
1,
fragment
a portion
kidney
various
to the
(BSA)
covalent
to
lamb
a series
to bind
half-maximal
conjugate
for
be the
the
representing
digestion
M8-Pl-A3
that
the
length)
albumin
may comprise
binding
to recognize
was found
serum
region
to
in
M8-Pl-A3,
shown
raised
ability
bovine
While than
their
acid
to
sequenced
Na+,K+-ATPase,
and
amino
represents
antibodies
for
One antibody,
Because
characterized.
tested
conjugated
6).
FITC
monoclonal
(11-15
of a (10).
4g6HLLVMKGAPER506
five
to
7 and 85 the
bound
peptide antibody
BIOCHEMICAL
Vol. 148, No. 1, 1987
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
I.07
cE
.8 -
: E T B 0 2 0 Li 0
.6 -
.4 -
.2 -
rl 123456709 PEPTIDE
NUMBER
Determination of Monoclonal Antibody M8-Pl-A3 Binding to Synthetic ps. ntibody binding to peptide-BSA conjugates was determined using the solidsurface adsorption assay and a B-galactosidase sheep anti-mouse IgG F(ab')p conjugate as second antibody. Monoclonal antibody concentration was 1 uM. The sequence regions for each of the a peptides were: (1) 1-12; (2) 16-30; (3) 111-122; (4) 303-314; (5) 366-377; (6) 496-506; (7) 823-833; (8) 932-943; and (9) 1,003-1,013. achieved
were
that
antibody
body
binding
Competition
similar. binding to both
to
holoenzyme
plate-adsorbed
binding "in
studies solution"
enzyme
ANTl6ODY
[M8-P
(Fig. effectively
and peptide
1 -A3)
3) then
6-BSA
demonstrated
prevented conjugate.
antiThese
nk&
Determination of M8-Pl-A3 Binding to Antigen as a Function of iii&&Y Concentration. bpen circles (0) and closed circles (0) represent antibody binding to Na+,K+-ATPase and peptide 6-BSA conjugate, respectively. All values are given as the percentage of antibody binding relative to the maxlmum amount bound to Antibody binding to antlgen was detected using a each particular antigen. solid-surface adsorption assay. Antigen was adsorbed to the plates at 50 pg/well (Na+,K+-ATPase) and 5 uglwell (peptide 6-BSA conjugate) and bound antibody quantitated using B-galactosidase sheep anti-mouse IgG F(ab')2 conjugate. 248
Vol. 148, No. 1, 1987
8lOCHEMlCALAND8lOPHYSlCALRESEARCH
200
COMMUNICATIONS
400
[N~+.K+-ATPw~J
pglml
;ig. 3.1 Competition Binding Study. pen c rcles (0) and closed circles (9) show decrease in M8-Pl-A3 binding to plate adsorbed Na+,K+-ATPase and peptide 6-BSA conjugate, respectively, after exposure to varying concentrations of Na+,K+-ATPase. Antibody concentration was 10 nM. Plate adsorbed antigen concentrations were 50 pg/well, Na+,K+-ATPase and 5 ug/Well, peptide 6-BSA conjugate. Binding of antibody to Na+,K+-ATPase in solution phase occurred before exposing antibody to either solid-surface bound peptide 6-BSA conjugate or Na+,K+-ATPase.
results this
showed binding
gens.
Having
dies
a
high
(pNPPase) binding
data In
binding
addition,
its
effects studies
FITC-modified
of
> native
ligand
to both were
enzyme
(9)
antibody
M8-Pl-A3
various not
data
and
holoenzyme.
also
plate-adsorbed
native
enzyme
determined.
(>50:1)
was;
was
no
conditions
that anti-
and
peptide
In these
stu-
because
our
curves
plate-adsorbed Excess
showed
isolated
antibody
was
a >
found
to
p-nitrophenylphosphatase
effect
(Mg2+;
used
binding
Kt-dependent had
and
the
competition
affinity
or
Na+,K+-ATPase
of
function
to
Na+,K+-ATPase
activity. under
Mg'+Pi,
FITC,
on
on enzyme
titer
holoenzyme effect
binding
antibody
order
plate-adsorbed no
of
"native"
recognition
antibody
binding
relative
recognized
to antibody
effects
ratio or
the
antibody
established
antibody
"affinity"
have
the
corresponded
conjugate,
that
that
on
the
Mgz+ATP;
rate
of
ouabain
K+Na+Mgz+ATP;
and
shown). since
the
on FITC were enzyme
done,
antibody
was binding
fluorescence
were
as before,
exactly
as
which it
249
did
to
the
investigated. showed
that
to
unlabeled
same region First, M8-Pl-A3
of a as
competition bound
enzyme.
to the Next,
Vol. 148,No. fluorescence enzyme
spectroscopy
(in
bound
BIOCHEMICAL
1.1987
Tris-HCl
measurements
buffer)
Further,
probe. fluorescence
intensity
bound
antibody.
These
enzyme
moiety not
of
and
(since
epitope
and
on the
it
by
clear
Na+ were that
environment
to
addition
of
the
of
of the in
effected
by
was the
regulatory
the
decreases
not
M8-Pl-A3
the
to
intensity
dependent
perturbing
responses
binding
fluorescence
reversal
made
nor
antibody
and Mg*+* ouabain
their
results
its
it
for
is antibody
mational
changes.
antibody
and enzyme
ligands
ditions the
where
and
of
little
state
neither
fluorescent ligands
(data
that
centration
bound
the
different
binding
in
the
changes.
shows
of enzyme
presence than
Mg*+Pi
20X,
was
M8-Pl-A3
the
not
4 clearly in
free
conditions, Mg*+Pi
was required
that
binding
solution
the
we found
that
Nat
as
a reduction
data
from this the
the
absence
conforenzyme
by
binding
sen-
concentration
of
To achieve a
in
demonstrated
enzyme's
illustrates
increased.
if
the
displaced
had
contrast,
caused
to
required
in the
we found
These
antibody is
bound,
addition, Mg*+ATP
addition con-
In
sensitive
was
Figure
of
to
respectively.
enzyme
the
Using
antibody.
and
conforin which
was determined.
to antibody
Mg*+,
decrease ligand
the
prior
region
enzyme's
or after
was enzyme
bound
the
exposed
of experiments
before
antibody
of
be an in
by a series
or Mg*+ATP
level
to
involved
of M8-PI-A3
18 and to
not
1 h either
Mg*+Pi
on the
conformational It
Mg*+,
but
but
for
70-753
35,
is
of unbound
effect
binding
under
level
combined
M8-Pl-A3
sitivity.
combined
K+,
appeared
was tested
were
75% to
enzyme,
concept
the
from
mational these
that
no effect
Kt had
that
accessible)
were
Na+,
and ligands
binding
therefore,
approximately
addition
enzyme
M8-Pl-A3,
This
and then
essentially
body
Mg*+Pi
that
shown). The
of
K+,
function,
FITC
showed
had no effect
the
FITC
altering
AND BiOPHYSlCALRESEARCHCOMMUNlCATlONS
four-fold of added
50% antihigher
con-
ligands.
DISCUSSION These represents ligand-induced
data
demonstrate
the
epitope conformational
that for
the
monoclonal or
tertiary 250
sequence
region
antibody structural
496-506
M8-Pl-A3,
of
a,
undergoes
rearrangements
which some which
Vol. 148,No.
1. 1987
8lOCHEMlCALAND8IOPHYSlCALRESEARCHCOMMUNICATlONS
Effect of ligands on antibody binding to Na+,K+-ATPase. w e ecreasing curves show the ability of Na+,K+-ATPase under various ligand conditions to compete for MB-Pl-A3 binding to plate adsorbed (SDS-treated) enzyme. Open circles (0) show Na+,K+-ATPase concentrations in Tris-HCl buffer only; Open triangles (A) buffer plus Mg2+; Open squares (Cl) buffer plus Mgz+ATP; and Closed triangles (A) buffer plus Mg2+Pi. Antibody (1.5 pg/ml) and enzyme binding was done for 1 hr at 4OC before the centrifugation step was done.
alter
M8-Pl-A3
binding.
bound
antibody.
displace effect
on either
the
M8-Pl-A3
but not with enzymes
the
are
for
are
of
native
rat in
not.
are
or
the
this
that
(9).
The
these
rat
we
to
has
which
kidney
acid
their
two
antibody
Further,
amino
while
however,
changes
denatured
region,
bound
FITC.
with
Nevertheless,
sufficient,
ligand-induced
enzyme-linked
enzyme
not
we find
cross-reacts
identical
figurations
function,
intensity
that
changes
In addition,
enzyme
fluorescence
interest
These
no
alter
find
it
of
Na+,K+-ATPase
sequences of these
apparent
enzymes
have
is
involved
tertiary
similar
con-
affinities
ATP (12). We therefore
binding the
or
hydrolysis.
Lys-501
(and
fluorescein
appears
to the
group. fluorescein
must site)
group result
of from
ATP-binding This
this
region
given
the
in
the
proximity
order
for
it
to serve
FITC.
The
region
rather also
is
fixing
is
than
consistent
a competitive
inhibitor 251
the
in
either
adenine-binding
site
reactive
site
of
ATPase
activity
the
in
the
a position modification
with
the with
ATP
ATP and FITC,
as the
FITC from
between
of
inactivation
irreversibly
not
interactions
reside in
hypothesis
derivative,
that
However,
residue
thiocyanate
block
conclude
fact respect
for
then
to
sterically
of
the
that
the
lysine
eosin,
to ATP,
and it
a
Vol. 148,No. inhibits
ATPase
seems
likely
emission This
that
to
-SH groups
(14).
of
effected
by the in
important
regions
shift the
using
is
is
the but
not
Lys-719 actual
sequence
at
These
difference
5'iodoacetamido-
with
intensity
higher
several
to
con-
different
changes
results
not.
and the
a 20-fold
reacts
does
this
the
least
techniques
regions
two ATP analogues distant
a
(18).
portions
of
require
from
It
eosin's
repositioned
results to
yet
FITC
by ATP and enzyme
(15,16).
involved
have been
from
the
ATP
shown
analogous
activity
identify
to
is
emphasize
not
the
dif-
functionally
The
ATP binding
be any
site
they
but
alkylating
(FSBA)
may not
have
at amino
(ClRATP)
adenosine regions
binding
to react
benzylamide-ATP
These the
in
Lys-501.
5'-(p-fluorosulfonyl)benzoyl of
is
(13).
of a,
while
FITC
clearly
blocked
enzyme
same region
contrast
requires
modification
the
binding,
fluorescence
y[4-(N-2-chlorethyl-N-methylamino)] and
in
COMMUNiCATlONS
of proteins.
considerably
(17)
upon
and
labeling
chemical
the
effects
which
shows
labeling
at
Lys residue
This
it
modifying
functional
Na+,K+-ATPase
covalent
Currently established
a red
derivative
its
ficulties
bind
labeling
Though
FITC,
chemically
locations.
label
AND BIOPHYSICALRESEARCH
probes
two probes'
(5'-IAF)
centration
dues
upon
specific
fluorescein
two
undergoes
in the
their
without
these
spectra
suggests
those
activity
that
differences in
BIOCHEMICAL
1, 1987
are
acid
ATP reacts
at
more
not
analogue
Cys-656 to
additional
resi-
at Asp-710
the
likely
been
and
represent
regions
that
investigation.
ACKNOWLEDGEMENTS We thank
Purabi
assistance.
This
ROl-HL-32214
(WJB).
Dey
work
was
WJB is
and
Chuck
Loftice
supported
by
an Established
for NIH
grants
Investigator
their
excellent T32-HL-07382 of
the
technical (MLF)
American
Heart
Association.
REFERENCES 1.
Racker, E. (1985) Reconstitutions Pathological St!
of Transporters
252
and Receptors,
and
and
Vol. 148, No. 1, 1987
2. 3. 4. 5. 6. 7. 8. 9.
10. 11. 12. 13. 14. 15. 16. 17.
18.
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
Farley, R.A., Tran, C.M., Carilli, C.T., Hawke, D, and Shively, J.E. (1984) J. Biol. Chem. 259, 9532-9535. Lane, L.K., Potter, J.D, and Collins, J.H. (1979) Prep. Biochem. 9, 157-170. Schwartz, A., Allen, J.C. and Harigaya, S. (1969) J. Pharmacol. Exp. Ther. 168, 31-41. Ball, W.J. (1986) Biochemistry 25, 7155-7162. Wallick, E.T. and Schwartz, A. (1974) J. Biol. Chem. 249, 5141-5147. Hegyvary, C. and Jorgensen, P.L. (1981) J. Biol. Chem. 256, 62966303. Ball, W.J., Schwartz, A. and Lessard, J.L. (1982) Biochim. Biophys. Acta 719, 413-423. Bal1,W.J. and Lane, L.K. (1986) Biochim. Biophys. Acta 873, 79-87. Ball, W.J. and Loftice, C.D. (1987) In press. Kirley, T.L., Wang, T., Wallick, E.T. and Lane, L.K. (1985) Biochem. Biophys. Res. Comnun. 130, 732-738. Periyasamy, S.M., Huang, W.H. and Askari, A. (1983) Comp. Biochem. Physiol. 76B(3), 449-454. Skou, J.C. and Esmann, M. (1981) Biochim. Biophys. Acta 647, 232-240. Steinberg, M. and Kirley, T. Unpublished results. Kapakos, J.G. and Steinberg, M. (1986) J. Biol. Chem. 261, 2084-2089. Kapakos, J.G. and Steinberg, M. (1986) J. Biol. Chem. 261, 2090-2095. Ovchinnikov, Yu.A., Dzhandzugazyan, K.N., Lutsenko, S.V., Mustayev, A.A. and Modyanov, N.N. (1987) FEBS Letters 217, 111-116. Ohta, T., Nagano, K. and Yoshida, M. (1986) Proc. Nat'1 Acad. Sci. USA 83, 2071-2075.
253