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Stability of isoproterenol bound to cyanogen bromide-activated agarose
Vol. 64, No. 3, 1975
BIOCHEMICAL
STABILITY
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
OF ISOPROTERENOL BOUND TO CYANOGEN BROMIDE-ACTIVATED
G. VAUQUELIN*,
M.-L.
LACOMBE**,
J.
AGAROSE. HANOUNE** and A.D.
STROSBERG'.
*Laboratorium Chemie der Proteinen, V.U.B., St. Genesius Rode 1640, Belgium. **Unite
Received
April
de Recherches Mondor, 94010
INSERM U-99, H8pital CrGteil, France.
Henri
24,1975
SUMMARY. The chemical stability and release of isoproterenol bound by diazotation to an insoluble agarose matrix has been investigated. It is demonstrated, by a double labeling procedure ([3H]isoproterenol and [14C]spacer arm), that the bound ligand is readily released in a soluble form. This occurs primarily through a chemical hydrolysis of the arm-linked ligand from the cyanogen bromide-activated agarose, and can be observed under extensive washing procedures as well as under more "physiological" incubation conditions. The instability of the agarose-arm linkage should lead to a critical analysis of physiological effects obtained with agarose bound hormones in vitro.
Peptides spacer
arm,
and small
to a solid
reportedly
released
physiological light
hormones
were
in vitro.
from
upon used
This
of free
matrix
(4),
et al
of this the
coupled we report that
link
strongly
at pH above
incubation to glass here
the release
to the instability
various
has been
Tesser
explained
this
5. Finally,
beads
(12).
Using
from
the agarose
of the agarose-arm
C&right D I9 75 b.v Aradenzic Press. Irx All rights of reproduction in ar?y form resewed.
for
from
coupling
spacer
the
arm and
Experiments
suggesting
by
a tlsolvolyse"
the
labeled
ligand
[3H]catecholamines arm and isoproterenol,
together,
in our conditions,
linkage. 1076
11).
labeled
are released matrix,
(6,
exchange
reported
desorption
used for
between
hypothesis,
differently
arm and hormone
immobilized systems
by the simple
suggested
tritium
under
whereby
azo-bond
of linkage
was also
supported
or incubation
are
has shed a new and (8-10)
either
a single
beads,
or subcellular
of the
Cleavage
or through
or agarose
storage
cellular
medium was recently
that
glass
approaches
or by the cleavage
to the spacer arm (11). (glass beads or agarose)
with
during
technical
ligand matrix
(6)
directly,
Such a phenomenon
to stimulate
release
ligand
matrix
(l-7).
several
coupled
such as porous
this
conditions
critical
molecules
which is
suggests mostly
due
Vol. 64, No. 3, 1975
EXPERIMENTAL
BIOCHEMICAL
PROCEDURE. MATERIALS.
dl-isoproterenol
was from Aldrich.
were
p-Nitrobenzylazide
from Merck.
and solvents (2.11
were
Ci/mmole)
was obtained HCl (7.95
by the
Sepharose
4B was suspended
dissolved
in a minimal stirred
from New England
in
from
for
prepared were
buffer
24 h at 4".
prepared
by the
dark
at 4" for unreacted
2-3
0.1 M phosphate at 4" for
buffer
groups
with
with
was determined
spectrometer.
The release
and incubation After
Data
conditions
washing,
containing from
with
stored (v/v).
the literature
report
water.
75 mg glycine,
was
obtained
in
stirred water.
in
the
In order
to
IO ml of in the dark
Labeled
gels
and [ 14C] -ethylenediamine of the gel preparation.
a Packard
0.5 % n-butanol
suspension
was stirred
50 ml distilled
Tri-Carb
ligand
liquid
under
in the legends
at 4" in
the dark,
the coupling
to the
scintillation
was followed
as depicted
gelswere
solution
100 ml distilled
of the bound
This
pH 4, to the previously
obtained by adding [3~] -isoproterenol compounds at the corresponding steps
Radioactivity
to 50 mg of
the gel was suspended
(pH 8) containing
24 h and then washed
with
Isoproterenol-agarose
This (14),
of
funnel
of 18.1 mg of dl-iosproterenol
buffer,
days and washed
diazonium
to the
p-aminobenzamidoethyl-agarose (13).
addition
added
on a glass
pH 10, and added
The diazotized
of washed
pH 11 by addition
washed
to Cuatrecasas
p-aminobenzamidoethyl-agarose.
block
around
was
bromide,
were
in 5 ml of the same buffer.
according
weight)
250 mg cyanogen
the gel was rapidly
in 20 ml of 0.1 M acetate
RESULTS.
[U-14C]Centre
Agarose
One gram (wet
and adjusted
diazotized
figures.
bromide reagents
Co. and
conjugates.
method.
dissolved
pH 4.8,
Nuclear
other
dZ-' lsoproterenol
[7-3H]
of dimethylformamide,
at 5-10"
dissolved
stirred
washing
All
the Radiochemical
10 ml water.
amount
0.5 M carbonate
ethylenediamine
conjugates
bromide
20 min,
25 ml of cold,
were cold
available.
Ci/mmole),
cyanogen
slurry
1 N NaOH. After
gently
grade
from Pharmacia.
and cyanogen
was from Eastman.
of isoproterenol-agarose
activated
was then
4B was obtained
England).
METHODS. Preparation
gently
Sepharose
Dimethylformamide
of the purest
ethylenediamine, (Amersham,
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
various
to the in 100 mM EDTA,
of catecholamines,
such as epinephrine and isoproterenol, to diazonium agarose and diazonium glass beads at pH 7.5 (2,9,15). However, under these conditions, the coupling
is
the formation whereas
accompanied
of pyrocatechol
the highest
pH 4 (data
by several,
yield
to be published).
unexpected
azoderivative of isoproterenol Thus
in order
1077
side-reactions as well
azoderivative to obtain
leading
as other is
to
by-products, observed
a maximal
amount
at of
Vol. 64, No. 3, 1975
the expected
BIOCHEMICAL
conjugate
(9),
AND BIOPHYSICAL
the coupling
RESEARCH COMMUNICATIONS
step was routinely
performed
at
pH 4. The release conditions. double
To elucidate
labeling
mine
of free
for
and bound
the "true"
procedure
hormones
mechanism
to prepare
the gels
the
spacer arm and [3H] isoproterenol both [ 14 C] labeled arm and tritiated
contained agarose.
Under
activity
was not
this
bound,
condition,
Structure agarose
of the conjugate
it
but
only
of release, (Table for
I):
[14c]
ethylenediaThus gel
that
bound
part
Content (pmoles/g
t
Gel II
2
Gel III Symbols
"A-B-N2-*IPR (agarose
*A
0.03
III
I3113 1.5
0.35
used: [14C]-ethylenediamine;
-*A
I I:
I .a5
and gel
in labeled products gel) before washing
*IPR
$A-B-NH~
*A:
Table
alone)
*A + "IPR
to the
of the radio-
Gel II
t4c1 Gel I
various
the hormone.
on the gel.
Labeled products adsorbed
under we used a
hormone
was possible adsorded
was studied
Structure
"IPX:
[3H]-isoproterenol.
i)H -Band labeling
’
“IPR -
of the gels.
Gel I was prepared as described under "Methods". Gel II was prepared by the treatment of inert agarose (not activated by cyanogen bromide) with [14C]-ethylenediamine, followed by the other steps described under of p-aminobenzamidoethyl "Methods". Gel III was prepared b treatment agarose (not diazotized) with [ 37H -1PR and by the subsequent steps described under "Methods". The specific activit 7 of L3Hl isoproterenol was 2.7 Ci/mole for gel I and III and that of [ 4C] ethylenediamine was 240 and 40 mCi/mole for gel I and II respectively.
1078
I
Vol. 64, No. 3, 1975
were
prepared
native
BIOCHEMICAL
to correct
[14c]
ethylenediamine
to be only
adsorded.
of unbound
material
subtract calculate
for
it
from
This
from
gel
with
10 mM HCl.
from gel
II.
allowed
release
As shown in Fig.
observed
of bound during
Almost
When the release
contained which
were
us to measure
washing
gel
I.
considered
the "desorption"
and incubation from
respectively
steps
and to
Thus we could
material.
1, appreciable
I and III,
they
isoproterenol
the various
release
released
possibility:
procedure
the total
and then
this
and [3H]
during
the actual
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
amounts
washing,
first
no release
of isoproterenol with
80 percent
of ethylenediamine
of chemically
bound
were methanol
was observed
isoproterenol
and spacer
1234123456
1
2
3
4 WASHING
....*.-.*.*. ..“(-I ....*.*.*.*.* .*. ..*. 1...*-*.**** .n....*..... *. 1
2
3
4
5
6
!sTEP!s
Fig.. The washing steps were performed as follows: one g of agarose conjugate (prepared as depicted in Table I) was suspended in 40 ml methanol-water (4:1, v/v), and shaken for 48 h at 4" in the dark. The gel was filtered on a Millipore filter disc (0.45 n pore size). The filtrate was collected and counted. The washing procedure was repeated in similar conditions for several times with either 40 ml methanol-water 4:1, v/v) or 10 mM Xl. Total amount of[l4C] arm (O--W* for gel I) and b H] isoproterenol (O -0 for gel I, and O---Ofor gel III) present in each washing solution is given as percent of their molar concentration in the original gel before washing. These concentrations were calculated from the specific activity data given in the legend to Table I. No release of [14C] arm adsorded to gel II was observed under this washing procedure. Insert: Release of bound[3H] isoproterenol (ol ) and bound [14C]arm was calculated from data in Fig. 1 by subtracting the amount (0 ---0) due to desorption (gel III) from the total amount of release (gel I).
1079
Vol. 64, No. 3, 1975
BIOCHEMICAL
arm was corrected original
molar
and
solutions:
0.6
10 mM HCl,
than
that
[14C]
the
step
was used
washing
for
an important
percent
level
for
each washing
after
five
essentially
It
step.
I percent
3 times
release
higher
the first
seems therefore
arm and matrix
of the hormone
Upon washing for
that
when 80 % methanol
catecholamine-agarose
arm and bound
[3H]
washing
was about
from
steps.
between
the innnobilized part
released
decreased
of the of
in the methanol
for
Furthermore,
this
release
of labeled
materials
(10 min at 37')
used
As shown in Table
renol
were
This
suggests
II,
released
(0.17
that,
during
Radioactivity from
gel
complex,
whereas
was due to the cleavage
isoproterenol
gel
III
13H]from
gel
I minus
from gel
II:
double
labeling
method also
for
when
10 mM HCl was
indicated
occurred
that
during
the adenylate
the
cyclase
similar
amounts
of [ 14C] arm and ['H]
and 0.18
percent
of the initial
incubation
under
released
I (total
[3H]from
Table
release which
between
incubations
[14C]
released
as percent proportions
washing.
appreciable
[3H]
similar
of isoproterenol
additional
of the azo-linkage
17).
-arm were
to 0.1 percent occurred
and expressed
1, insert),
of ethylenediamine
the cleavage
time
(Fig.
to 0.7
with
used
the desorption
amount
isoproterenol
washing
for
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
molar
"physiologicalnconditions,
Percent
of the original amount
short
assay
(16,
isoproteamount). as
molar
0.23
release)
0.06
(desorption) L3H] from
gel
III
0.17
I
Ligand
release
during
incubation.
After the washing steps described in Fig. 1, 60 mg aliquots of gel and III (prepared as described in the legend to Table I) were suspended in 1 ml of incubation medium containing 50 mM Tris-HCl buffer pH 7.4, 3 mM MgC12 and 0.5 mM ATP. The suspensions were shaken for 10 min at 37" and the supernatants were removed after centrifugation and counted. The total amount of labeled material present in gel I before incubation was 1.4 pmole/g gel for the [14C] arm, 0.9 pmole/g gel for [3H] to as 100 percent. Values depicted isoproterenol, and was referred are means of four experiments.
1080
I
BIOCHEMICAL
Vol. 64, No. $1975
well
as during
washing
arm and matrix. amount
with
of arm-bound
ligand
to give
a final
represents
a contamination
system
(16,
methanol,
in Table
released
procedure
were
also
described
settled
unbound
isoproterenol
release
of bound
DISCUSSION.
Several
mation
have
the
process,
we observed.
of the hormone
should
of "bound"
physiological be exercized
ligand
of membrane detrimental
is
it
adenylate to affinity
of ligand-binding
for
et a2 (6)
release lead
authors,
of the radio-
to a slight
obviously
. An by
by these
explain
conditions(Table
when interpreting in biological
proteins binding
could
bond,
overesti-
the
from agarose-bound hormones by free, and In fact, since this "chemical" release
cyclase.Release chromatography,
receptor methods
cannot
desorption of arm-bound
reported
described
arm
of ligand
of the arm-agarose
of the total
arm
labeled part
whereas
has been
was due
spacer
release
to by Tesser
incubation
studied
Thus,
the
release
between
washing,
hormone
phenomenon but
from to assess
this
the major
the conditions
of the supernatant active, material. under
that
instability
5 percent This
that
arm itself.
alluded
under
release
of ligand designed
linkages
by extensive
the tritiated
at most
caution
spacer
already
from
of adsorded
by the use of differently evidence
due to the
represent
does occur
study,
observed.
material.
a release
was suggested
of
whereas
presently the level
especially
It
one
desorption
percent)
of the bound
reported
now direct
occur,
(0.02
II,
to that
and iminocarbonate
However,
that
release
purpose,
a continuous flow of 12 1 the subsequent incubation
diminished
incubations
et aZ (12).
contamination physiologically
Alternative
the
with
of tritium
would
procedure
be eliminated
by a "solvolytic"
it
cyclase
to the extensive
For this
to Table
comparable
In this
could
can still
activity
was This
shown)
(4).
with During
was minimal
washing
provide
NaCl.
II
of isourea
together
ligand
Venter
between the total
the adenylate not
and Kaplan
was washed
of the gels.
(6,ll).
released
exchange
that
10 min incubation
(data
in the caption
gel
during
activity
and agarose
ligand
the
remained
authors
carriers,
and hormone,we free
from
affecting
to the cleavage
is
described
column
without
biological
was calculated
to stimulate
by Venter
material
extensive
insoluble
occurred
of 0.1 PM isoproterenol.
submitted
in a column,
the conditions
material
a cleavage
17).
gram of gel,
Thus,
it
during
concentration
of 0.1 M HCl and 18 1 of 0.8 percent under
II,
susceptible
Gel I and III washing
80 percent
From the data
sufficient
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
experiments systems
of arm-bound especially are
ligands
1081
II), where
the effect
such as the activation ligand
might
when very
to be selectively to insoluble
great
matrix,
also
small
be amounts
purified. e.g.
the use
of
Vol. 64, No. 3, 1975
BIOCHEMICAL
of macromolecular suitable,
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
arms or epoxy-activated
and are now under
Sepharose,
are conceivably
more
investigation.
ACKNOWLEDGMENTS. We are grateful
to Drs. E. Kanarek and P. Berthelot for helpful and valuable discussion of this study. This work was supported by the "Institut National de la Sante et de la Recherche Medicale" and by the "DelBgation G&-&r-ale ?i la Recherche Scientifique et Technique". G.V. is aspirant of the "National Fonds voor WetenschappeliJkOnderzoek".
REFERENCES
I.
TESSER, G.I.,
2. YONG, M.S.
FISCH, (1973)
3. VAUQUELIN, G., Hoppe-Seyler's 4. VENTER, J.C. 5. YONG, M.S.
H.U.
and SCHWYZER, R. (1972)
Science,
182,
3,
(1974)
and RICHARDSON, J.B. FISCH,
H.U.
56-58.
157-158.
HANOUNE, J. and STROSBERG, A.D. LACOMBE, M.-L., Z. Physiol. Chem., 335, 1263. and KAPLAN, N.O.
6. TESSER, G.I., Is, 1718-1730.
FEBS Lett.,
Science,
(1974)
185,
Science,
and SCHWYZER, R.
459-460.
185,
(1974)
(1974)
460-461.
Helvetica
Chimica
7. KOLB, H.J., RENNER, R., HEPP, K.D., WEISS, L. and WIELAND, O.H. Proc. Nat. Acad. Sci. USA, 72, 248-252. 8. CUATRECASAS, P. (1969)
Proc.
Nat.
Acad.
9. VENTER, J.C., DIXON, J.E., MAROKO, P.R. Nat. Acad. Sci. USA, 69, 1141-1145. HABER, E. and O'HARA, 10. LEFKOWITZ, R.J., USA, 2, 2828-2832. 11. CUATRECASAS, P. and PARIKH, 12. VENTER, J.C., 1-9.
ARNOLD, L.J.
13. CUATRECASAS, P. (1970) 14. WELIKY,
N. and WEETALL,
15. VENTER, J.C., ROSS, J., (1973) Proc. Nat. Acad.
I.
D. (1972)
245,
(1975)
17. HANOUNE, J., (in press).
and PECKER, F.
LACOMBE, M.-L.
1082
Nat.
Proc.
Acad.
2291-2299.
Mol.
Pharmacol.
Sci.
fl,
3059-3065.
DIXON, J.E., MAYER, S.E. Sci. USA, 70, 1214-1217. PERRENOUD, M.-L.
(1972)
11,
Immunochemistry,
16. LERAY, F., CHAMBAUT, A.-M., J, Biochem., 3&, 185-192.
(1975)
450-457.
Proc.
Biochemistry,
Chem., (1965)
USA, 63,
and KAPLAN, N.O.
and KAPLAN, N.O.
J. Biol. H.H.
(1972)
Sci.
Acta,
2, 293-322. and KAPLAN, N.O.
and HANOUNE, J. (1975)
J.
Biol.
(1973)
Chem.
Eur.
BIOCHEMICAL
STABILITY
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
OF ISOPROTERENOL BOUND TO CYANOGEN BROMIDE-ACTIVATED
G. VAUQUELIN*,
M.-L.
LACOMBE**,
J.
AGAROSE. HANOUNE** and A.D.
STROSBERG'.
*Laboratorium Chemie der Proteinen, V.U.B., St. Genesius Rode 1640, Belgium. **Unite
Received
April
de Recherches Mondor, 94010
INSERM U-99, H8pital CrGteil, France.
Henri
24,1975
SUMMARY. The chemical stability and release of isoproterenol bound by diazotation to an insoluble agarose matrix has been investigated. It is demonstrated, by a double labeling procedure ([3H]isoproterenol and [14C]spacer arm), that the bound ligand is readily released in a soluble form. This occurs primarily through a chemical hydrolysis of the arm-linked ligand from the cyanogen bromide-activated agarose, and can be observed under extensive washing procedures as well as under more "physiological" incubation conditions. The instability of the agarose-arm linkage should lead to a critical analysis of physiological effects obtained with agarose bound hormones in vitro.
Peptides spacer
arm,
and small
to a solid
reportedly
released
physiological light
hormones
were
in vitro.
from
upon used
This
of free
matrix
(4),
et al
of this the
coupled we report that
link
strongly
at pH above
incubation to glass here
the release
to the instability
various
has been
Tesser
explained
this
5. Finally,
beads
(12).
Using
from
the agarose
of the agarose-arm
C&right D I9 75 b.v Aradenzic Press. Irx All rights of reproduction in ar?y form resewed.
for
from
coupling
spacer
the
arm and
Experiments
suggesting
by
a tlsolvolyse"
the
labeled
ligand
[3H]catecholamines arm and isoproterenol,
together,
in our conditions,
linkage. 1076
11).
labeled
are released matrix,
(6,
exchange
reported
desorption
used for
between
hypothesis,
differently
arm and hormone
immobilized systems
by the simple
suggested
tritium
under
whereby
azo-bond
of linkage
was also
supported
or incubation
are
has shed a new and (8-10)
either
a single
beads,
or subcellular
of the
Cleavage
or through
or agarose
storage
cellular
medium was recently
that
glass
approaches
or by the cleavage
to the spacer arm (11). (glass beads or agarose)
with
during
technical
ligand matrix
(6)
directly,
Such a phenomenon
to stimulate
release
ligand
matrix
(l-7).
several
coupled
such as porous
this
conditions
critical
molecules
which is
suggests mostly
due
Vol. 64, No. 3, 1975
EXPERIMENTAL
BIOCHEMICAL
PROCEDURE. MATERIALS.
dl-isoproterenol
was from Aldrich.
were
p-Nitrobenzylazide
from Merck.
and solvents (2.11
were
Ci/mmole)
was obtained HCl (7.95
by the
Sepharose
4B was suspended
dissolved
in a minimal stirred
from New England
in
from
for
prepared were
buffer
24 h at 4".
prepared
by the
dark
at 4" for unreacted
2-3
0.1 M phosphate at 4" for
buffer
groups
with
with
was determined
spectrometer.
The release
and incubation After
Data
conditions
washing,
containing from
with
stored (v/v).
the literature
report
water.
75 mg glycine,
was
obtained
in
stirred water.
in
the
In order
to
IO ml of in the dark
Labeled
gels
and [ 14C] -ethylenediamine of the gel preparation.
a Packard
0.5 % n-butanol
suspension
was stirred
50 ml distilled
Tri-Carb
ligand
liquid
under
in the legends
at 4" in
the dark,
the coupling
to the
scintillation
was followed
as depicted
gelswere
solution
100 ml distilled
of the bound
This
pH 4, to the previously
obtained by adding [3~] -isoproterenol compounds at the corresponding steps
Radioactivity
to 50 mg of
the gel was suspended
(pH 8) containing
24 h and then washed
with
Isoproterenol-agarose
This (14),
of
funnel
of 18.1 mg of dl-iosproterenol
buffer,
days and washed
diazonium
to the
p-aminobenzamidoethyl-agarose (13).
addition
added
on a glass
pH 10, and added
The diazotized
of washed
pH 11 by addition
washed
to Cuatrecasas
p-aminobenzamidoethyl-agarose.
block
around
was
bromide,
were
in 5 ml of the same buffer.
according
weight)
250 mg cyanogen
the gel was rapidly
in 20 ml of 0.1 M acetate
RESULTS.
[U-14C]Centre
Agarose
One gram (wet
and adjusted
diazotized
figures.
bromide reagents
Co. and
conjugates.
method.
dissolved
pH 4.8,
Nuclear
other
dZ-' lsoproterenol
[7-3H]
of dimethylformamide,
at 5-10"
dissolved
stirred
washing
All
the Radiochemical
10 ml water.
amount
0.5 M carbonate
ethylenediamine
conjugates
bromide
20 min,
25 ml of cold,
were cold
available.
Ci/mmole),
cyanogen
slurry
1 N NaOH. After
gently
grade
from Pharmacia.
and cyanogen
was from Eastman.
of isoproterenol-agarose
activated
was then
4B was obtained
England).
METHODS. Preparation
gently
Sepharose
Dimethylformamide
of the purest
ethylenediamine, (Amersham,
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
various
to the in 100 mM EDTA,
of catecholamines,
such as epinephrine and isoproterenol, to diazonium agarose and diazonium glass beads at pH 7.5 (2,9,15). However, under these conditions, the coupling
is
the formation whereas
accompanied
of pyrocatechol
the highest
pH 4 (data
by several,
yield
to be published).
unexpected
azoderivative of isoproterenol Thus
in order
1077
side-reactions as well
azoderivative to obtain
leading
as other is
to
by-products, observed
a maximal
amount
at of
Vol. 64, No. 3, 1975
the expected
BIOCHEMICAL
conjugate
(9),
AND BIOPHYSICAL
the coupling
RESEARCH COMMUNICATIONS
step was routinely
performed
at
pH 4. The release conditions. double
To elucidate
labeling
mine
of free
for
and bound
the "true"
procedure
hormones
mechanism
to prepare
the gels
the
spacer arm and [3H] isoproterenol both [ 14 C] labeled arm and tritiated
contained agarose.
Under
activity
was not
this
bound,
condition,
Structure agarose
of the conjugate
it
but
only
of release, (Table for
I):
[14c]
ethylenediaThus gel
that
bound
part
Content (pmoles/g
t
Gel II
2
Gel III Symbols
"A-B-N2-*IPR (agarose
*A
0.03
III
I3113 1.5
0.35
used: [14C]-ethylenediamine;
-*A
I I:
I .a5
and gel
in labeled products gel) before washing
*IPR
$A-B-NH~
*A:
Table
alone)
*A + "IPR
to the
of the radio-
Gel II
t4c1 Gel I
various
the hormone.
on the gel.
Labeled products adsorbed
under we used a
hormone
was possible adsorded
was studied
Structure
"IPX:
[3H]-isoproterenol.
i)H -Band labeling
’
“IPR -
of the gels.
Gel I was prepared as described under "Methods". Gel II was prepared by the treatment of inert agarose (not activated by cyanogen bromide) with [14C]-ethylenediamine, followed by the other steps described under of p-aminobenzamidoethyl "Methods". Gel III was prepared b treatment agarose (not diazotized) with [ 37H -1PR and by the subsequent steps described under "Methods". The specific activit 7 of L3Hl isoproterenol was 2.7 Ci/mole for gel I and III and that of [ 4C] ethylenediamine was 240 and 40 mCi/mole for gel I and II respectively.
1078
I
Vol. 64, No. 3, 1975
were
prepared
native
BIOCHEMICAL
to correct
[14c]
ethylenediamine
to be only
adsorded.
of unbound
material
subtract calculate
for
it
from
This
from
gel
with
10 mM HCl.
from gel
II.
allowed
release
As shown in Fig.
observed
of bound during
Almost
When the release
contained which
were
us to measure
washing
gel
I.
considered
the "desorption"
and incubation from
respectively
steps
and to
Thus we could
material.
1, appreciable
I and III,
they
isoproterenol
the various
release
released
possibility:
procedure
the total
and then
this
and [3H]
during
the actual
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
amounts
washing,
first
no release
of isoproterenol with
80 percent
of ethylenediamine
of chemically
bound
were methanol
was observed
isoproterenol
and spacer
1234123456
1
2
3
4 WASHING
....*.-.*.*. ..“(-I ....*.*.*.*.* .*. ..*. 1...*-*.**** .n....*..... *. 1
2
3
4
5
6
!sTEP!s
Fig.. The washing steps were performed as follows: one g of agarose conjugate (prepared as depicted in Table I) was suspended in 40 ml methanol-water (4:1, v/v), and shaken for 48 h at 4" in the dark. The gel was filtered on a Millipore filter disc (0.45 n pore size). The filtrate was collected and counted. The washing procedure was repeated in similar conditions for several times with either 40 ml methanol-water 4:1, v/v) or 10 mM Xl. Total amount of[l4C] arm (O--W* for gel I) and b H] isoproterenol (O -0 for gel I, and O---Ofor gel III) present in each washing solution is given as percent of their molar concentration in the original gel before washing. These concentrations were calculated from the specific activity data given in the legend to Table I. No release of [14C] arm adsorded to gel II was observed under this washing procedure. Insert: Release of bound[3H] isoproterenol (ol ) and bound [14C]arm was calculated from data in Fig. 1 by subtracting the amount (0 ---0) due to desorption (gel III) from the total amount of release (gel I).
1079
Vol. 64, No. 3, 1975
BIOCHEMICAL
arm was corrected original
molar
and
solutions:
0.6
10 mM HCl,
than
that
[14C]
the
step
was used
washing
for
an important
percent
level
for
each washing
after
five
essentially
It
step.
I percent
3 times
release
higher
the first
seems therefore
arm and matrix
of the hormone
Upon washing for
that
when 80 % methanol
catecholamine-agarose
arm and bound
[3H]
washing
was about
from
steps.
between
the innnobilized part
released
decreased
of the of
in the methanol
for
Furthermore,
this
release
of labeled
materials
(10 min at 37')
used
As shown in Table
renol
were
This
suggests
II,
released
(0.17
that,
during
Radioactivity from
gel
complex,
whereas
was due to the cleavage
isoproterenol
gel
III
13H]from
gel
I minus
from gel
II:
double
labeling
method also
for
when
10 mM HCl was
indicated
occurred
that
during
the adenylate
the
cyclase
similar
amounts
of [ 14C] arm and ['H]
and 0.18
percent
of the initial
incubation
under
released
I (total
[3H]from
Table
release which
between
incubations
[14C]
released
as percent proportions
washing.
appreciable
[3H]
similar
of isoproterenol
additional
of the azo-linkage
17).
-arm were
to 0.1 percent occurred
and expressed
1, insert),
of ethylenediamine
the cleavage
time
(Fig.
to 0.7
with
used
the desorption
amount
isoproterenol
washing
for
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
molar
"physiologicalnconditions,
Percent
of the original amount
short
assay
(16,
isoproteamount). as
molar
0.23
release)
0.06
(desorption) L3H] from
gel
III
0.17
I
Ligand
release
during
incubation.
After the washing steps described in Fig. 1, 60 mg aliquots of gel and III (prepared as described in the legend to Table I) were suspended in 1 ml of incubation medium containing 50 mM Tris-HCl buffer pH 7.4, 3 mM MgC12 and 0.5 mM ATP. The suspensions were shaken for 10 min at 37" and the supernatants were removed after centrifugation and counted. The total amount of labeled material present in gel I before incubation was 1.4 pmole/g gel for the [14C] arm, 0.9 pmole/g gel for [3H] to as 100 percent. Values depicted isoproterenol, and was referred are means of four experiments.
1080
I
BIOCHEMICAL
Vol. 64, No. $1975
well
as during
washing
arm and matrix. amount
with
of arm-bound
ligand
to give
a final
represents
a contamination
system
(16,
methanol,
in Table
released
procedure
were
also
described
settled
unbound
isoproterenol
release
of bound
DISCUSSION.
Several
mation
have
the
process,
we observed.
of the hormone
should
of "bound"
physiological be exercized
ligand
of membrane detrimental
is
it
adenylate to affinity
of ligand-binding
for
et a2 (6)
release lead
authors,
of the radio-
to a slight
obviously
. An by
by these
explain
conditions(Table
when interpreting in biological
proteins binding
could
bond,
overesti-
the
from agarose-bound hormones by free, and In fact, since this "chemical" release
cyclase.Release chromatography,
receptor methods
cannot
desorption of arm-bound
reported
described
arm
of ligand
of the arm-agarose
of the total
arm
labeled part
whereas
has been
was due
spacer
release
to by Tesser
incubation
studied
Thus,
the
release
between
washing,
hormone
phenomenon but
from to assess
this
the major
the conditions
of the supernatant active, material. under
that
instability
5 percent This
that
arm itself.
alluded
under
release
of ligand designed
linkages
by extensive
the tritiated
at most
caution
spacer
already
from
of adsorded
by the use of differently evidence
due to the
represent
does occur
study,
observed.
material.
a release
was suggested
of
whereas
presently the level
especially
It
one
desorption
percent)
of the bound
reported
now direct
occur,
(0.02
II,
to that
and iminocarbonate
However,
that
release
purpose,
a continuous flow of 12 1 the subsequent incubation
diminished
incubations
et aZ (12).
contamination physiologically
Alternative
the
with
of tritium
would
procedure
be eliminated
by a "solvolytic"
it
cyclase
to the extensive
For this
to Table
comparable
In this
could
can still
activity
was This
shown)
(4).
with During
was minimal
washing
provide
NaCl.
II
of isourea
together
ligand
Venter
between the total
the adenylate not
and Kaplan
was washed
of the gels.
(6,ll).
released
exchange
that
10 min incubation
(data
in the caption
gel
during
activity
and agarose
ligand
the
remained
authors
carriers,
and hormone,we free
from
affecting
to the cleavage
is
described
column
without
biological
was calculated
to stimulate
by Venter
material
extensive
insoluble
occurred
of 0.1 PM isoproterenol.
submitted
in a column,
the conditions
material
a cleavage
17).
gram of gel,
Thus,
it
during
concentration
of 0.1 M HCl and 18 1 of 0.8 percent under
II,
susceptible
Gel I and III washing
80 percent
From the data
sufficient
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
experiments systems
of arm-bound especially are
ligands
1081
II), where
the effect
such as the activation ligand
might
when very
to be selectively to insoluble
great
matrix,
also
small
be amounts
purified. e.g.
the use
of
Vol. 64, No. 3, 1975
BIOCHEMICAL
of macromolecular suitable,
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
arms or epoxy-activated
and are now under
Sepharose,
are conceivably
more
investigation.
ACKNOWLEDGMENTS. We are grateful
to Drs. E. Kanarek and P. Berthelot for helpful and valuable discussion of this study. This work was supported by the "Institut National de la Sante et de la Recherche Medicale" and by the "DelBgation G&-&r-ale ?i la Recherche Scientifique et Technique". G.V. is aspirant of the "National Fonds voor WetenschappeliJkOnderzoek".
REFERENCES
I.
TESSER, G.I.,
2. YONG, M.S.
FISCH, (1973)
3. VAUQUELIN, G., Hoppe-Seyler's 4. VENTER, J.C. 5. YONG, M.S.
H.U.
and SCHWYZER, R. (1972)
Science,
182,
3,
(1974)
and RICHARDSON, J.B. FISCH,
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56-58.
157-158.
HANOUNE, J. and STROSBERG, A.D. LACOMBE, M.-L., Z. Physiol. Chem., 335, 1263. and KAPLAN, N.O.
6. TESSER, G.I., Is, 1718-1730.
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185,
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7. KOLB, H.J., RENNER, R., HEPP, K.D., WEISS, L. and WIELAND, O.H. Proc. Nat. Acad. Sci. USA, 72, 248-252. 8. CUATRECASAS, P. (1969)
Proc.
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9. VENTER, J.C., DIXON, J.E., MAROKO, P.R. Nat. Acad. Sci. USA, 69, 1141-1145. HABER, E. and O'HARA, 10. LEFKOWITZ, R.J., USA, 2, 2828-2832. 11. CUATRECASAS, P. and PARIKH, 12. VENTER, J.C., 1-9.
ARNOLD, L.J.
13. CUATRECASAS, P. (1970) 14. WELIKY,
N. and WEETALL,
15. VENTER, J.C., ROSS, J., (1973) Proc. Nat. Acad.
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17. HANOUNE, J., (in press).
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2291-2299.
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DIXON, J.E., MAYER, S.E. Sci. USA, 70, 1214-1217. PERRENOUD, M.-L.
(1972)
11,
Immunochemistry,
16. LERAY, F., CHAMBAUT, A.-M., J, Biochem., 3&, 185-192.
(1975)
450-457.
Proc.
Biochemistry,
Chem., (1965)
USA, 63,
and KAPLAN, N.O.
and KAPLAN, N.O.
J. Biol. H.H.
(1972)
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Acta,
2, 293-322. and KAPLAN, N.O.
and HANOUNE, J. (1975)
J.
Biol.
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Eur.