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[3H] corticosterone binding activity of adrenal incubation media in response to in vivo and in vitro ACTH stimulation
BIOCHEMICAL
Vol. 90, No. 4, 1979 October
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
29, 1979
[I3H
Pages
CORTICOSTERONE BINDING ACTIVITY
1355-1363
OF ADRENAL INCUBATION MEDIA
IN RESPONSE TO --IN VIVO AND IN VITRO ACTH STIMULATION J.
Departments Received
F. Pritchett*, W. L. Harper, D. N. Marple .I. T. Bradley, and M. L. Till
of Zoology-Entomology Agricultural Experiment
September
20,
and Animal Science; Auburn University Station; Auburn, Alabama 36830
1979 SUMMARY
ad nistration of ACTH upon --in vitro The influence of --in vivo or --in vitro binding adrenal corticosterone production as well as % ] corticosterone ACTH, regardless of the activity of incubation media have been examined. route of administration, significantly elevated corticosterone during an initial incubation period. During initial incubation periods ACTH also elevatedPI%] corticosterone binding activity of the incubation media. Ensuing incubations were characterized by either a marked decline in binding activity (in -- vivo ACTH administration) or a marked decline with sn attendant negative correlation between binding activity and ACTH level. Corticosteroidogenic response to ACTH remained intact during ensuing incubations. The data suggest the existence of an ACTH-sensitive intraglandular corticosterone binding ligand(s), the activity or concentration of which is dramatically altered by incubation protocol and time of sacrifice. INTRODUCTION Competitive
protein
binding
coids
routinely
involve
an initial
might
otherwise
compete
with
tated.
Such extractions
dichloromethane Since cortical were
our laboratory
expected
modify
plasma
corticoid *To whom all
values
rather
obtained
correspondence
assay
performed
involved
tedious
with
for
the steroid
in our
laboratory
determination
plasma
corti-
proteins being
which
quanti-
utilizing
incubation
corticoid
of --in vitro
concentrations
of plasma
media,
extraction
step.
proteins
in incubation However
samples
adreno-
we attempted
quantification
from non-extracted should
for
(1).
in adrenal for
procedures
to remove binding
protein
to ACTH and since
CPB procedures the
the
by Murphy is
to be minimal
by eliminating
radioassay
extraction
have been
as described
responsiveness
(CPB)
were
comparisons consistently
to media of lower
be addressed
0006-291X/79/201355-09$01.00/0 1355
Copyright All rights
@ I979
by Academic Press, Inc. in any form reserved
of reproduction
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL
than those obtained from the samesamples extracted Furthermore these differences in vitro gland.
RESEARCH COMMUNICATIONS
with dichloromethane.
appeared to be related not only to the specific
incubation method employed but also to the functional These findings prompted us to investigate
tissue in incubation may liberate and/or activity
status of the
the possibility
a corticoid-binding
ligand,
that adrenal
the concentration
of which is dependent not only upon incubation protocol but
also upon exposure of the tissue to ACTH. MATBHIALSANDMETHODS Animals and incubation
procedures
Male Sprague-Dawley rats 85 to 90 days of age were utilized. Prior to experimental procedures all animals were housed 3 per cage at an ambient temperature of 24 + .5OC with a photoperiod of 14 hours light:10 hours darkness Animals were provided with Purina Laboratory Chow (lights on at 0730 hours). and tap water -ad libitum. Wo hours prior to sacrifice, animals were transferred to individual cages. For determination of --in vitro and -in vivo responses to ACTUadministered in vivo, animals were injected subcutaneously 60 minutes prior to sacrifice with either 0.5 ml 0.9% NaCl or 0.5 ml 0.9% NaCl containing either 1 or 3 IU AC'JX (Nutritional Biochemicals). Animals utilized for study of in vitro response to --in vitro administration of ACTHor for determination of time of sacrifice upon corticosterone binding activity were allow to remain undisturbed until time of sacrifice. All animals were decapitated between either 0945-1015 or 1945-2015 hours. Trunk blood was collected from only the latter group for subsequent determination of plasma corticosterone. Adrenal glands from each animal were rapidly removed to a dish of cold (3-5OC) Krebs Ringer Bicarbonate solution (KRBC) and trimmed of extraneous tissue. Glands were then quartered, rinsed thoroughly in KRBC, and incubated in a Dubnoff metabolic incubator (37OC, 60 oscillations/ min., 95% 02-5% CO2atmosphere). To assess the influence of -in vivo ACTHon --in vitro corticosterone secretion and binding activity, glands were incubated for an initial 60 minutes in 2 ml KRBCcontaining 2 mg glucose/ml (KRBG). Following the initial incubation periods, glands were transferred to a second 60 minute incubation in 2 ml fresh KRBG. For study of the influence of time of sacrifice upon corticosterone binding activity, an initial incubation only was performed. Following each incubation period, media were decanted into glass vials and frozen (-2OoC). To determine the influence of --in vitro administration of ACTUupon in vitro corticosterone secretion and media binding activity, gland quartersfrom each animal were incubated for an initial 60 minutes in 2 ml KRBGor in a like volume of KKBGfortified with either 50, 200 or 400 milliunits/ml ACTU (Sigma At the end of the first incubation period, glands not initially Biochemicals). exposed to ACTUwere transferred to 2 ml fresh KRBG containing 50, 200, or 400 milliunits/ml ACTS and incubated for an additional 60 minute period. All incubation media were collected and frozen as before. Corticosterone
determination
in plasma and incubation media
Assay of incubation media and plasma samples for corticosterone was accomplished via the CPB radioassay described by Murphy (1, 2) utilizing rabbit serum as the source of the binding ligand and 1, 2 PH] corticosterone
1356
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Both plasma samples and aliquots of (New England Nuclear) as the radiolabel. incubation media were extracted with dichloromethane l/10 (v/v) prior to corticosterone determination. Separation of bound from free corticoid was accomplished by charcoal adsorption. The bound fraction was counted (Searle Isocap/ 300) in a scintillation cocktail of toluene-Triton X (2:l) with Omnifluor (6 grams/liter). Interand intra-assay variabilities were less than 7% and 5% respectively. Incubation
medium binding
activity
Aliquots of incubation medium were filtered utilizing a Millipore apparatus To remove endogenous corticosterone and filters (type HA, pore size = 0.45 um). from the samples, 500 ul portions of media were each added to an equal volume of 2.5% dextran-coated charcoal in phosphate buffered saline (PBS), and with constant agitation, were brought to and maintained at 45'C for 30 minutes. Samples were then centrifuged (2-3'C) for 30 minutes (2000 X g) and the supernatants were filtered as before, twice. Removal of endogenous corticosterone was confirmed via CPB assay of portions of the filtered fraction. Binding studies were performed in duplicate upon 500 pl aliquots of each sample. Tritiated corticosterone (specific activity = 136.9 mCi/mg) was added in 100 pl of PBS; DPM added per assay tube are indicated in the tables and figure. The mixture was vortexed and then incubated at 45'C for 10 minutes. Samples were then cooled to 2-3OC and maintained for a 10 minute period. Separation of free from bound isotope was via charcoal adsorption (500 pl added) followed by centrifugation (2000 X g for 20 minutes, 2-3OC). Bound isotope in 500 ~1 of supernatant was counted as before. Coefficients of determination for intraand inter-assay variability was less than 5%. To test the hypothesis that corticosterone binding activity of incubation' medium was influenced by extraction procedures, aliquots of corticosterone free incubation medium were incubated with isotope and then mixed l/10 (v/v) with dichloromethane and vortexed. The organic layer was removed. Free isotope from 400 ~1 aliquots of these samples as well as from 400 ul quantities of non-dichloromethane treated media samples and KRBG was removed as before and bound activity was quantitated as described above. RESULTS The effect activity
of incubation
previously
removed
a mean binding treated
compared
media is
activity,
to the KRBC-glucose
The action corticosterone 2.
of injected production
Both
upon
endogenous
in Table
1.
Although
greater
remained
terone
initial
had been
samples (p
<
exhibited
.05)
extraction in
binding
than
either
significantly
the treated
samples
as
blanks. ACTB upon --in vivo
1 and 3 IU levels concentration
corticosterone
corticosterone
dichloromethane
some activity
PI
Non-treated
was significantly
and corticosterone
corticosterone values,
from which
which
or blanks.
binding
extraction
illustrated
activity
samples
diminished
Table
of dichloromethane
within
incubation
produced
binding significant
one hour. levels
1357
plasma
were
corticosterone, activity elevations
Considering also
is
--in vitro
significantly
&vitro presented
in
in plasma corticoshigher
in the
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE Effect
of
dichloromethane binding activity
1
treatment upon of incubation
[&I] corticosterone media
Treatment
N
DPM Addeda
DPM Boundb
Nontreated
6
45750
894 t
Treated
6
45750
171 2 15d
Blank
6
45750
4Sc
75+ -
6e
aDPM added per determination; specific activity = 136.9 mCi/mg. bAll values represent DPM in 500 pl of supematant (means + SEM). cs ds eWithin the indicated column, values with different superscripts differ significantly (p ( 0.05).
TABLE Effect of secretion
Treatment
exogenous and[3H]
ACTH administered corticosterone
2
--in binding
vivo upon activity
corticosterone --in vitro of incubation mediaa.
Corticosterone Secretion (micrograms/hr)
DPM Boundb
N
Plasma Corticosterone (nanograms/ml)
Initial Incubation
Second Incubation
Initial Incubation
Second Incubation
Saline
Inject
6
195.9 + 34.1c
4.28 + .56c
4.71 + .52c
2379 f. 444c
1 Unit
ACTH
6
309.3 + 36.5d
6.22 + .4Bd
5.32 + .83c
3348 2 468d
6
321.5 + 48.5d
7.22 + .56d
4.13 f. .43c
3744 + 48gd
3 Units aAll
ACTH values
represent
means
group
of the second
as compared
to the
incubation,
no ACTH treatment
corticosterone incubation second
in response incubation,
in each below
binding
of the
that
activity
observed
saline-injected
837 + 153cse
the
significantly (p < 0.05). than DPM bound in
effects
However,
at the end
were
detected.
Tritiated
elevated
during
ACTH administration. on binding
activity
initial
incubation
1358
the
initial
At the end of the was apparent.
[‘HI corticosterone
incubations, during
9gcBe
of supematant;
group.
was significantly
to --in vivo
no ACTH effect second
1104 +
f. SEM.
b62250 DPM added per determination; DPM bound are per 500 nl specific activity = 136.9 mCi/mg. CsdWithin columns, values with different superscripts differ eDPM bound in second incubation significantly less (p < 0.01) initial incubation.
treated
642 + 135cBe
binding period.
Moreover,
was significantly
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL
TABLE Effect activity
of
upon PH] corticosterone binding during an initial incubationa.
Time
No.
Trial 1 2 3
2 2 2
2691 2475 2745
+ 156= T 144' z 135c
8:00
p.m.
1 2 3
2 2 2
3891 3993 3939
+ 144d + 204d + 60d
The influence
a single
media
exhibited
DPM bound are = 136.9 mCi/mg. values with (p < 0.05).
of sacrifice 60 minute
associated
significantly
killed
means + SEM. per determination; specific activity
the indicated colwm, differ significantly
of time
during
trials,
DPM Boundb
a.m.
cp dWithin scripts
all
N
1O:OO
aValues represent b60800 DPM added of supematsnt;
activity
3
time of sacrifice incubation media
of
Sacrifice
RESEARCH COMMUNICATIONS
incubation
with
less
(morning
animals
binding
per
super-
evening)
upon binding
is presented
activity
during than
pl
different
vs.
killed
500
in Table
3.
the morning
did
media
from
In
hours animals
at night. Regression
costerone
analyses
secretion
an initial without
upon
ACTH are given
in Figure
content
corticosterone
during
correlated
regression
line
Corticosterone
and negatively
for
ACTH level,
observed
for
equivalent
1.
Both were
an initial
less
of binding
Media
was also the slope
than
to --in vitro
activity during
1359
either incubation
activity
and
that
the initial
content
of
of and
the second
of the first
incu-
incubation.
incubation
ACTH level.
was significantly
corre-
positively
at the end of the second
correlated
ACTH levels
during
by an initial
period.
incubation although
corti-
and significantly
incubation
activity
binding
preceded
positively
second
and --in vitro
ACTH exposure
the degree
was significantly
significantly any given
incubation
to ACTH level
binding
binding
of --in vitro
of the media
at the end of the
significantly
corticosterone
the level
or a second
to ACTH level
bation
[3~]
incubation
corticosterone lated
of
was
Additionally less
incubation
than period.
that
Vol. 90, No. 4, 1979
BIOCHEMICAL
-0
5 ‘r
8
0
‘;^ 4am &E $i? a8 /‘:-
.Y
Incubation
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
1
i
-Incubation1 -
.---*Incubation
2 i
+l
2.
r s 50
400
200
In Vitro
ACTH
Dose
Level
(Milliunits/ml)
Figure 1. [%-I] Corticosterone binding activity of incubation media and corticosterone secretion in response to in vitro ACTH administration. Each point represents the mean with attendant SEM of 6 observations. Each line For represents the regression of the indicated variable upon ACTH dose level. each regression, an absolute value of the correlation coefficient (r)k .468 the slope of the regression line represents p < .05. For either variable, representing incubation 1 differs significantly (p < .025) from the corresponding value for incubation 2. *For either variable and within ACTH dose level, incubation 1 value differs significantly (p c.05) from incubation 2 value. For each determination of binding activity, 62250 DPMPH] corticosterone were added; DPM bound are per 500 pl of supematant; specific activity = 136.9 mCi/mg.
DISCUSSION Results activity
presented
of adrenal
of whether is presented
and refined
strongly
incubation
media
the ACTH is which
upon AC!JX and is --In vitro
herein
administered
suggests related
adrenal primarily
that
indicate in --in
response viva
the degree
to the specific incubation for
of binding
activity protocol
and protocols
binding
ACRID, regardless
Additionally
or in vitro.
of ACTH or for
1360
corticosterone
to exogenous
incubation
procedures
the bioassay
altered
is
evidence dependent
utilized. have been
studies
developed
on the mechanisms
Vol. 90, No. 4, 1979
BIOCHEMICAL
of corticosteroidogenesis. --in vitro Others
adrenal (4,
reliable
index
e,
provided
since
been
total
--in vivo
within
of both that
animal
out
degree
they
for
and constant
the gland
at the
medium shortly
tion)
periods
ACTH-induced
of response incubation (6)
systems
time
of sacrifice
as from
alterations
possible
physiological
isolated
cell
in which
study ensuing
observed
or constant
flow
systems
8).
incubations
were
would
present
have
into
cell within
out prior
initial
this
to
(preincubaConsequently,
whereas
rendered
-in
the incubation
period
be considered
the
recently
analyzed.
the preincubation
with-
to isolated
be washed from
of the
discarded
More
fluid
media
initial
altered
evolved
incubation
could
were
released
would
minute
which
extracellular materials
during
implications)
media
have
has or
by transfer
ACTH (7,
tissue
it
present
a 30-60
properties
to exogenous
-in
adrenocortical
employed
of the tissue
In the present as well
of --in vitro
to possess
and/or
preparation
factors
Preincubation
of adrenal
flow
after
ACTH treatment.
found
activity
from partial
of ACTH followed
medium.
can be a
However
obtained
therefore
the absence
--in vitro
immediately.
studies
elevated
of ACTS.
cortical
by extra-adrenal
ACTH have
were
adrenal
of data
Subsequently,
in
described
production
incubated
may be confounded
and uniformity
vi&protocols (9)
interpretation
ACTH-fortified
since
corticoid
is
first
administration
and ACTH-stimulated
that
period
(3)
to --in vitro
adrenal
tissue
to exogenous
to fresh analysis
that
adrenal
(6).
or pre-incubation
and coworkers
response
basal
systems
responsiveness
in
reported
suggested
the
tissue
Saffran
secretion
5) have
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
(and
the
the use of approach
unten-
able. Considering istration present media direct in
--in vivo
and --in vitro
of ACTH, a significant
stimulatory
as indicated levels
by elevated
of corticosterone
interest
the initial
injection
both
was the incubation
of the animal
plasma during
observation media, with
adrenal
response
corticosteroidogenic corticosterone
the initial
levels incubation
of corticosterone the magnitude
of which
ACTH and B) presumably
1361
binding
to in vivo admin-effect was and elevated period. activity
was A) related
dependent
upon the
Of more present to prior activity
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL
of the gland at or shortly
after
--in vivo glandular activity
and binding activity
binding activity
of initial
at night was significantly
RESEARCH COMMUNICATIONS
the time of sacrifice.
The relationship
of
is amplified by the fact that
incubation media associated with animals killed greater than that observed in samples obtained
during the mid-morning hours and hence corresponds to the time of maximal natural
activity.
Transfer of the tissue to and subsequent incubation without
in fresh medium
ACTHresulted in a moderate decline in corticosterone
ACTHtreated
groups to levels not different
from the saline injected
and may be due to the decay of the biological sharp decline in corticosterone
high level of binding activity to A) the functional
in the initial
of ACT&
group,
However, a
of all media occurred in both
It is therefore
possible that the relatively
incubation may have been related
status of the gland --in vivo with subsequent alterations
the composition of the extracellular
fluids
of death or B) the possible introduction mediumas a result
activity
binding activity
saline and ACTHtreated groups.
levels in the
in
of the gland before or at the time
of an intracellular
of tissue damageor secretion,
factor(s)
into the
the concentration(s)
of which
were AClX-dependent. To determine whether similar
alterations
obtained in response to ACTHadded directly
in binding activity
to the incubates (Figure l),
tissue was exposed to different
ACTHlevels either
immediately following
or during second incubations
incubations without
sacrifice
ACTS. In terms of corticoid
content of the media increased with AC'JI-Ilevel cating a continuing
capability
ACTH. During the initial was also positively
correlated
period,
to ACTHlevel.
the absence of ACTHand subsequent transfer only was binding activity
during initial
significantly
incubation but was also negatively
incubations
following
production,
initial
corticosterone
during either
in terms of corticoid
incubation
could be
incubation,
indi-
release in response to
corticosterone
binding activity
However, after
preincubation
to fresh ACID-fortified
medium, not
lower than observed during the initial
correlated
1362
in
to the level of ACTHexposure.
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL
Results obtained from these initial in binding activity not be directly
due to ACTRis an intraglandular
in response to ACTB after
than observed without preincubation seemslikely
incubations suggest that the elevation
dependent upon extraglandular
binding activity
phenomenonand thus may
ACTS actions -in vivo.
preincubation
and negatively
that a component essential
RESEARCH COMMUNICATIONS
ligand(s)
its possible physiological
was substantially
correlated
less
to ACIH level,
it
to the development of binding activity
of glandular origin was removed during the preincubation of the specific
Since
phase.
Characterization
responsible for the observed binding phenomenonand significance
are subjects of current studies in our
laboratory. ACKNOWLEDGEMENTS The authors express their appreciation to Mrs. Charlotte Butler for her assistance in preparation of the manuscript. This study was supported in part by Auburn University Grant-in-Aid 2275-01-7424. REFERENCES 1. 2. 3. 4. 5. 6. 7. 8. 9.
Murphy, B. E. P. (1967) J. Clin. Endocr. 27, 973-990. Murphy, B. E. P. in Odell, W. D. and Daughaday, W. II., eds. (1971) Principles of competitive protein-binding assays, pp 108-127, Lippincott, Philadelphia. Saffran, M., Grad, B., and Bayliss, M. J. (1952) Endocrinology 50, 639643. Van Goch, J. J., DeWied, D., snd Schonbaum,E. (1963) Am. J. Physiol. 205, 1083-1088. DeWied, D., Van Der Wal, B., and Van Goch, J. J. (1964) Excerpta Medica Int. Congr. Ser. 83(1):64-69. Schulster, D., Tait, S. A. S., Tait, J. F., and Mrotek, J., (1970) Endocrinology 86, 487-502. Bakker, R. F. M., and DeWied, D. (1961) Can. J. Biochem. Physiol. 39, 23-29. Birmingham, M. K., and Kurlents, E. (1958) Endocrinology 62, 47-60. Sayers, G., Swallow, R. L., and Giordano, N. D. (1971) Endocrinology 88, 1063-1068.
1363
and
Vol. 90, No. 4, 1979 October
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
29, 1979
[I3H
Pages
CORTICOSTERONE BINDING ACTIVITY
1355-1363
OF ADRENAL INCUBATION MEDIA
IN RESPONSE TO --IN VIVO AND IN VITRO ACTH STIMULATION J.
Departments Received
F. Pritchett*, W. L. Harper, D. N. Marple .I. T. Bradley, and M. L. Till
of Zoology-Entomology Agricultural Experiment
September
20,
and Animal Science; Auburn University Station; Auburn, Alabama 36830
1979 SUMMARY
ad nistration of ACTH upon --in vitro The influence of --in vivo or --in vitro binding adrenal corticosterone production as well as % ] corticosterone ACTH, regardless of the activity of incubation media have been examined. route of administration, significantly elevated corticosterone during an initial incubation period. During initial incubation periods ACTH also elevatedPI%] corticosterone binding activity of the incubation media. Ensuing incubations were characterized by either a marked decline in binding activity (in -- vivo ACTH administration) or a marked decline with sn attendant negative correlation between binding activity and ACTH level. Corticosteroidogenic response to ACTH remained intact during ensuing incubations. The data suggest the existence of an ACTH-sensitive intraglandular corticosterone binding ligand(s), the activity or concentration of which is dramatically altered by incubation protocol and time of sacrifice. INTRODUCTION Competitive
protein
binding
coids
routinely
involve
an initial
might
otherwise
compete
with
tated.
Such extractions
dichloromethane Since cortical were
our laboratory
expected
modify
plasma
corticoid *To whom all
values
rather
obtained
correspondence
assay
performed
involved
tedious
with
for
the steroid
in our
laboratory
determination
plasma
corti-
proteins being
which
quanti-
utilizing
incubation
corticoid
of --in vitro
concentrations
of plasma
media,
extraction
step.
proteins
in incubation However
samples
adreno-
we attempted
quantification
from non-extracted should
for
(1).
in adrenal for
procedures
to remove binding
protein
to ACTH and since
CPB procedures the
the
by Murphy is
to be minimal
by eliminating
radioassay
extraction
have been
as described
responsiveness
(CPB)
were
comparisons consistently
to media of lower
be addressed
0006-291X/79/201355-09$01.00/0 1355
Copyright All rights
@ I979
by Academic Press, Inc. in any form reserved
of reproduction
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL
than those obtained from the samesamples extracted Furthermore these differences in vitro gland.
RESEARCH COMMUNICATIONS
with dichloromethane.
appeared to be related not only to the specific
incubation method employed but also to the functional These findings prompted us to investigate
tissue in incubation may liberate and/or activity
status of the
the possibility
a corticoid-binding
ligand,
that adrenal
the concentration
of which is dependent not only upon incubation protocol but
also upon exposure of the tissue to ACTH. MATBHIALSANDMETHODS Animals and incubation
procedures
Male Sprague-Dawley rats 85 to 90 days of age were utilized. Prior to experimental procedures all animals were housed 3 per cage at an ambient temperature of 24 + .5OC with a photoperiod of 14 hours light:10 hours darkness Animals were provided with Purina Laboratory Chow (lights on at 0730 hours). and tap water -ad libitum. Wo hours prior to sacrifice, animals were transferred to individual cages. For determination of --in vitro and -in vivo responses to ACTUadministered in vivo, animals were injected subcutaneously 60 minutes prior to sacrifice with either 0.5 ml 0.9% NaCl or 0.5 ml 0.9% NaCl containing either 1 or 3 IU AC'JX (Nutritional Biochemicals). Animals utilized for study of in vitro response to --in vitro administration of ACTHor for determination of time of sacrifice upon corticosterone binding activity were allow to remain undisturbed until time of sacrifice. All animals were decapitated between either 0945-1015 or 1945-2015 hours. Trunk blood was collected from only the latter group for subsequent determination of plasma corticosterone. Adrenal glands from each animal were rapidly removed to a dish of cold (3-5OC) Krebs Ringer Bicarbonate solution (KRBC) and trimmed of extraneous tissue. Glands were then quartered, rinsed thoroughly in KRBC, and incubated in a Dubnoff metabolic incubator (37OC, 60 oscillations/ min., 95% 02-5% CO2atmosphere). To assess the influence of -in vivo ACTHon --in vitro corticosterone secretion and binding activity, glands were incubated for an initial 60 minutes in 2 ml KRBCcontaining 2 mg glucose/ml (KRBG). Following the initial incubation periods, glands were transferred to a second 60 minute incubation in 2 ml fresh KRBG. For study of the influence of time of sacrifice upon corticosterone binding activity, an initial incubation only was performed. Following each incubation period, media were decanted into glass vials and frozen (-2OoC). To determine the influence of --in vitro administration of ACTUupon in vitro corticosterone secretion and media binding activity, gland quartersfrom each animal were incubated for an initial 60 minutes in 2 ml KRBGor in a like volume of KKBGfortified with either 50, 200 or 400 milliunits/ml ACTU (Sigma At the end of the first incubation period, glands not initially Biochemicals). exposed to ACTUwere transferred to 2 ml fresh KRBG containing 50, 200, or 400 milliunits/ml ACTS and incubated for an additional 60 minute period. All incubation media were collected and frozen as before. Corticosterone
determination
in plasma and incubation media
Assay of incubation media and plasma samples for corticosterone was accomplished via the CPB radioassay described by Murphy (1, 2) utilizing rabbit serum as the source of the binding ligand and 1, 2 PH] corticosterone
1356
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Both plasma samples and aliquots of (New England Nuclear) as the radiolabel. incubation media were extracted with dichloromethane l/10 (v/v) prior to corticosterone determination. Separation of bound from free corticoid was accomplished by charcoal adsorption. The bound fraction was counted (Searle Isocap/ 300) in a scintillation cocktail of toluene-Triton X (2:l) with Omnifluor (6 grams/liter). Interand intra-assay variabilities were less than 7% and 5% respectively. Incubation
medium binding
activity
Aliquots of incubation medium were filtered utilizing a Millipore apparatus To remove endogenous corticosterone and filters (type HA, pore size = 0.45 um). from the samples, 500 ul portions of media were each added to an equal volume of 2.5% dextran-coated charcoal in phosphate buffered saline (PBS), and with constant agitation, were brought to and maintained at 45'C for 30 minutes. Samples were then centrifuged (2-3'C) for 30 minutes (2000 X g) and the supernatants were filtered as before, twice. Removal of endogenous corticosterone was confirmed via CPB assay of portions of the filtered fraction. Binding studies were performed in duplicate upon 500 pl aliquots of each sample. Tritiated corticosterone (specific activity = 136.9 mCi/mg) was added in 100 pl of PBS; DPM added per assay tube are indicated in the tables and figure. The mixture was vortexed and then incubated at 45'C for 10 minutes. Samples were then cooled to 2-3OC and maintained for a 10 minute period. Separation of free from bound isotope was via charcoal adsorption (500 pl added) followed by centrifugation (2000 X g for 20 minutes, 2-3OC). Bound isotope in 500 ~1 of supernatant was counted as before. Coefficients of determination for intraand inter-assay variability was less than 5%. To test the hypothesis that corticosterone binding activity of incubation' medium was influenced by extraction procedures, aliquots of corticosterone free incubation medium were incubated with isotope and then mixed l/10 (v/v) with dichloromethane and vortexed. The organic layer was removed. Free isotope from 400 ~1 aliquots of these samples as well as from 400 ul quantities of non-dichloromethane treated media samples and KRBG was removed as before and bound activity was quantitated as described above. RESULTS The effect activity
of incubation
previously
removed
a mean binding treated
compared
media is
activity,
to the KRBC-glucose
The action corticosterone 2.
of injected production
Both
upon
endogenous
in Table
1.
Although
greater
remained
terone
initial
had been
samples (p
<
exhibited
.05)
extraction in
binding
than
either
significantly
the treated
samples
as
blanks. ACTB upon --in vivo
1 and 3 IU levels concentration
corticosterone
corticosterone
dichloromethane
some activity
PI
Non-treated
was significantly
and corticosterone
corticosterone values,
from which
which
or blanks.
binding
extraction
illustrated
activity
samples
diminished
Table
of dichloromethane
within
incubation
produced
binding significant
one hour. levels
1357
plasma
were
corticosterone, activity elevations
Considering also
is
--in vitro
significantly
&vitro presented
in
in plasma corticoshigher
in the
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE Effect
of
dichloromethane binding activity
1
treatment upon of incubation
[&I] corticosterone media
Treatment
N
DPM Addeda
DPM Boundb
Nontreated
6
45750
894 t
Treated
6
45750
171 2 15d
Blank
6
45750
4Sc
75+ -
6e
aDPM added per determination; specific activity = 136.9 mCi/mg. bAll values represent DPM in 500 pl of supematant (means + SEM). cs ds eWithin the indicated column, values with different superscripts differ significantly (p ( 0.05).
TABLE Effect of secretion
Treatment
exogenous and[3H]
ACTH administered corticosterone
2
--in binding
vivo upon activity
corticosterone --in vitro of incubation mediaa.
Corticosterone Secretion (micrograms/hr)
DPM Boundb
N
Plasma Corticosterone (nanograms/ml)
Initial Incubation
Second Incubation
Initial Incubation
Second Incubation
Saline
Inject
6
195.9 + 34.1c
4.28 + .56c
4.71 + .52c
2379 f. 444c
1 Unit
ACTH
6
309.3 + 36.5d
6.22 + .4Bd
5.32 + .83c
3348 2 468d
6
321.5 + 48.5d
7.22 + .56d
4.13 f. .43c
3744 + 48gd
3 Units aAll
ACTH values
represent
means
group
of the second
as compared
to the
incubation,
no ACTH treatment
corticosterone incubation second
in response incubation,
in each below
binding
of the
that
activity
observed
saline-injected
837 + 153cse
the
significantly (p < 0.05). than DPM bound in
effects
However,
at the end
were
detected.
Tritiated
elevated
during
ACTH administration. on binding
activity
initial
incubation
1358
the
initial
At the end of the was apparent.
[‘HI corticosterone
incubations, during
9gcBe
of supematant;
group.
was significantly
to --in vivo
no ACTH effect second
1104 +
f. SEM.
b62250 DPM added per determination; DPM bound are per 500 nl specific activity = 136.9 mCi/mg. CsdWithin columns, values with different superscripts differ eDPM bound in second incubation significantly less (p < 0.01) initial incubation.
treated
642 + 135cBe
binding period.
Moreover,
was significantly
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL
TABLE Effect activity
of
upon PH] corticosterone binding during an initial incubationa.
Time
No.
Trial 1 2 3
2 2 2
2691 2475 2745
+ 156= T 144' z 135c
8:00
p.m.
1 2 3
2 2 2
3891 3993 3939
+ 144d + 204d + 60d
The influence
a single
media
exhibited
DPM bound are = 136.9 mCi/mg. values with (p < 0.05).
of sacrifice 60 minute
associated
significantly
killed
means + SEM. per determination; specific activity
the indicated colwm, differ significantly
of time
during
trials,
DPM Boundb
a.m.
cp dWithin scripts
all
N
1O:OO
aValues represent b60800 DPM added of supematsnt;
activity
3
time of sacrifice incubation media
of
Sacrifice
RESEARCH COMMUNICATIONS
incubation
with
less
(morning
animals
binding
per
super-
evening)
upon binding
is presented
activity
during than
pl
different
vs.
killed
500
in Table
3.
the morning
did
media
from
In
hours animals
at night. Regression
costerone
analyses
secretion
an initial without
upon
ACTH are given
in Figure
content
corticosterone
during
correlated
regression
line
Corticosterone
and negatively
for
ACTH level,
observed
for
equivalent
1.
Both were
an initial
less
of binding
Media
was also the slope
than
to --in vitro
activity during
1359
either incubation
activity
and
that
the initial
content
of
of and
the second
of the first
incu-
incubation.
incubation
ACTH level.
was significantly
corre-
positively
at the end of the second
correlated
ACTH levels
during
by an initial
period.
incubation although
corti-
and significantly
incubation
activity
binding
preceded
positively
second
and --in vitro
ACTH exposure
the degree
was significantly
significantly any given
incubation
to ACTH level
binding
binding
of --in vitro
of the media
at the end of the
significantly
corticosterone
the level
or a second
to ACTH level
bation
[3~]
incubation
corticosterone lated
of
was
Additionally less
incubation
than period.
that
Vol. 90, No. 4, 1979
BIOCHEMICAL
-0
5 ‘r
8
0
‘;^ 4am &E $i? a8 /‘:-
.Y
Incubation
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
1
i
-Incubation1 -
.---*Incubation
2 i
+l
2.
r s 50
400
200
In Vitro
ACTH
Dose
Level
(Milliunits/ml)
Figure 1. [%-I] Corticosterone binding activity of incubation media and corticosterone secretion in response to in vitro ACTH administration. Each point represents the mean with attendant SEM of 6 observations. Each line For represents the regression of the indicated variable upon ACTH dose level. each regression, an absolute value of the correlation coefficient (r)k .468 the slope of the regression line represents p < .05. For either variable, representing incubation 1 differs significantly (p < .025) from the corresponding value for incubation 2. *For either variable and within ACTH dose level, incubation 1 value differs significantly (p c.05) from incubation 2 value. For each determination of binding activity, 62250 DPMPH] corticosterone were added; DPM bound are per 500 pl of supematant; specific activity = 136.9 mCi/mg.
DISCUSSION Results activity
presented
of adrenal
of whether is presented
and refined
strongly
incubation
media
the ACTH is which
upon AC!JX and is --In vitro
herein
administered
suggests related
adrenal primarily
that
indicate in --in
response viva
the degree
to the specific incubation for
of binding
activity protocol
and protocols
binding
ACRID, regardless
Additionally
or in vitro.
of ACTH or for
1360
corticosterone
to exogenous
incubation
procedures
the bioassay
altered
is
evidence dependent
utilized. have been
studies
developed
on the mechanisms
Vol. 90, No. 4, 1979
BIOCHEMICAL
of corticosteroidogenesis. --in vitro Others
adrenal (4,
reliable
index
e,
provided
since
been
total
--in vivo
within
of both that
animal
out
degree
they
for
and constant
the gland
at the
medium shortly
tion)
periods
ACTH-induced
of response incubation (6)
systems
time
of sacrifice
as from
alterations
possible
physiological
isolated
cell
in which
study ensuing
observed
or constant
flow
systems
8).
incubations
were
would
present
have
into
cell within
out prior
initial
this
to
(preincubaConsequently,
whereas
rendered
-in
the incubation
period
be considered
the
recently
analyzed.
the preincubation
with-
to isolated
be washed from
of the
discarded
More
fluid
media
initial
altered
evolved
incubation
could
were
released
would
minute
which
extracellular materials
during
implications)
media
have
has or
by transfer
ACTH (7,
tissue
it
present
a 30-60
properties
to exogenous
-in
adrenocortical
employed
of the tissue
In the present as well
of --in vitro
to possess
and/or
preparation
factors
Preincubation
of adrenal
flow
after
ACTH treatment.
found
activity
from partial
of ACTH followed
medium.
can be a
However
obtained
therefore
the absence
--in vitro
immediately.
studies
elevated
of ACTS.
cortical
by extra-adrenal
ACTH have
were
adrenal
of data
Subsequently,
in
described
production
incubated
may be confounded
and uniformity
vi&protocols (9)
interpretation
ACTH-fortified
since
corticoid
is
first
administration
and ACTH-stimulated
that
period
(3)
to --in vitro
adrenal
tissue
to exogenous
to fresh analysis
that
adrenal
(6).
or pre-incubation
and coworkers
response
basal
systems
responsiveness
in
reported
suggested
the
tissue
Saffran
secretion
5) have
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
(and
the
the use of approach
unten-
able. Considering istration present media direct in
--in vivo
and --in vitro
of ACTH, a significant
stimulatory
as indicated levels
by elevated
of corticosterone
interest
the initial
injection
both
was the incubation
of the animal
plasma during
observation media, with
adrenal
response
corticosteroidogenic corticosterone
the initial
levels incubation
of corticosterone the magnitude
of which
ACTH and B) presumably
1361
binding
to in vivo admin-effect was and elevated period. activity
was A) related
dependent
upon the
Of more present to prior activity
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL
of the gland at or shortly
after
--in vivo glandular activity
and binding activity
binding activity
of initial
at night was significantly
RESEARCH COMMUNICATIONS
the time of sacrifice.
The relationship
of
is amplified by the fact that
incubation media associated with animals killed greater than that observed in samples obtained
during the mid-morning hours and hence corresponds to the time of maximal natural
activity.
Transfer of the tissue to and subsequent incubation without
in fresh medium
ACTHresulted in a moderate decline in corticosterone
ACTHtreated
groups to levels not different
from the saline injected
and may be due to the decay of the biological sharp decline in corticosterone
high level of binding activity to A) the functional
in the initial
of ACT&
group,
However, a
of all media occurred in both
It is therefore
possible that the relatively
incubation may have been related
status of the gland --in vivo with subsequent alterations
the composition of the extracellular
fluids
of death or B) the possible introduction mediumas a result
activity
binding activity
saline and ACTHtreated groups.
levels in the
in
of the gland before or at the time
of an intracellular
of tissue damageor secretion,
factor(s)
into the
the concentration(s)
of which
were AClX-dependent. To determine whether similar
alterations
obtained in response to ACTHadded directly
in binding activity
to the incubates (Figure l),
tissue was exposed to different
ACTHlevels either
immediately following
or during second incubations
incubations without
sacrifice
ACTS. In terms of corticoid
content of the media increased with AC'JI-Ilevel cating a continuing
capability
ACTH. During the initial was also positively
correlated
period,
to ACTHlevel.
the absence of ACTHand subsequent transfer only was binding activity
during initial
significantly
incubation but was also negatively
incubations
following
production,
initial
corticosterone
during either
in terms of corticoid
incubation
could be
incubation,
indi-
release in response to
corticosterone
binding activity
However, after
preincubation
to fresh ACID-fortified
medium, not
lower than observed during the initial
correlated
1362
in
to the level of ACTHexposure.
Vol. 90, No. 4, 1979
BIOCHEMICAL
AND BIOPHYSICAL
Results obtained from these initial in binding activity not be directly
due to ACTRis an intraglandular
in response to ACTB after
than observed without preincubation seemslikely
incubations suggest that the elevation
dependent upon extraglandular
binding activity
phenomenonand thus may
ACTS actions -in vivo.
preincubation
and negatively
that a component essential
RESEARCH COMMUNICATIONS
ligand(s)
its possible physiological
was substantially
correlated
less
to ACIH level,
it
to the development of binding activity
of glandular origin was removed during the preincubation of the specific
Since
phase.
Characterization
responsible for the observed binding phenomenonand significance
are subjects of current studies in our
laboratory. ACKNOWLEDGEMENTS The authors express their appreciation to Mrs. Charlotte Butler for her assistance in preparation of the manuscript. This study was supported in part by Auburn University Grant-in-Aid 2275-01-7424. REFERENCES 1. 2. 3. 4. 5. 6. 7. 8. 9.
Murphy, B. E. P. (1967) J. Clin. Endocr. 27, 973-990. Murphy, B. E. P. in Odell, W. D. and Daughaday, W. II., eds. (1971) Principles of competitive protein-binding assays, pp 108-127, Lippincott, Philadelphia. Saffran, M., Grad, B., and Bayliss, M. J. (1952) Endocrinology 50, 639643. Van Goch, J. J., DeWied, D., snd Schonbaum,E. (1963) Am. J. Physiol. 205, 1083-1088. DeWied, D., Van Der Wal, B., and Van Goch, J. J. (1964) Excerpta Medica Int. Congr. Ser. 83(1):64-69. Schulster, D., Tait, S. A. S., Tait, J. F., and Mrotek, J., (1970) Endocrinology 86, 487-502. Bakker, R. F. M., and DeWied, D. (1961) Can. J. Biochem. Physiol. 39, 23-29. Birmingham, M. K., and Kurlents, E. (1958) Endocrinology 62, 47-60. Sayers, G., Swallow, R. L., and Giordano, N. D. (1971) Endocrinology 88, 1063-1068.
1363
and