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Interactions between ionophores, Mg2+ and Ca2+ on acetylcholine formation and release in brain slices
Pharmacological Research Communications, Vol. 13, No. 2, 1981 INTI,:RACTIO[,IS ]]ETWEEN IONOPHOHES, FOR[,IATION AND R E L E A S E
P. M a n t o v a n i Department Morgagni
Mg 2+ AND Ca 2+ O1': ACETYLC, HOLINE
IN B]~AIN SLICES
and G. Pepeu
of P h a r m a c o l o g y ,
65,
175
50134
University
of Florence,
Viale
Florence, I t a l y
SU ~,~,iAR Y The effect the i n c u b a t i o n ACh output BrX-B37A
of different medium
with
(Bromolasolacid) were
solution
put was m e a s u r e d BrX-537A effect
enhanced
synthesis
in
slices and on their
of the t w o ~ i o n o p h o r e s
and A 23187 was studied. from rat cerebral
cortex,
incubated
ACh c o n t e n t
and out-
by bioassay. ACh output
also in C a 2 + - f r e e The a d d i t i o n
medium
and total ACh
formation.
effect
to the i n c u b a t i o n
of B r X - ~ 3 V A
on ACh output.
that C a 2+ and Mg 2+ c o n c e n t r a t i o n
primarily
The
m e d i u m and in C a 2 + - e n r l c h e d
o f Mg 2+ (9.3 ~1)
the s t l m u l a t o r y
It is concluded incubation
the addition
prepared
stimulated
occurred
in brain
c o n t a i n i n g physostigmine.
(5.0 ~,I) medium. medium
on ACh level
and without
The slices in Krebs
Ca 2+ and Ng 2+ c o n c e n t r a t i o n s
modulate
and exert only an indirect
ACh release, influence
in the
cor~tent and
on BrX-53?A.
INTROOUCT!ON Acetylcholine about
by c a l c i u m
(ACh)
fluid
thereby d e p r e s s e s
from nerve
entrs, (Katz and Miledi,
Mg 2+, a p r e d o m i n a n t l y extracellular
release
Intracellular
competes
ACh output
0031-6989/8 I/'020175-10/$02.00/0
endings
1965;
cation,
is br~uF~ht
Miledl,
1973).
when present i n
with Ca 2+ for active from motor nerve
sites
terminal
the
and (Del
0 1981 The itai,an Pharmacolog,cal Society
PharmacologicalResearch Communications, I/ol. 13, No. 2, 1981
1 76
C a s t i l l o and Engback, sympathetic
ganglia
Substitution
1954, Hubbard,
(Hurter and Kostlal,
1954).
of Ca 2+ with Mg 2+ strongly
from the frog spinal cord (Nistrl, s ynthesis and release stimulat e d the isolated
et al., 1968) and from
1976).
Mg 2+ inhibits ACh
by high K + c o n c e n t r a t i o n
ileum (Gerhards, et al., 1964)
(Molenaar and Polak,
reduced ACh release
and in b r a i n slices
1970).
E x t r a c e l l u l a r Mg 2+ seems t h e r e f o r e to depress A C h in all e x p e r i m e n t a l an
in
conditions
so far investigated.
Increase in Mg 2+ c o n c e n t r a t i o n
output
However,
in the incubation medium
p o t e n t i a t e s the s t l m u l a t o r y effect o f the ionophore B r X - 5 3 7 A (Bromolasolacid) et al., 1978),
on A C h output
from brain slices
(Casamenti,
In the present paper this e f f e c t of. Mg 2+ is
i nvestigated by studying
the interactions
between B r X - 5 3 7 A ,
Ca 2+ and Mg 2+ on ACh formation and release.
M A T E H I A L S A_ND [~ETHODS Slices were prepared
from the cerebral cortex of adult
male Wistar rats killed by decapitation. incubated at 37 ° C in Krebs sol u t i o n tion (raM):
The slices were
of the followinF~ composi-
NaCI 113, KCI 4.7, CaCI 2 2.5, KH2PO 4 1.2, MgSO 4 1.2,
NaHCO 3 25, glucose 11.5,
p h y s o s t l g m l n e sulphate
1.54 uM.
The
s o l u t i o n was gassed with 5% CO 2 in 0 2 . In some experiments modified Krebs solutions were used: free solution was obtained by omission of CaCl2;
Ca 2+-
Mg 2+ was raised
to 9.3 mM and Ca 2+ to 5 mM by a d d i t i o n of M g S O 4 or CaCl 2 respectively.
In the latter case Ns~{CO 3 was also s u b s t i t u t e d
with NaCl
in order to avoid Ca precipitation. ACh ~as extracted Beani et al.
from the slices a c c o r d l n K
to the method o f
(1963), either at the end of 60 mln p r e i n c u b a t l o n
(O time) or at the end of the following 60 rain incubation.
ACh
Pharmacological Research Communications, VoL 13, No. 2, 1981 o f the e x t r a c t s
was measured
~ig ileum a c c o r d i n g After
60 mln
and ACh o u t p u t
177
by b i o a s s a y
to Beanl
et al.
preincubation,
on the isolated
~ulnea-
(1978).
fresh medium was s u b s t i t u t e d
in the i n c u b a t i o n
m e d i u m was measured
e i t h e r every
I0 mln or at the end of 60 rain incubation. Sodium-dependent by the method
affinity
of S i m o n et al.
from the incubated 130 Ci/mmol
hiF~
brain slices.
containing
(0.25 mg of protein)
over M i l l i p o r e
transferred
samples
filters
of 20 mm Jig.
ethylether
Methyl
and
were c o u n t e d
filters vials
Instagel
incubated
Manifold
expressed
method.
as pmol of choline
with
were a l l o w e d
was added
of choline in ~ O u b n o f f ~oured
a suction
to dry and were
to vfnich ethylenc-lycol-mono-
(Packard)
in a Packard
standard
chloride
of s y n a p t o s o m e s
concentration
were added
Triearb
(mod 577)
tion s p e c t r o m e t e r with a counting, e f f i c i e n c y by the e x t e r n a l
choline
The content of the tubes was
on a M i l l i p o r e The
obtained
- Amersham,
The tubes were
to s c i n t i l l a t o r (Merck)
3H
Centre
to o b t a i n a final
s h a k e r at 30 ° C for 4 rain.
was measured
in s y n a p t o s o m e s
a resusper:ded a l i o u o t
in the m e d i u m o f 0.04 uM.
pressure
(1976)
from the R a d i o c h e m l c a l
to the tubes
c h o l i n e uptake
and
the
scintilla-
of 35% d e t e r m i n e d
The rates of c h o l i n e uptake
per 4 min i n c u b a t i o n
v,ere
time per mF, of
prote in. The method
protein
content o f the s y n a p t o s o m e s
of Lowry et al.
Concentrated were made
attained
solutions
(I - I0 mg/ml) and w e r e
The h i ~ h e s t c o n c e n t r a t i o n
in the i n c u b a t i o n m e d i u m was
no e f f e c t on ACh o u t p u t and c o n t e n t to all controls.
by the
(1951).
in d i m e t h y l s u l p h o x i d e
as necessary,
was m e a s u r e d
of B r X - 5 3 7 A and A 23187
diluted
500 to 200 folds
of d i m e t h y l s u l p h o x i d e
25 m~4 and while
this had
it was n e v e r t h e l e s s
added
178
Pharmacological Research Communications, VoL 13, No. 2, 1981
EE SULTS Fig 1 shows every
the e f f e c t
of B r X - 5 3 7 A
10 rain in the presence
i n c u b a t i o n medium,
Of two Mg 2+ c o n c e n t r a t i o n s
increase
6 times
larger
It can be seen that the m a x i m u m
in ACh output e l i c i t e d
in presence
by B r X - 5 3 7 A
a s e c o n d ionophore,
to the i n c u b a t i o n medium at the c o n c e n t r a t i o n
increase
1978),
caused a 2 8 0 %
increase
A 23187,
was 6 3 2 % with Mg 2+ 9.3 raM.
3000
WITH
Mg 2.9.3 mM
LtJ
Z
2000
g ID a. ID
1000
O U <[
Mg ~" 1.2 mM 200 L
,J
0.15
0 45
....
0.9
CONCENTRATIONS
Fig.
I
1.8 OF
3.6
BrX~S37A
(pM)
added
of 58 uM (Casamenti
in 4 e x p e r i m e n t s
Brx-537A DOSE.EFFECT RELATIONSHIP D I F F E R E N T Mg 2÷ C O N C E N T R A T I O N S
U) < UJ nO
1.8 uM was
of 9.3 than in that of 1.2 mM Mg 2+.
Under the l a t t e r c o n d i t i o n s
et al.,
in the
With Mg 2+ 9.3 ~ff4 the output after B r X - 5 3 7 A
was larger than with 1.2 n~4. percent
on ACh output m e a s u r e d
v~ile the
Pharmacological Research Communications, Vol. 13, No. 2, 1981
179
However, by e x p r e s s i n g t h e effect of the ionophores on ACh output
as percenb
ences
caused
increase
o v e r the basal
b v t h e two Mg 2+ c o n c e n t r a t i o n s
ent if h i g h Mg 2+ also d e p r e s s e s son b e t w e e n therefore slices
the absolute
be made'
o f ACh
differ-
would o n l y b e
the basal ACh output,
values, r e p o r t e d
Table
at the b e g i n n i n g
the amount
output, t h e
1 also
shov~
appar-
A comparl-
in table I, should
ACh content
in brain
and at the end of 60 mln incubation,
total ACh formed d u r i n g k i n the presence o f d i f f e r e n t Mg 2+ and C a 2+
incubation
r e l e a s e d a n d the
concentrations. The changes
content after
in i o n
i
of theslices
concentrations
at
the beginning
60 mln preincubation).
in C a 2 + - e n r i c h e d solution.
affected
ACh
of the incuba~ton
ACh content
"(5.O m M ) a n d
Increasing
firstly
was much lower
in C a 2 ÷ - f r e e
Mg 2+ c o n c e n t r a t i o n
(i.e. both
than in n o r m a l Krebs
caused
a slight
increase
in ACh content. The r e l a t i v e l y brain slices
small
in normal
basal A C h
Krebs
output
solution
from the u n s t i m u l a t e d
was decre~u;ed by the r e m o v a l
of Ca 2+ and b y the increase i n Mg 2+. On the contrary it v~s \ s t r o n g l y enhanced by d o u b l i n g Ca 2+ c o n c e n t r a t i o n and by the addition
of BrX-537A.
Little incubation both
or no ACh was formed in normal
the a b s e n c e
markedly however
or M g 2 + - e n r i c h e d
ACh
formation.
of the ACh
in the slices
was much
formed lower
was
ACh
of BrX-537A
formation.
on ACh o u t p u t
In h i g h
always
was twice,as
solution.
In the latter released
60 min Conversely
conditions
and ACh c o n t e n t Krebs.
in the i n c u b a t i o n
stimulated
M~,2+ Krebs
during
of its c o n c e n t r a t i o n
than in normal
h~latever the ion c o n c e n t r a t i o n the a d d i t i o n
Krebs
of Ca 2+ and the doubling
stimulated most
by brain slices
solution
ACh release the e f f e c t
large as in.normal
Krebs.
medium, and total of BrX-537A However
an
I: E F F E C T
a
a
d
b,c v e r s u s
d versus
e,f v e r s u s
edlfferent
1 with
P
P<0.01
P
0
0 1.8
1.8
a
g versus h versus
b
e versus
P<0.01
versus
p,q v e r s u s
P
r
n versus
i versus
(6) (4)
(4)
(12)
(4)
P <0.05
P<0.02
2.72+0.28 i 5.06+0.611
1.03+O.09 h
0.31+0.03g
3.21+-0.38 f
O. 25~--0.o15d (15) 3.35+0.28 e (6)
0 1.8 3.6
1 . 6 7 + 0 . 3 b (i0) i.O7+0.13 c (6)
0.43+0.21 a (21)
ACh o u t p u t d u r i n g 60 min
S
o
m
b,i
A/~D 0 U T P U T , E X P R E S S E D
1.8 3.6
0
BrX-537A uN
0N ACh C C N T E N T
of e x p e r i m e n t s .
2.79+0.120 (4)
number
from
In p a r e n t h e s i s
Mg2+ 1.2 mM Ca 2+ 5.0
(4)
5,06+0.95~
Mg2+ 1.2 mM
mM
(8)
Ca 2+ 2.5 mM
Ca 2+ 0
12.854"0.76
llg 2+ 9.3 ~
"
(12)
"
9 62+0 76 1
ACh c o n t e n t at 0 time
OF B r X - 5 3 7 A
C a 2+ 2.5 mM
;4g 2+ 1.2 mM
Conditions
TABLE
+ S.E.,IN
(4)
P<0.05
P<0.05
P<0.05
P<0.01
t lu v e r s u s
SLICES
m
P
.O1
P
5.96 6.94
7.71
2.77
4.93
5.84
6.92 1.16
0.87
Total ACh formed in 60 m i n
BRAIN
r versus
6 . 0 3 + 0 . 8 t (4) 4.67+0.35 u (4)
1 1 . 7 4 ±I.06 s
7.52+-0.82 r (4)
1 4 . 5 7 + 1 . 5 7 q (4)
11.34+0.92 ° (8) 15.34+1.28 p (4)
1 4 . 8 7 + 0 . 6 4 n (4) 9.71+0.5 (4)
10.06±1.01 m (8)
ACh c o n t e n t a f t e r 60 rain
AS ug/g
o0
CO
c%
cb
c~
0
Pharmacological Research Communications, Vol. 13. No. 2. 1981
increase Krebs
in the synthesis
was
Even
exerted
in C a 2 + - f r e e
(HC-3)
t i o n did not e l i m i n a t e uM) on ACh o u t p u t . was only
a difference
Drain
was
obtained 1980).
effect
percent
in s y n a p t o s o m e s DrX-537A
solu-
of BrX-537A over
protein
prepared
choline
At
solution hich
Drool/4 m i n / m g
to
(i.8
the basal (n=15),
significant.
investiKated.
Krebs
able
ME 2+ K r e b s
increase
of B r X - 5 3 7 A on hi qh affinity
in normal
I.I + 0.07
to high
from 1572 +- 200 to II12 +- 153%
s l i c e s was also
incubation
~ras still
formation.
10 -2 added
not s t a t l s t i c ~ l l y
The e f f e c t
BrX-537A
the s t i m u l a t o r y
reduced
A similar
Krebs solution.
and ACh
The maximum
in normal
dose o f BrX-537A.
Krebs s o l u t i o n
ACh output
Hemicholinium-3
output
t h e largest
in C a 2 + - e n r i c h e d
stimulate markedly
the
of ACh over that o c c u r r i n E
was only s e e n with
effect
181
in
the end of 60 rain
affinity- choline
(n=4):,
from
uptake
A
s i m i l a r value
fresh slices
1.8 uM did not a f f e c t h i K n
untake was
(Pedata
et al.,
uotake
neither
affinity
in 1 . 2 nor in 9.3 mM i4~2+ i n c u b a t i o n m e d i u m .
D I SC US SION U n d e r restinK slices .incubated
conditions
i n normal
the additio~
Krebs
solution
increase
in A C h
output
A direct
effect
of the parent
ionophore
been excluded
by R i c h t e r
transferase enhanced uptake
has
ACh c o n t e n t
%.Jhose rate
content Wen solution
in the slices
is i n v e r s e l y
(Roskowski, brain
indirectly
1978;
slices
the present
a marked
activatinF, also ACh synthesis. X-537A
on choline
(1977)
~rX-5~7A
and hip.h a f f i n i t y
related
1978)
of BrX-537A
experiments
was
acetvlelso
choline
to s y n a p t o s o m a l
?~esleP et al.,
output
to brain
brouKht a b o u t
ACh
:.:as n o t stimulated.
~'iere i n c u b a t e d in ~4g2+ enrie~ed
the e f f e c t on ACh
tions used i n
of B r X - 5 3 7 A
at both
ootentinted
Krebs concentrabut only at
Pharmacological Research Communications, Vol. 13, No. 2, 1981
182 the largest
concentration
enhanced.
ACh
incubation
in Mg 2+ enriched
medlum
content
the effect
and t h e r e f o r e
ACh store
bigger
release
was
a t the b e g i n n i n g
could have
of the
than in normal
acted u p o n a larger
release.
can be raised
ACh f o r m a t i o n a n d
formation
m e d i u m was larger
BrX-SB7A
stimulating
The q u e s t i o n
in the slices
on ACh
as to w h e t h e r B r X - 5 3 7 A
only
through
its
stimulates
ionophoric
properties
or by some other mechansims. Richter
(1977)
the analogue duced and
showed
X-B37A o n
a similar
Sokolowsky
(1978)
that in Ca2+~-free medium the effect
ACh r e l e a s e
observation
in Torpedo
reduced
The p o s s i b i l i t y
that
cellular
has been s u g g e s t e d
stores
We observed solution
still
endings,
unrelated
released ACh,
was a p p a r e n t l y
larger t h a n in normal (1966)also
lobster n e r v e
was
showed
larger
(Tucek,
activity
Ca2+-dependent.
is not
The s t l m u l a t o r y neurotransmltters
it has
agent
is reduced (Holz,
been claimed
increase
effect
1977;
transferring Ito et al.,
cations 1978;
output
Dettbarn in the sea w a t e r
acetyltransferase
1977; Ito et al.,
by d e p o l a r i z a t i o n (~asamentl
and Sokolovsky,
of several
m e d i u m added
and its a n a l o g u e
as an i o n o ~ h o r e
Michaelson
formation
in C a 2 + - f r e e
Richter,
that B r X - B B T A
neurotransmitter
solution.
synthesis
of B r X - 8 3 7 A on the release only
Krebs
from cut nerve
than in normal
I'9?7) that choline
1978).
in Ca2+-free
and their ACh
that ACh
in C a 2 + - f r e e
and it is known
and Currel,
a leakage
Krebs
on
Ca 2+ from intra-
incubated
activity,
of BrX-537A
and accumulation.
(Nordman
probably
to neuronal
and R o s e n b e r g
chelating
the effect
might release
that brain slices
and
In our e x p e r i m e n t s
but did not affect ACh f o r m a t i o n BrX-537A
was not re-
was made by M i c h a e l s o n
synaptosomes.
the lack of Ca 2+ only s l i g h t l y ACh output
from brain slices
of
1978)
and
X - 5 3 7 A could as well as by
et al.,
1978).
with
1978;
a
Pharmacological Research Communications, VoL 13, No. 2, 1981
Finally, reduced ACh
d o u b l i n g C a 2+ c o n c e n t r a t i o n
level in the
£anglion
increased
ACh output,
by H u r t e r and Kostial
and ACh synthesis.
In C a 2 + - e n r i p h e d increase amount
in the I'.rebs solution
slices and m a r k e d l y
as shovn~ in the per'fused cervical (I~54),
183
the already
of ACh
at the expense
Krebs s o l u t i o n
released
in normal
of ACh content,
Krebs.
the same
This occurred
partly
partly by stimulatin}~ ACh s y n t h e s i s
an additive
effect of B r X - 5 3 7 A
and h i g h Ca 2+
on ACh output.
In c o n c l u s i o n ,
these
results d e m o n s t r a t e
brain slices Ca 2+ and Mg 2+ c o n c e n t r a t i o n s influence
was still able to
larRe ACh output by p r a c t i c a l l y
This finding s u g g e s t s concentration
BrX-537A
on B r X - 5 3 7 A
that in resting
exert an i n d i r e c t
a c t i o n by m o d u l a t i n g ACh
release, content
and synthesis.
ACKNOh;LEI)GENENTS This work was C.I!.R.
s u p p o r t e d b y grant n~ 7 8 , 0 2 2 2 6 . 0 4
BrX-537A.was
a generous
gift of Roche
from the
and A 23187
of
Ely Lilly Co.
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J. Neurochem.,
3_~5, 606, 1980;
Life Sciences,:20, 701, 1977;
Roskoski, R. Jr.: Simon, J.R., Atweh,
J. Neurochem., S. and Kuhar,
Tueek, S. : "Aeetylcholine London, 1977;
3__OO, 1357, 1978; M.J.:
J. Neurochem.,
26, 909, 1976;
synthesis in neurons", Chapman and [lall,
Weiler, M.H.-, Jope, R.S. and Jenden, D J.: 1978.
J. Neurochem
, 31, 789
P. M a n t o v a n i Department Morgagni
Mg 2+ AND Ca 2+ O1': ACETYLC, HOLINE
IN B]~AIN SLICES
and G. Pepeu
of P h a r m a c o l o g y ,
65,
175
50134
University
of Florence,
Viale
Florence, I t a l y
SU ~,~,iAR Y The effect the i n c u b a t i o n ACh output BrX-B37A
of different medium
with
(Bromolasolacid) were
solution
put was m e a s u r e d BrX-537A effect
enhanced
synthesis
in
slices and on their
of the t w o ~ i o n o p h o r e s
and A 23187 was studied. from rat cerebral
cortex,
incubated
ACh c o n t e n t
and out-
by bioassay. ACh output
also in C a 2 + - f r e e The a d d i t i o n
medium
and total ACh
formation.
effect
to the i n c u b a t i o n
of B r X - ~ 3 V A
on ACh output.
that C a 2+ and Mg 2+ c o n c e n t r a t i o n
primarily
The
m e d i u m and in C a 2 + - e n r l c h e d
o f Mg 2+ (9.3 ~1)
the s t l m u l a t o r y
It is concluded incubation
the addition
prepared
stimulated
occurred
in brain
c o n t a i n i n g physostigmine.
(5.0 ~,I) medium. medium
on ACh level
and without
The slices in Krebs
Ca 2+ and Ng 2+ c o n c e n t r a t i o n s
modulate
and exert only an indirect
ACh release, influence
in the
cor~tent and
on BrX-53?A.
INTROOUCT!ON Acetylcholine about
by c a l c i u m
(ACh)
fluid
thereby d e p r e s s e s
from nerve
entrs, (Katz and Miledi,
Mg 2+, a p r e d o m i n a n t l y extracellular
release
Intracellular
competes
ACh output
0031-6989/8 I/'020175-10/$02.00/0
endings
1965;
cation,
is br~uF~ht
Miledl,
1973).
when present i n
with Ca 2+ for active from motor nerve
sites
terminal
the
and (Del
0 1981 The itai,an Pharmacolog,cal Society
PharmacologicalResearch Communications, I/ol. 13, No. 2, 1981
1 76
C a s t i l l o and Engback, sympathetic
ganglia
Substitution
1954, Hubbard,
(Hurter and Kostlal,
1954).
of Ca 2+ with Mg 2+ strongly
from the frog spinal cord (Nistrl, s ynthesis and release stimulat e d the isolated
et al., 1968) and from
1976).
Mg 2+ inhibits ACh
by high K + c o n c e n t r a t i o n
ileum (Gerhards, et al., 1964)
(Molenaar and Polak,
reduced ACh release
and in b r a i n slices
1970).
E x t r a c e l l u l a r Mg 2+ seems t h e r e f o r e to depress A C h in all e x p e r i m e n t a l an
in
conditions
so far investigated.
Increase in Mg 2+ c o n c e n t r a t i o n
output
However,
in the incubation medium
p o t e n t i a t e s the s t l m u l a t o r y effect o f the ionophore B r X - 5 3 7 A (Bromolasolacid) et al., 1978),
on A C h output
from brain slices
(Casamenti,
In the present paper this e f f e c t of. Mg 2+ is
i nvestigated by studying
the interactions
between B r X - 5 3 7 A ,
Ca 2+ and Mg 2+ on ACh formation and release.
M A T E H I A L S A_ND [~ETHODS Slices were prepared
from the cerebral cortex of adult
male Wistar rats killed by decapitation. incubated at 37 ° C in Krebs sol u t i o n tion (raM):
The slices were
of the followinF~ composi-
NaCI 113, KCI 4.7, CaCI 2 2.5, KH2PO 4 1.2, MgSO 4 1.2,
NaHCO 3 25, glucose 11.5,
p h y s o s t l g m l n e sulphate
1.54 uM.
The
s o l u t i o n was gassed with 5% CO 2 in 0 2 . In some experiments modified Krebs solutions were used: free solution was obtained by omission of CaCl2;
Ca 2+-
Mg 2+ was raised
to 9.3 mM and Ca 2+ to 5 mM by a d d i t i o n of M g S O 4 or CaCl 2 respectively.
In the latter case Ns~{CO 3 was also s u b s t i t u t e d
with NaCl
in order to avoid Ca precipitation. ACh ~as extracted Beani et al.
from the slices a c c o r d l n K
to the method o f
(1963), either at the end of 60 mln p r e i n c u b a t l o n
(O time) or at the end of the following 60 rain incubation.
ACh
Pharmacological Research Communications, VoL 13, No. 2, 1981 o f the e x t r a c t s
was measured
~ig ileum a c c o r d i n g After
60 mln
and ACh o u t p u t
177
by b i o a s s a y
to Beanl
et al.
preincubation,
on the isolated
~ulnea-
(1978).
fresh medium was s u b s t i t u t e d
in the i n c u b a t i o n
m e d i u m was measured
e i t h e r every
I0 mln or at the end of 60 rain incubation. Sodium-dependent by the method
affinity
of S i m o n et al.
from the incubated 130 Ci/mmol
hiF~
brain slices.
containing
(0.25 mg of protein)
over M i l l i p o r e
transferred
samples
filters
of 20 mm Jig.
ethylether
Methyl
and
were c o u n t e d
filters vials
Instagel
incubated
Manifold
expressed
method.
as pmol of choline
with
were a l l o w e d
was added
of choline in ~ O u b n o f f ~oured
a suction
to dry and were
to vfnich ethylenc-lycol-mono-
(Packard)
in a Packard
standard
chloride
of s y n a p t o s o m e s
concentration
were added
Triearb
(mod 577)
tion s p e c t r o m e t e r with a counting, e f f i c i e n c y by the e x t e r n a l
choline
The content of the tubes was
on a M i l l i p o r e The
obtained
- Amersham,
The tubes were
to s c i n t i l l a t o r (Merck)
3H
Centre
to o b t a i n a final
s h a k e r at 30 ° C for 4 rain.
was measured
in s y n a p t o s o m e s
a resusper:ded a l i o u o t
in the m e d i u m o f 0.04 uM.
pressure
(1976)
from the R a d i o c h e m l c a l
to the tubes
c h o l i n e uptake
and
the
scintilla-
of 35% d e t e r m i n e d
The rates of c h o l i n e uptake
per 4 min i n c u b a t i o n
v,ere
time per mF, of
prote in. The method
protein
content o f the s y n a p t o s o m e s
of Lowry et al.
Concentrated were made
attained
solutions
(I - I0 mg/ml) and w e r e
The h i ~ h e s t c o n c e n t r a t i o n
in the i n c u b a t i o n m e d i u m was
no e f f e c t on ACh o u t p u t and c o n t e n t to all controls.
by the
(1951).
in d i m e t h y l s u l p h o x i d e
as necessary,
was m e a s u r e d
of B r X - 5 3 7 A and A 23187
diluted
500 to 200 folds
of d i m e t h y l s u l p h o x i d e
25 m~4 and while
this had
it was n e v e r t h e l e s s
added
178
Pharmacological Research Communications, VoL 13, No. 2, 1981
EE SULTS Fig 1 shows every
the e f f e c t
of B r X - 5 3 7 A
10 rain in the presence
i n c u b a t i o n medium,
Of two Mg 2+ c o n c e n t r a t i o n s
increase
6 times
larger
It can be seen that the m a x i m u m
in ACh output e l i c i t e d
in presence
by B r X - 5 3 7 A
a s e c o n d ionophore,
to the i n c u b a t i o n medium at the c o n c e n t r a t i o n
increase
1978),
caused a 2 8 0 %
increase
A 23187,
was 6 3 2 % with Mg 2+ 9.3 raM.
3000
WITH
Mg 2.9.3 mM
LtJ
Z
2000
g ID a. ID
1000
O U <[
Mg ~" 1.2 mM 200 L
,J
0.15
0 45
....
0.9
CONCENTRATIONS
Fig.
I
1.8 OF
3.6
BrX~S37A
(pM)
added
of 58 uM (Casamenti
in 4 e x p e r i m e n t s
Brx-537A DOSE.EFFECT RELATIONSHIP D I F F E R E N T Mg 2÷ C O N C E N T R A T I O N S
U) < UJ nO
1.8 uM was
of 9.3 than in that of 1.2 mM Mg 2+.
Under the l a t t e r c o n d i t i o n s
et al.,
in the
With Mg 2+ 9.3 ~ff4 the output after B r X - 5 3 7 A
was larger than with 1.2 n~4. percent
on ACh output m e a s u r e d
v~ile the
Pharmacological Research Communications, Vol. 13, No. 2, 1981
179
However, by e x p r e s s i n g t h e effect of the ionophores on ACh output
as percenb
ences
caused
increase
o v e r the basal
b v t h e two Mg 2+ c o n c e n t r a t i o n s
ent if h i g h Mg 2+ also d e p r e s s e s son b e t w e e n therefore slices
the absolute
be made'
o f ACh
differ-
would o n l y b e
the basal ACh output,
values, r e p o r t e d
Table
at the b e g i n n i n g
the amount
output, t h e
1 also
shov~
appar-
A comparl-
in table I, should
ACh content
in brain
and at the end of 60 mln incubation,
total ACh formed d u r i n g k i n the presence o f d i f f e r e n t Mg 2+ and C a 2+
incubation
r e l e a s e d a n d the
concentrations. The changes
content after
in i o n
i
of theslices
concentrations
at
the beginning
60 mln preincubation).
in C a 2 + - e n r i c h e d solution.
affected
ACh
of the incuba~ton
ACh content
"(5.O m M ) a n d
Increasing
firstly
was much lower
in C a 2 ÷ - f r e e
Mg 2+ c o n c e n t r a t i o n
(i.e. both
than in n o r m a l Krebs
caused
a slight
increase
in ACh content. The r e l a t i v e l y brain slices
small
in normal
basal A C h
Krebs
output
solution
from the u n s t i m u l a t e d
was decre~u;ed by the r e m o v a l
of Ca 2+ and b y the increase i n Mg 2+. On the contrary it v~s \ s t r o n g l y enhanced by d o u b l i n g Ca 2+ c o n c e n t r a t i o n and by the addition
of BrX-537A.
Little incubation both
or no ACh was formed in normal
the a b s e n c e
markedly however
or M g 2 + - e n r i c h e d
ACh
formation.
of the ACh
in the slices
was much
formed lower
was
ACh
of BrX-537A
formation.
on ACh o u t p u t
In h i g h
always
was twice,as
solution.
In the latter released
60 min Conversely
conditions
and ACh c o n t e n t Krebs.
in the i n c u b a t i o n
stimulated
M~,2+ Krebs
during
of its c o n c e n t r a t i o n
than in normal
h~latever the ion c o n c e n t r a t i o n the a d d i t i o n
Krebs
of Ca 2+ and the doubling
stimulated most
by brain slices
solution
ACh release the e f f e c t
large as in.normal
Krebs.
medium, and total of BrX-537A However
an
I: E F F E C T
a
a
d
b,c v e r s u s
d versus
e,f v e r s u s
edlfferent
1 with
P
P<0.01
P
0
0 1.8
1.8
a
g versus h versus
b
e versus
P<0.01
versus
p,q v e r s u s
P
r
n versus
i versus
(6) (4)
(4)
(12)
(4)
P <0.05
P<0.02
2.72+0.28 i 5.06+0.611
1.03+O.09 h
0.31+0.03g
3.21+-0.38 f
O. 25~--0.o15d (15) 3.35+0.28 e (6)
0 1.8 3.6
1 . 6 7 + 0 . 3 b (i0) i.O7+0.13 c (6)
0.43+0.21 a (21)
ACh o u t p u t d u r i n g 60 min
S
o
m
b,i
A/~D 0 U T P U T , E X P R E S S E D
1.8 3.6
0
BrX-537A uN
0N ACh C C N T E N T
of e x p e r i m e n t s .
2.79+0.120 (4)
number
from
In p a r e n t h e s i s
Mg2+ 1.2 mM Ca 2+ 5.0
(4)
5,06+0.95~
Mg2+ 1.2 mM
mM
(8)
Ca 2+ 2.5 mM
Ca 2+ 0
12.854"0.76
llg 2+ 9.3 ~
"
(12)
"
9 62+0 76 1
ACh c o n t e n t at 0 time
OF B r X - 5 3 7 A
C a 2+ 2.5 mM
;4g 2+ 1.2 mM
Conditions
TABLE
+ S.E.,IN
(4)
P<0.05
P<0.05
P<0.05
P<0.01
t lu v e r s u s
SLICES
m
P
.O1
P
5.96 6.94
7.71
2.77
4.93
5.84
6.92 1.16
0.87
Total ACh formed in 60 m i n
BRAIN
r versus
6 . 0 3 + 0 . 8 t (4) 4.67+0.35 u (4)
1 1 . 7 4 ±I.06 s
7.52+-0.82 r (4)
1 4 . 5 7 + 1 . 5 7 q (4)
11.34+0.92 ° (8) 15.34+1.28 p (4)
1 4 . 8 7 + 0 . 6 4 n (4) 9.71+0.5 (4)
10.06±1.01 m (8)
ACh c o n t e n t a f t e r 60 rain
AS ug/g
o0
CO
c%
cb
c~
0
Pharmacological Research Communications, Vol. 13. No. 2. 1981
increase Krebs
in the synthesis
was
Even
exerted
in C a 2 + - f r e e
(HC-3)
t i o n did not e l i m i n a t e uM) on ACh o u t p u t . was only
a difference
Drain
was
obtained 1980).
effect
percent
in s y n a p t o s o m e s DrX-537A
solu-
of BrX-537A over
protein
prepared
choline
At
solution hich
Drool/4 m i n / m g
to
(i.8
the basal (n=15),
significant.
investiKated.
Krebs
able
ME 2+ K r e b s
increase
of B r X - 5 3 7 A on hi qh affinity
in normal
I.I + 0.07
to high
from 1572 +- 200 to II12 +- 153%
s l i c e s was also
incubation
~ras still
formation.
10 -2 added
not s t a t l s t i c ~ l l y
The e f f e c t
BrX-537A
the s t i m u l a t o r y
reduced
A similar
Krebs solution.
and ACh
The maximum
in normal
dose o f BrX-537A.
Krebs s o l u t i o n
ACh output
Hemicholinium-3
output
t h e largest
in C a 2 + - e n r i c h e d
stimulate markedly
the
of ACh over that o c c u r r i n E
was only s e e n with
effect
181
in
the end of 60 rain
affinity- choline
(n=4):,
from
uptake
A
s i m i l a r value
fresh slices
1.8 uM did not a f f e c t h i K n
untake was
(Pedata
et al.,
uotake
neither
affinity
in 1 . 2 nor in 9.3 mM i4~2+ i n c u b a t i o n m e d i u m .
D I SC US SION U n d e r restinK slices .incubated
conditions
i n normal
the additio~
Krebs
solution
increase
in A C h
output
A direct
effect
of the parent
ionophore
been excluded
by R i c h t e r
transferase enhanced uptake
has
ACh c o n t e n t
%.Jhose rate
content Wen solution
in the slices
is i n v e r s e l y
(Roskowski, brain
indirectly
1978;
slices
the present
a marked
activatinF, also ACh synthesis. X-537A
on choline
(1977)
~rX-5~7A
and hip.h a f f i n i t y
related
1978)
of BrX-537A
experiments
was
acetvlelso
choline
to s y n a p t o s o m a l
?~esleP et al.,
output
to brain
brouKht a b o u t
ACh
:.:as n o t stimulated.
~'iere i n c u b a t e d in ~4g2+ enrie~ed
the e f f e c t on ACh
tions used i n
of B r X - 5 3 7 A
at both
ootentinted
Krebs concentrabut only at
Pharmacological Research Communications, Vol. 13, No. 2, 1981
182 the largest
concentration
enhanced.
ACh
incubation
in Mg 2+ enriched
medlum
content
the effect
and t h e r e f o r e
ACh store
bigger
release
was
a t the b e g i n n i n g
could have
of the
than in normal
acted u p o n a larger
release.
can be raised
ACh f o r m a t i o n a n d
formation
m e d i u m was larger
BrX-SB7A
stimulating
The q u e s t i o n
in the slices
on ACh
as to w h e t h e r B r X - 5 3 7 A
only
through
its
stimulates
ionophoric
properties
or by some other mechansims. Richter
(1977)
the analogue duced and
showed
X-B37A o n
a similar
Sokolowsky
(1978)
that in Ca2+~-free medium the effect
ACh r e l e a s e
observation
in Torpedo
reduced
The p o s s i b i l i t y
that
cellular
has been s u g g e s t e d
stores
We observed solution
still
endings,
unrelated
released ACh,
was a p p a r e n t l y
larger t h a n in normal (1966)also
lobster n e r v e
was
showed
larger
(Tucek,
activity
Ca2+-dependent.
is not
The s t l m u l a t o r y neurotransmltters
it has
agent
is reduced (Holz,
been claimed
increase
effect
1977;
transferring Ito et al.,
cations 1978;
output
Dettbarn in the sea w a t e r
acetyltransferase
1977; Ito et al.,
by d e p o l a r i z a t i o n (~asamentl
and Sokolovsky,
of several
m e d i u m added
and its a n a l o g u e
as an i o n o ~ h o r e
Michaelson
formation
in C a 2 + - f r e e
Richter,
that B r X - B B T A
neurotransmitter
solution.
synthesis
of B r X - 8 3 7 A on the release only
Krebs
from cut nerve
than in normal
I'9?7) that choline
1978).
in Ca2+-free
and their ACh
that ACh
in C a 2 + - f r e e
and it is known
and Currel,
a leakage
Krebs
on
Ca 2+ from intra-
incubated
activity,
of BrX-537A
and accumulation.
(Nordman
probably
to neuronal
and R o s e n b e r g
chelating
the effect
might release
that brain slices
and
In our e x p e r i m e n t s
but did not affect ACh f o r m a t i o n BrX-537A
was not re-
was made by M i c h a e l s o n
synaptosomes.
the lack of Ca 2+ only s l i g h t l y ACh output
from brain slices
of
1978)
and
X - 5 3 7 A could as well as by
et al.,
1978).
with
1978;
a
Pharmacological Research Communications, VoL 13, No. 2, 1981
Finally, reduced ACh
d o u b l i n g C a 2+ c o n c e n t r a t i o n
level in the
£anglion
increased
ACh output,
by H u r t e r and Kostial
and ACh synthesis.
In C a 2 + - e n r i p h e d increase amount
in the I'.rebs solution
slices and m a r k e d l y
as shovn~ in the per'fused cervical (I~54),
183
the already
of ACh
at the expense
Krebs s o l u t i o n
released
in normal
of ACh content,
Krebs.
the same
This occurred
partly
partly by stimulatin}~ ACh s y n t h e s i s
an additive
effect of B r X - 5 3 7 A
and h i g h Ca 2+
on ACh output.
In c o n c l u s i o n ,
these
results d e m o n s t r a t e
brain slices Ca 2+ and Mg 2+ c o n c e n t r a t i o n s influence
was still able to
larRe ACh output by p r a c t i c a l l y
This finding s u g g e s t s concentration
BrX-537A
on B r X - 5 3 7 A
that in resting
exert an i n d i r e c t
a c t i o n by m o d u l a t i n g ACh
release, content
and synthesis.
ACKNOh;LEI)GENENTS This work was C.I!.R.
s u p p o r t e d b y grant n~ 7 8 , 0 2 2 2 6 . 0 4
BrX-537A.was
a generous
gift of Roche
from the
and A 23187
of
Ely Lilly Co.
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C.,
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