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Calcineurin is a calmodulin-dependent protein phosphatase
vol. 106, No. 4, 1982 June 30, 1982
BIOCHEMICAL
CALCINEURIN
IS A CALMODULIN-DEPENDENT
Shiaw-Der
Yang,
RESEARCH COMMUNICATIONS Pages 1419-1425
AND BIOPHYSICAL
E. Ann Tallant
PROTEIN PHOSPHATASE
and Wai Yiu
Cheung
Departments of Biochemistry St. Jude Children's Research Hospital and The University of Tennessee Center for the Health Memphis, Tennessee 38101 Received
Sciences
May 19, 1982
SUMMARY: Calcineurin, one of the major calmodulin-binding proteins in the brain, dephosphorylates a phosphorylated protein termed inhibitor-l, a potent inhibitor of protein phosphatase 1. The phosphatase activity was Ca2+- and calmodulin-dependent and was reversed by ECTA or trifluoperazine, an antagonist of calmodulin. Using a radioimmunoassay of calcineurin and a phosphatase activity assay, we found that the two activities coincided in a sucrose density gradient and in a non-denaturing polyacrylamide gel. These results demonstrate that calcineurin is a calmodulin-dependent protein phosphatase. INTRODUCTION Calmodulin,
originally
of CaZ+-dependent dependent
of divergent
there
are numerous
ties
remain
regulated
a Mr of 80,000,
has been The large subunit ( lO-6 dent
(for
(for
inhibitor
four
protein
of this
apparently protein
60,000
is primarily
C&i-BPS0
calcineurin
sites
with
for
proteins,
(5)
in the
with
daltons, brain
calmodulin,
in
(5),
or calcineurin
--in vitro
adenylate
been
calmodulin-
dissociation
inhibits
by competition has not
with
activi-
and 16,500
found
a
In addition,
One of these
interacts
Ca 2+-binding
3).
whose biological
4).
(6),
Ca2+-
regulating
may be additional
of two subunits,
of phosphodiesterase, (4),
see ref.
see ref.
protein
as an activator
is a multifunctional
proteins
of calcineurin
Although
activities
review,
and they
review,
termed
2),
laboratory
in eukaryotes,
calmodulin-binding
This
M (7).
function
enzymes
ratios.
harbors
Ca2+-ATPase
ubiquitous
consists
subunit
(1,
protein
to be identified, enzymes
equimolar
in our
phosphodiesterase
regulatory
variety
discovered
and (7).
and the
small
constants calmodulin-depen-
cyclase calmodulin,
and erythrocyte the biological
clarified. 0006-291X/82/121419-07$01.00/0
1419
Cop.vrrghr 0 1982 .AN rights of reproductfon
by Acirdwnic Press, Inc. m an Y form reserved.
Vol. 106, No. 4, 1982 Recently, contains with
Stewart,
protein
--et al.
phosphatase
calcineurin.
calcineurin
BIOCHEMICAL
In this
is
indeed
(8)
AND BIOPHYSICAL
and suggested
communication,
a protein
that a calcineurin
reported
activity
RESEARCH COMMUNICATIONS
its
we present
phosphatase
whose
preparation
probable
evidence activity
identity to show that
is Ca 2+-
and
calmodulin-dependent. MATERIALS
AND METHODS
Chemicals and Reagents: lz51 (16-20 mCi/jlg) and [Y-~~P]ATP (2 mCi/mmol) were purchased from Amersham; [methyl-14C] methylated bovine serum albumin (0.016 mCi/mg) from New England Nuclear; Triton X-100, phenylmethylsulfonylfluoride, leupeptin, aprotinin, dithiothreitol (DTT), histone (Type II) and casein from Sigma; sodium dodecyl sulfate and Affi-gel blue from Bio-Rad; iodogen (1,3,4,6-tetrachloro-3a, 6a-diphenyl glycoluril) from Pierce Chemical Co. and Sephadex G-100 from Pharmacia. Goat anti-rabbit IgG serum was a gift from Dr. William Walker, St. Jude Children's Research Hospital. Bovine brain was generously supplied by Fineberg Packing Co., Memphis. Rabbit skeletal muscle troponin c was a gift from Dr. Thomas C. Vanaman, Duke University. Protein Preparations: Inhibitor-l was isolated from bovine brain according to a procedure developed for skeletal muscle (9). The catalytic subunit of CAMP-dependent protein kinase was isolated from bovine heart (10). Inhibitor-l, casein and histone were labeled with 32Pi by the cataCalmodulin was lytic subunit of CAMP-dependent protein kinase (11, 12). isolated from bovine brain (13). Calcineurin was also isolated from bovine brain (14), with minor modifications (15). Assay of Protein Phosphatase: Phosphatase activity was assayed by the release of 32Pi from [JLP]-labeled inhibitor-l. The assay mixture, in a final volume of 50 ~1 containing 20 mM Tris-HCl (pH 7.0), 0.5 mM DTT, 0.1 mM 50 ug bovine serum albumin and an appropriate CaC12, 2.5 x 10m7 M calmodulin, amount of calcineurin, was preincubated at 30°C for 5 min. The reaction was initiated with 10 ~1 of [32P]-labeled inhibitor-l (0.4 mg/ml). After 5 min, was determined (16). The amount the reaction was terminated; the 32Pi release of labeled phosphate released generally did not exceed 15% of the substrate originally added to the reaction mixture. Analytical Methods: Calcineurin was assayed by radioimmunoassay (5) Protein was either determined by the method with minor modifications (15). as a standard or estimated of Lowry, --et al. (17) with bovine serum albumin discontinuous polyacrylamide from the absorbance at 280 nm. Non-denaturing The gel was pre-run gel (6%) electrophoresis was performed as in (18). without sample to remove substances which might interfere with subsequent Sucrose density centrifugation determination of the phosphatase activity. using a linear gradient from 5% to 20% sucrose was run in a Beckman SW50.1 weight was determined rotor at 45,000 rpm for 16 h at 4°C; the molecular with [14C]-bovine serum albumin as an internal marker (19). Discontinuous polyacrylamide gel electrophoresis in the presence of SDS and 1 mM EGTA was performed at 22°C in a slab gel containing a linear gradient of 7.5-15% acrylamide (20). RESULTS AND DISCUSSION Calcineurin [3*P]-labeled (2.5
x
10T7
exhibited inhibitor-l
M),
the
some basal as substrate
activity
phosphatase (Table
was increased 1420
1).
activity
when assayed
In the presence
several-fold.
When Ca2'
with
of calmodulin was
BIOCHEMICAL
Vol. 106, No. 4, 1982
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
TABLE 1 Effect
of Ca2+ and Calmodulin
on Protein
Phosphatase
Additions
Activity
' Phosphatase
of
cpm released/5 ?Jone
Calcineurin
Activity min
1223
EGTA
0
Calmodulin
(minus
Ca2+)
1081
Calmodulin
6400
Calmodulin
+ EGTA
43
Trifluoperazine
1152
Calmodulin Troponin
+ Trifluoperazine
1863
c
1208
Each reaction mixture in a final volume of 50 1~1 contained 4 ug inhibitor-l (25,000 cpm), 20 mM Tris-HCl (pH 7.0), 0.5 mM DTT, 50 ug bovine serum albumin, 1.3 x 10-7 11 calcineurin, 0.1 mI1 Ca2+ (unless indicated otherwise), and where present, 2.5 x 10-7 M calmodulin, 1 mF1EGTA, 2.5 x 10-7 M troponin c or 50 IIM trifluoperazine. The phosphatase was assayed as summarized under "Materials and Methods", and is expressed as cpm released per 5 min, the background having been subtracted.
omitted
from
the reaction
the phosphatase
activity
mixture, was slightly
when 1 mM EGTA was included abolished,
whether
troponin
c, a close
activity
at a concentration
troponin
c to 2.5 x 10-6
activity
slightly
that tissue
content
troponin
c free observed
a trace that
troponin
did
c does agent
not
M, lo-fold than
affect
higher
the basal
than level,
(data
not
shown).
substitute to block
the basal
activity
for
is
it
is
remains
in line
calmodulin
the biological but 1421
in an
lower
difficult that
than
of the high
in the physical
of troponin
This
of
resulted
Because
similarity
The possibility concentration
the concentration
calmodulin,
c,
muscle
phosphatase
but dramatically
and troponin
of calmodulin.
known
M. Raising
was
skeletal
stimulate
and
Moreover,
activity
Rabbit not
stimulatory
level.
phosphatase
did
and the close
a high
was not
the basal
was present.
of 2.5 x lo-.'
of calmodulin
not
all
of calmodulin,
of calmodulin. with
itself than
the assay,
of calmodulin
contaminant
anti-psychotic (21),
analogue
of calmodulin
properties
less
calmodulin
greater
chemical
lation
in
or not
in the presence
calmodulin
and
to prepare
the slight
stimu-
c may be contributed with
the general
(3).
Trifluoperazine,
activity
suppressed
the
by
finding
of calmodulin calmodulin-stimu-
an
Vol. 106, No. 4, 1982
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
.c Z 6000 t 4 : 4000 ,o ,” 2Lf? 2000 a \ I
20% Bottom
1
IO
1
Fraction
aa!
1
I
I
20
‘0
1
5% TOP
Number
of calcineurin. A linear Figure 1. Sucrose density gradient centrifugation gradient of 5-20% sucrose in 20 mM Tris-HCl (pH 7.0), 1.0 ti DTT, loaded with 40 ug calcineurin was centrifuged at 45,000 rpm in the Beckman rotor SW50.1 for 16 h at 4oC. Fractions (about 200 ~1) were collected by puncturing the bottom of the tubes; phosphatase and radioimmunological activities were performed as outlined under "Materials and Methods".
lated
activity
to near
the phosphatase
activity
To demonstrate analytical native
its
the
assay
gel
symmetrical, cineurin tube
with also
10, although
calcineurin.
the peak
is not
as an internal
78,000,
a value
by gel
strikingly
filtration
demonstrate
is
of phosphatase corresponded
the
by polyacrylamide
conditions.
Two gels
phatase
that
to the
1 shows
and by phosphatase activity
peak
1251+alcineurin
This
is
using
for
at
probably
recognized
due to
by the
[14C]-bovine
antiserum
weight
calcineurin
is
of cal-
with
to a molecular 80,000
Figure
Radioimmunoassay
symmetrical.
close
was examined
other
10.
and
of obtained
(14).
To further
the
that
phosphatase,
performed.
competition
of calcineurin
marker
the notion
centrifugation
The phosphatase at tube
greatest
albumin
gradient were
gradient.
The peak activity
the
by radioimmunoassay
the
product
support
with
density
maximum activity
exhibits
some degradation
sucrose electrophoresis
density
results
of calcineurin
of calcineurin
in a sucrose
These
and calmodulin-dependent.
identity with
polyacrylamide profile
level.
is Ca2+-
experiments
the activity
basal
was sliced activity.
identity gel
of these
electrophoresis
used.
one was stained
to determine
radioimmunological
were
Again
the peak of phosphatase 1422
two proteins, under for
non-denaturing
protein activity
activity
calcineurin
pattern; and phos-
was symmetrical,
BIOCHEMICAL
Vol. 106, No. 4, 1982
AND BIOPHYSICAL
Sltce
Figure 2. calcineurin. 2 h. The
Non-denaturing The gel was reservoir buffer
RESEARCH COMMUNICATIONS
Number
discontinuous 6% polyacrylamide was replaced
polyacrylamide gel electrophoresis and pre-run without sample by a fresh buffer and 30 ~g of
cineurin was applied to the gel. At the end of electrophoresis, stained for protein with Coomassie brilliant blue and the other 2-mm slices. The protein, extracted from each slice by shaking 4oC
at
in
200
~1 of
20 ti
Tris-HCl
(pH
7.0),
1.0
phosphatase and for calcineurin as outlined anode is at the bottom of the gel.
although
that
seen in peaks
of the
the sucrose
were
mirror
density images
migrated
as a diffused
diffused
region
tase
activity;
presumably
radioimmunoassay
the main
however,
it
sodium
dodecyl
protein
bands
(Lane
of the A).
activity taminating
usually
sulfate
calcineurin
the
may be associated
with
(4-7). before
these calcineurin
preparation. with
Calcineurin
not
results
and not with
of protein 1423
electrophoresis. gradient
was examined 3 (Lane
pattern
that
the
some minor
in a
and 16,500, identical
sucrose
gradient
phosphatase proteins
phosphatase
co-migrates
in
B) shows two
appears
in the
that that
activity,
of 60,000
indicate
gel.
show any phospha-
density
centrifugation
The possibility a trace
2.
Figure
This
pattern
in Figure
during
weights
The
two activity
pattern
gel.
to molecular
of calcineurin
Collectively, resides
and the protein
corresponding
of the
polyacrylamide
sucrose
for
and Methods".
some immunological
from the
polyacrylamide
assayed
was
the
band did
showed
one gel cut into overnight
Further,
of calcineurin
fraction
1 was concentrated,
two subunits
1.
as shown
protein
due to some denaturation
Figure
to that
of Figure
of one another,
trailing
was
reminiscent
band in the non-denaturing
The peak activity
the
was not,
gradient
mM DTT,
in "Materials
of for cal-
con-
activity with
cal-
The
Vol. 106, No. 4, 1982
BIOCHEMICAL
AND BIOPHYSICAL
A
B
RESEARCH COMMUNICATIONS
C
--
Electrophoresis of calcineurin on SDS-polyacrylamide gel. ElecFigure 3. trophoresis was performed on a 7.515% gradient polyacrylamide slab gel, in the presence of 1 mEI EGTA, as described in "Materials and Methods". Lane A, 10 ug of calcineurin before sucrose gradient centrifugation; Lane B, activity weight markers: peak from sucrose gradient of Figure 1; Lane C, molecular phosphorylase b (Mr = 94,000), bovine serum albumin (Mr = 67,000), ovalbumin (Mr = 43,000), carbonic anhydrase (Mr = 30,000), trypsin inhibitor (Mr = 20,100) and a-lactalbumin (Mr = 14,400). The anode is at the bottom of the gel.
cineurin but
under
it
our
appears
it
the
interest.
inhibits
(11).
In addition
to
Calcineurin
that
of inhibitor-l
has a rather
be totally
excluded,
broad
for
phosphatase
calcineurin
in this
by a CAMP-dependent 1 (22,
23),
which
has
study,
broad
that
of
many
other
inhibitor-l,
we have
catalyzed (data substrate
their not
used
casein
is not
specificity. 1424
thus
active.
regulatory
pro-
mechanism. and histone
dephosphorylation
shown),
kinase,
substrate
form of inhibitor-l like
is of
protein
by a phosphorylation-dephosphorylation
strates. to
used
of inhibitor-l,
is controlled
teins,
cannot
The dephosphorylated
the activity
Thus,
substrate
When phosphorylated
a protein
specificity
conditions
unlikely.
Inhibitor-l, special
experimental
suggesting
as sub-
at a rate that
comparable
the enzyme
BIOCHEMICAL
Vol. 106, No. 4, 1982 We have the that
caudate
shown that nucleus
calcineurin
and dendritic
is primarily microtubules
shown that
that
calcineurin
is
activities
are
whose with
a specific
nervous
calcineurin
and putamen
have
is (5).
rich
associated
increases
a protein regulated activity
in the brain,
with
with
phosphatase by calmodulin. will
RESEARCH COMMUNICATIONS
Immunohistochemical
in mouse basal
calcineurin
enzymic
AND BIOPHYSICAL
help
particularly studies
the postsynaptic
ganglia
(24).
synaptogenesis
More
More to define
densities recently,
we
The finding list
importantly, its
revealed
(25).
adds to the growing
in
function
of enzymes its
identity in the
system.
Acknowledgements: This work was supported by grants CA 21765, NS 08059 and GM 28178 from the National Institutes of Health and by ALSAC. We are grateful to Shawn Hawkins for excellent technical assistance and to Pat Nicholas for typing the manuscript. REFERENCES 1. 2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16. 17. 18. 19. 20. 21. 22. 23. 24. 25.
Cheung, W.Y. (1981) J. Cyclic Nucleotide Res. 7, 71-84. Cheung, W.Y. (1970) Biochem. Biophys. Res. Commun. 38, 533-538. Cheung, W.Y. (1980) Science 207, 19-27. Wang, J.H., Sharma, R.K. and Tam, S.W. (1980) In Calcium and Cell Function (Cheung, W.Y., ed.) Vol. 1, pp. 305-328, Academic Press, New Yor;;. Wallace, R.W., Tallant, E.A. and Cheung, W.Y. (1980) Biochemistry 19, 1831-1837. Wang, J.H. and Desai, R. (1976) Biochem. Biophys. Res. Commun. 72, 926-937. Klee, C.B., Crouch, T.H. and Krinks, M.H. (1979) Proc. Natl. Acad. Sci. USA 76, 6270-6273. Stewart, A.A., Ingebritsen, T.S., Manalan, A., Klee, C.B. and Cohen,. P. (1982) FEBS Lett. 137, 80-84. Foulkes, J.G. and Cohen, P. (1979) Eur. J. Biochem. 97, 251-256. Sugden, P.H., Holladay, L.A., Reimann, E.M. and Corbin, J.D. (1976) Biochem. 3. 159, 409-422. Stewart, A.A., Hemmings, B.A., Cohen, P., Goris, J. and Merlevede, W. (1981) Eur. J. Biochem. 115, 197-205. Khandelwal, R.L., Vandenheede, J.R. and Krebs, E.G. (1976) J. Biol. Chem. 251, 4850-4868. Wallace, R.W., Tallant, E.A. and Cheung, W.Y. (1980) In Calcium and Cell Function (Cheung, W.Y., ed.) Vol. 1, pp. 13-40, Academic Press, NewYork. Wallace, R.W., Lynch, T.J., Tallant, E.A. and Cheung, W.Y. (1978) J. Biol. Chem. 254, 377-382. Tallant, E.A., Wallace, R.W., Yang, S.D. and Cheung, W.Y. (1952) Meth. Enzymol. ( in preparation). Yang, S.-D., Vandenheede, J.R., Goris, J. and Merlevede, W. (1980) J. Biol. Chem. 255, 11759-11767. Lowry, O-H., Rosebrough, N.J., Farr, A.L. and Randall, R.J. (1951) J. Biol. Chem. 183, 265-275. Davis, B.J. (1964) Ann. N. Y. Acad. Sci. 121, 405-427. Martin, R.G. and Ames, B.N. (1961) J. Biol. Chem. 236, 1372-1379. Laemmli, U.K. (1970) Nature 227, 680-684. Levin, R.M. and Weiss, B. (1976) Mol. Pharmacol. 12, 581-589. Huang, F.L. and Glinsmann, W.H. (1976) Eur. J. Biochem. 70, 419-426. Cohen, P. (1978) Curr. Top. Cell Reg. 14, 117-196. Wood, J.G., Wallace, R.W., Whitaker, J.N. and Cheung, W.Y. (1980) J. Cell Biol. 84, 66-76. Tallant, E.A. and Cheung, W.Y. (1982) Fed. Proc. 41, 1213 (Abstr.). 1425
BIOCHEMICAL
CALCINEURIN
IS A CALMODULIN-DEPENDENT
Shiaw-Der
Yang,
RESEARCH COMMUNICATIONS Pages 1419-1425
AND BIOPHYSICAL
E. Ann Tallant
PROTEIN PHOSPHATASE
and Wai Yiu
Cheung
Departments of Biochemistry St. Jude Children's Research Hospital and The University of Tennessee Center for the Health Memphis, Tennessee 38101 Received
Sciences
May 19, 1982
SUMMARY: Calcineurin, one of the major calmodulin-binding proteins in the brain, dephosphorylates a phosphorylated protein termed inhibitor-l, a potent inhibitor of protein phosphatase 1. The phosphatase activity was Ca2+- and calmodulin-dependent and was reversed by ECTA or trifluoperazine, an antagonist of calmodulin. Using a radioimmunoassay of calcineurin and a phosphatase activity assay, we found that the two activities coincided in a sucrose density gradient and in a non-denaturing polyacrylamide gel. These results demonstrate that calcineurin is a calmodulin-dependent protein phosphatase. INTRODUCTION Calmodulin,
originally
of CaZ+-dependent dependent
of divergent
there
are numerous
ties
remain
regulated
a Mr of 80,000,
has been The large subunit ( lO-6 dent
(for
(for
inhibitor
four
protein
of this
apparently protein
60,000
is primarily
C&i-BPS0
calcineurin
sites
with
for
proteins,
(5)
in the
with
daltons, brain
calmodulin,
in
(5),
or calcineurin
--in vitro
adenylate
been
calmodulin-
dissociation
inhibits
by competition has not
with
activi-
and 16,500
found
a
In addition,
One of these
interacts
Ca 2+-binding
3).
whose biological
4).
(6),
Ca2+-
regulating
may be additional
of two subunits,
of phosphodiesterase, (4),
see ref.
see ref.
protein
as an activator
is a multifunctional
proteins
of calcineurin
Although
activities
review,
and they
review,
termed
2),
laboratory
in eukaryotes,
calmodulin-binding
This
M (7).
function
enzymes
ratios.
harbors
Ca2+-ATPase
ubiquitous
consists
subunit
(1,
protein
to be identified, enzymes
equimolar
in our
phosphodiesterase
regulatory
variety
discovered
and (7).
and the
small
constants calmodulin-depen-
cyclase calmodulin,
and erythrocyte the biological
clarified. 0006-291X/82/121419-07$01.00/0
1419
Cop.vrrghr 0 1982 .AN rights of reproductfon
by Acirdwnic Press, Inc. m an Y form reserved.
Vol. 106, No. 4, 1982 Recently, contains with
Stewart,
protein
--et al.
phosphatase
calcineurin.
calcineurin
BIOCHEMICAL
In this
is
indeed
(8)
AND BIOPHYSICAL
and suggested
communication,
a protein
that a calcineurin
reported
activity
RESEARCH COMMUNICATIONS
its
we present
phosphatase
whose
preparation
probable
evidence activity
identity to show that
is Ca 2+-
and
calmodulin-dependent. MATERIALS
AND METHODS
Chemicals and Reagents: lz51 (16-20 mCi/jlg) and [Y-~~P]ATP (2 mCi/mmol) were purchased from Amersham; [methyl-14C] methylated bovine serum albumin (0.016 mCi/mg) from New England Nuclear; Triton X-100, phenylmethylsulfonylfluoride, leupeptin, aprotinin, dithiothreitol (DTT), histone (Type II) and casein from Sigma; sodium dodecyl sulfate and Affi-gel blue from Bio-Rad; iodogen (1,3,4,6-tetrachloro-3a, 6a-diphenyl glycoluril) from Pierce Chemical Co. and Sephadex G-100 from Pharmacia. Goat anti-rabbit IgG serum was a gift from Dr. William Walker, St. Jude Children's Research Hospital. Bovine brain was generously supplied by Fineberg Packing Co., Memphis. Rabbit skeletal muscle troponin c was a gift from Dr. Thomas C. Vanaman, Duke University. Protein Preparations: Inhibitor-l was isolated from bovine brain according to a procedure developed for skeletal muscle (9). The catalytic subunit of CAMP-dependent protein kinase was isolated from bovine heart (10). Inhibitor-l, casein and histone were labeled with 32Pi by the cataCalmodulin was lytic subunit of CAMP-dependent protein kinase (11, 12). isolated from bovine brain (13). Calcineurin was also isolated from bovine brain (14), with minor modifications (15). Assay of Protein Phosphatase: Phosphatase activity was assayed by the release of 32Pi from [JLP]-labeled inhibitor-l. The assay mixture, in a final volume of 50 ~1 containing 20 mM Tris-HCl (pH 7.0), 0.5 mM DTT, 0.1 mM 50 ug bovine serum albumin and an appropriate CaC12, 2.5 x 10m7 M calmodulin, amount of calcineurin, was preincubated at 30°C for 5 min. The reaction was initiated with 10 ~1 of [32P]-labeled inhibitor-l (0.4 mg/ml). After 5 min, was determined (16). The amount the reaction was terminated; the 32Pi release of labeled phosphate released generally did not exceed 15% of the substrate originally added to the reaction mixture. Analytical Methods: Calcineurin was assayed by radioimmunoassay (5) Protein was either determined by the method with minor modifications (15). as a standard or estimated of Lowry, --et al. (17) with bovine serum albumin discontinuous polyacrylamide from the absorbance at 280 nm. Non-denaturing The gel was pre-run gel (6%) electrophoresis was performed as in (18). without sample to remove substances which might interfere with subsequent Sucrose density centrifugation determination of the phosphatase activity. using a linear gradient from 5% to 20% sucrose was run in a Beckman SW50.1 weight was determined rotor at 45,000 rpm for 16 h at 4°C; the molecular with [14C]-bovine serum albumin as an internal marker (19). Discontinuous polyacrylamide gel electrophoresis in the presence of SDS and 1 mM EGTA was performed at 22°C in a slab gel containing a linear gradient of 7.5-15% acrylamide (20). RESULTS AND DISCUSSION Calcineurin [3*P]-labeled (2.5
x
10T7
exhibited inhibitor-l
M),
the
some basal as substrate
activity
phosphatase (Table
was increased 1420
1).
activity
when assayed
In the presence
several-fold.
When Ca2'
with
of calmodulin was
BIOCHEMICAL
Vol. 106, No. 4, 1982
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
TABLE 1 Effect
of Ca2+ and Calmodulin
on Protein
Phosphatase
Additions
Activity
' Phosphatase
of
cpm released/5 ?Jone
Calcineurin
Activity min
1223
EGTA
0
Calmodulin
(minus
Ca2+)
1081
Calmodulin
6400
Calmodulin
+ EGTA
43
Trifluoperazine
1152
Calmodulin Troponin
+ Trifluoperazine
1863
c
1208
Each reaction mixture in a final volume of 50 1~1 contained 4 ug inhibitor-l (25,000 cpm), 20 mM Tris-HCl (pH 7.0), 0.5 mM DTT, 50 ug bovine serum albumin, 1.3 x 10-7 11 calcineurin, 0.1 mI1 Ca2+ (unless indicated otherwise), and where present, 2.5 x 10-7 M calmodulin, 1 mF1EGTA, 2.5 x 10-7 M troponin c or 50 IIM trifluoperazine. The phosphatase was assayed as summarized under "Materials and Methods", and is expressed as cpm released per 5 min, the background having been subtracted.
omitted
from
the reaction
the phosphatase
activity
mixture, was slightly
when 1 mM EGTA was included abolished,
whether
troponin
c, a close
activity
at a concentration
troponin
c to 2.5 x 10-6
activity
slightly
that tissue
content
troponin
c free observed
a trace that
troponin
did
c does agent
not
M, lo-fold than
affect
higher
the basal
than level,
(data
not
shown).
substitute to block
the basal
activity
for
is
it
is
remains
in line
calmodulin
the biological but 1421
in an
lower
difficult that
than
of the high
in the physical
of troponin
This
of
resulted
Because
similarity
The possibility concentration
the concentration
calmodulin,
c,
muscle
phosphatase
but dramatically
and troponin
of calmodulin.
known
M. Raising
was
skeletal
stimulate
and
Moreover,
activity
Rabbit not
stimulatory
level.
phosphatase
did
and the close
a high
was not
the basal
was present.
of 2.5 x lo-.'
of calmodulin
not
all
of calmodulin,
of calmodulin. with
itself than
the assay,
of calmodulin
contaminant
anti-psychotic (21),
analogue
of calmodulin
properties
less
calmodulin
greater
chemical
lation
in
or not
in the presence
calmodulin
and
to prepare
the slight
stimu-
c may be contributed with
the general
(3).
Trifluoperazine,
activity
suppressed
the
by
finding
of calmodulin calmodulin-stimu-
an
Vol. 106, No. 4, 1982
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
.c Z 6000 t 4 : 4000 ,o ,” 2Lf? 2000 a \ I
20% Bottom
1
IO
1
Fraction
aa!
1
I
I
20
‘0
1
5% TOP
Number
of calcineurin. A linear Figure 1. Sucrose density gradient centrifugation gradient of 5-20% sucrose in 20 mM Tris-HCl (pH 7.0), 1.0 ti DTT, loaded with 40 ug calcineurin was centrifuged at 45,000 rpm in the Beckman rotor SW50.1 for 16 h at 4oC. Fractions (about 200 ~1) were collected by puncturing the bottom of the tubes; phosphatase and radioimmunological activities were performed as outlined under "Materials and Methods".
lated
activity
to near
the phosphatase
activity
To demonstrate analytical native
its
the
assay
gel
symmetrical, cineurin tube
with also
10, although
calcineurin.
the peak
is not
as an internal
78,000,
a value
by gel
strikingly
filtration
demonstrate
is
of phosphatase corresponded
the
by polyacrylamide
conditions.
Two gels
phatase
that
to the
1 shows
and by phosphatase activity
peak
1251+alcineurin
This
is
using
for
at
probably
recognized
due to
by the
[14C]-bovine
antiserum
weight
calcineurin
is
of cal-
with
to a molecular 80,000
Figure
Radioimmunoassay
symmetrical.
close
was examined
other
10.
and
of obtained
(14).
To further
the
that
phosphatase,
performed.
competition
of calcineurin
marker
the notion
centrifugation
The phosphatase at tube
greatest
albumin
gradient were
gradient.
The peak activity
the
by radioimmunoassay
the
product
support
with
density
maximum activity
exhibits
some degradation
sucrose electrophoresis
density
results
of calcineurin
of calcineurin
in a sucrose
These
and calmodulin-dependent.
identity with
polyacrylamide profile
level.
is Ca2+-
experiments
the activity
basal
was sliced activity.
identity gel
of these
electrophoresis
used.
one was stained
to determine
radioimmunological
were
Again
the peak of phosphatase 1422
two proteins, under for
non-denaturing
protein activity
activity
calcineurin
pattern; and phos-
was symmetrical,
BIOCHEMICAL
Vol. 106, No. 4, 1982
AND BIOPHYSICAL
Sltce
Figure 2. calcineurin. 2 h. The
Non-denaturing The gel was reservoir buffer
RESEARCH COMMUNICATIONS
Number
discontinuous 6% polyacrylamide was replaced
polyacrylamide gel electrophoresis and pre-run without sample by a fresh buffer and 30 ~g of
cineurin was applied to the gel. At the end of electrophoresis, stained for protein with Coomassie brilliant blue and the other 2-mm slices. The protein, extracted from each slice by shaking 4oC
at
in
200
~1 of
20 ti
Tris-HCl
(pH
7.0),
1.0
phosphatase and for calcineurin as outlined anode is at the bottom of the gel.
although
that
seen in peaks
of the
the sucrose
were
mirror
density images
migrated
as a diffused
diffused
region
tase
activity;
presumably
radioimmunoassay
the main
however,
it
sodium
dodecyl
protein
bands
(Lane
of the A).
activity taminating
usually
sulfate
calcineurin
the
may be associated
with
(4-7). before
these calcineurin
preparation. with
Calcineurin
not
results
and not with
of protein 1423
electrophoresis. gradient
was examined 3 (Lane
pattern
that
the
some minor
in a
and 16,500, identical
sucrose
gradient
phosphatase proteins
phosphatase
co-migrates
in
B) shows two
appears
in the
that that
activity,
of 60,000
indicate
gel.
show any phospha-
density
centrifugation
The possibility a trace
2.
Figure
This
pattern
in Figure
during
weights
The
two activity
pattern
gel.
to molecular
of calcineurin
Collectively, resides
and the protein
corresponding
of the
polyacrylamide
sucrose
for
and Methods".
some immunological
from the
polyacrylamide
assayed
was
the
band did
showed
one gel cut into overnight
Further,
of calcineurin
fraction
1 was concentrated,
two subunits
1.
as shown
protein
due to some denaturation
Figure
to that
of Figure
of one another,
trailing
was
reminiscent
band in the non-denaturing
The peak activity
the
was not,
gradient
mM DTT,
in "Materials
of for cal-
con-
activity with
cal-
The
Vol. 106, No. 4, 1982
BIOCHEMICAL
AND BIOPHYSICAL
A
B
RESEARCH COMMUNICATIONS
C
--
Electrophoresis of calcineurin on SDS-polyacrylamide gel. ElecFigure 3. trophoresis was performed on a 7.515% gradient polyacrylamide slab gel, in the presence of 1 mEI EGTA, as described in "Materials and Methods". Lane A, 10 ug of calcineurin before sucrose gradient centrifugation; Lane B, activity weight markers: peak from sucrose gradient of Figure 1; Lane C, molecular phosphorylase b (Mr = 94,000), bovine serum albumin (Mr = 67,000), ovalbumin (Mr = 43,000), carbonic anhydrase (Mr = 30,000), trypsin inhibitor (Mr = 20,100) and a-lactalbumin (Mr = 14,400). The anode is at the bottom of the gel.
cineurin but
under
it
our
appears
it
the
interest.
inhibits
(11).
In addition
to
Calcineurin
that
of inhibitor-l
has a rather
be totally
excluded,
broad
for
phosphatase
calcineurin
in this
by a CAMP-dependent 1 (22,
23),
which
has
study,
broad
that
of
many
other
inhibitor-l,
we have
catalyzed (data substrate
their not
used
casein
is not
specificity. 1424
thus
active.
regulatory
pro-
mechanism. and histone
dephosphorylation
shown),
kinase,
substrate
form of inhibitor-l like
is of
protein
by a phosphorylation-dephosphorylation
strates. to
used
of inhibitor-l,
is controlled
teins,
cannot
The dephosphorylated
the activity
Thus,
substrate
When phosphorylated
a protein
specificity
conditions
unlikely.
Inhibitor-l, special
experimental
suggesting
as sub-
at a rate that
comparable
the enzyme
BIOCHEMICAL
Vol. 106, No. 4, 1982 We have the that
caudate
shown that nucleus
calcineurin
and dendritic
is primarily microtubules
shown that
that
calcineurin
is
activities
are
whose with
a specific
nervous
calcineurin
and putamen
have
is (5).
rich
associated
increases
a protein regulated activity
in the brain,
with
with
phosphatase by calmodulin. will
RESEARCH COMMUNICATIONS
Immunohistochemical
in mouse basal
calcineurin
enzymic
AND BIOPHYSICAL
help
particularly studies
the postsynaptic
ganglia
(24).
synaptogenesis
More
More to define
densities recently,
we
The finding list
importantly, its
revealed
(25).
adds to the growing
in
function
of enzymes its
identity in the
system.
Acknowledgements: This work was supported by grants CA 21765, NS 08059 and GM 28178 from the National Institutes of Health and by ALSAC. We are grateful to Shawn Hawkins for excellent technical assistance and to Pat Nicholas for typing the manuscript. REFERENCES 1. 2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16. 17. 18. 19. 20. 21. 22. 23. 24. 25.
Cheung, W.Y. (1981) J. Cyclic Nucleotide Res. 7, 71-84. Cheung, W.Y. (1970) Biochem. Biophys. Res. Commun. 38, 533-538. Cheung, W.Y. (1980) Science 207, 19-27. Wang, J.H., Sharma, R.K. and Tam, S.W. (1980) In Calcium and Cell Function (Cheung, W.Y., ed.) Vol. 1, pp. 305-328, Academic Press, New Yor;;. Wallace, R.W., Tallant, E.A. and Cheung, W.Y. (1980) Biochemistry 19, 1831-1837. Wang, J.H. and Desai, R. (1976) Biochem. Biophys. Res. Commun. 72, 926-937. Klee, C.B., Crouch, T.H. and Krinks, M.H. (1979) Proc. Natl. Acad. Sci. USA 76, 6270-6273. Stewart, A.A., Ingebritsen, T.S., Manalan, A., Klee, C.B. and Cohen,. P. (1982) FEBS Lett. 137, 80-84. Foulkes, J.G. and Cohen, P. (1979) Eur. J. Biochem. 97, 251-256. Sugden, P.H., Holladay, L.A., Reimann, E.M. and Corbin, J.D. (1976) Biochem. 3. 159, 409-422. Stewart, A.A., Hemmings, B.A., Cohen, P., Goris, J. and Merlevede, W. (1981) Eur. J. Biochem. 115, 197-205. Khandelwal, R.L., Vandenheede, J.R. and Krebs, E.G. (1976) J. Biol. Chem. 251, 4850-4868. Wallace, R.W., Tallant, E.A. and Cheung, W.Y. (1980) In Calcium and Cell Function (Cheung, W.Y., ed.) Vol. 1, pp. 13-40, Academic Press, NewYork. Wallace, R.W., Lynch, T.J., Tallant, E.A. and Cheung, W.Y. (1978) J. Biol. Chem. 254, 377-382. Tallant, E.A., Wallace, R.W., Yang, S.D. and Cheung, W.Y. (1952) Meth. Enzymol. ( in preparation). Yang, S.-D., Vandenheede, J.R., Goris, J. and Merlevede, W. (1980) J. Biol. Chem. 255, 11759-11767. Lowry, O-H., Rosebrough, N.J., Farr, A.L. and Randall, R.J. (1951) J. Biol. Chem. 183, 265-275. Davis, B.J. (1964) Ann. N. Y. Acad. Sci. 121, 405-427. Martin, R.G. and Ames, B.N. (1961) J. Biol. Chem. 236, 1372-1379. Laemmli, U.K. (1970) Nature 227, 680-684. Levin, R.M. and Weiss, B. (1976) Mol. Pharmacol. 12, 581-589. Huang, F.L. and Glinsmann, W.H. (1976) Eur. J. Biochem. 70, 419-426. Cohen, P. (1978) Curr. Top. Cell Reg. 14, 117-196. Wood, J.G., Wallace, R.W., Whitaker, J.N. and Cheung, W.Y. (1980) J. Cell Biol. 84, 66-76. Tallant, E.A. and Cheung, W.Y. (1982) Fed. Proc. 41, 1213 (Abstr.). 1425