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Ca++ induced conformational changes in the Ca++ binding component of troponin
Vol. 47, No. 4, 1972
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
ca++ INDUCED CONFORMATIONAL CHANGES IN THE Ca++ BI"IJDING COMPONENT OF TROPONIN Jean-Paul van Eerd and Yukishige Kawasaki Institute of Molecular Biology and Department of Physics, Nagoya University, Nagoya, Japan 464.
Received April
17, 1972
The Ca++binding component of troponin undergoes reversible conformational changes in the presence or absence of micromolar amounts of Ca++. The presence of Ca++ causes an increase in the fluorescence intensity of the tyrosine residues as well as an The binding constant is 5.106M-1. increase of the helix content. Fluorescence polarisation shows that the motion of the tyrosine residues is much smaller in the presence than in the absence of Ca++. Thus the Ca++ binding component of troponin appears more rigid in the presence than in the absence of Ca++. Summary.
Muscle which
contraction
released
the nerve,
from the
bind
assumed that
troponin,
which
troponin. into
interest In three
(Greaser
Ca++. This usually
Phe/Tyr
component
conformation
induces
1972, by Academic
to myosin.
has been fractionated
only
substructure
et al. 3),
one of which identified
because of the
and 4 sub-
appears as it
absence
of
to bind
has an unof tryptophan
ratio5. whether
indeed
the conformation
on the presence
Ca++ induces
component. 859
Copyright 0
actin
and ulti-
troponin
3 (Ebashi
is
change in
in the
can be readily
(CBC) changes
of this
filaments
a conformational
of
of 1 . It
recently
and Mueller2),
to test
that
on excitation
on the thin
in the binding
ratio
amounts of Ca++,
a change in tropomyosin
laboratories
low E2So/E2b0
We have found
located
and Gergely4),
We set out ding
reticulum
has arisen
component
and the high
sarcoplasmic
resulting
2 (~Hartshorne
units
by small
Ca++ induces
in turn
in actin,
Accordingly
regulated
to troponin
generally
mately
is
Press, Inc.
of this
or absence
a striking
Ca++ binof Ca++.
change in the
Vol. 47, No. 4, 1972
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
MATERIALS AND METHODS. Preparation rabbit
of
skeletal
muscle
al. 6 . Troponin inability
in the
troponin
described
the
absence
and CBC. Troponin
according
was checked
to regulate
myosin from
troponin
for
to the
procedure
the absence
of
electrophoresis
in the presence
and showed very
little
in 6M ura as
CBC showed a single of sodium dodecyl
tryptophan
acto-
CBC was prepared
on DEAE Sephadex
and Gergely4.
et
by its
synthetic
of any added tropomyosin.
from
of Ebashi
of tropomyosin
superprecipitation
by chromatography
by Greaser
was prepared
fluorescence
band on gel
sulphate
(SDS)'
on excitation
at
290 nm. Ultraviolet with
absorption.
The UV spectrum
a Zeiss model PMQ 2 spectrophotometer. Fluorescence
cence
An Hitachi
spectroscopy.
spectrophotometer
was used for
was water-jacketed
Haake thermoregulator.
Tyrosine
after
always
rin's
less
and connected
fluorescence
a
at
306
than
at 276 nm. The OD value of the sample was 276 0.10. Polacoat ultraviolet polarising filters measuring
the degree
P, at
a number of temperatures
was used to change the viscosity Optical
Rotation
Dispersion
was a Jasco Autospectrometer ted from
with
was observed
of
fluorescence
The rotary molecular motion was calculated 8 equation , from observations of the degree of
polarisation cerol
measurements.
excitation
(105 UV) were used for risation.
model MPF-2A fluores-
fluorescence
The sample compartment
nm.,
of CBC was measured
the
[ml ;33 value was taken 9 .
specific of 14,700,
ca++ concentration.
at constant
measurements.
and for
at
+-I- concentrations Ca
860
Per-
fluorescence Gly-
temperature.
The apparatus content
233 nm. For
0% helix
using
and viscosities.
UV 5. The helix
rotations
pola-
was calcula-
100% helix
a [ml;33
used
value
a of
were adjusted
2200
using
BIOCHEMICAL
Vol. 47, No. 4, 1972
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
++ of Ca and 0.5 mM EGTA (ethylene
a Ca-buffer
tetraacetic
ethyl
ether)-N,N' 10 at pH 6.8 . Protein
acid)
bis
(n-amino-
in 10 mM cacodylate-HCl
concentration.
Protein 11 the method of Lowry .
mined using
glycol
concentrations
buffer
were deter-
.15-
d d
.I o-
.05-
I 260
I 260 WQVO
Figure
I 300 Length (n m )
1. Absorption spectrum of the Ca+' binding component of troponin. The protein concentration is 0.26 mg/ml in 0.3 mM NaHC03. The spectrum is identical in the presence and absence of Ca++.
RESULTS AND DISCUSSION. Ultraviolet gure
spectrum.
1. The maximum at
tyrosine
absorption.
The UV spectrum
275 nm. corresponds
The maxima at 259,
pond to maxima of the phenylalanine the
finestructure
served than
of the
because those
the molar
of tyrosine
phan is
present
structure
of
extinction
and the
tyrosine
intensity
In most proteins cannot
of phenylalanine
absorption and helix
861
is
low5,
easily
content.
be ob-
is much lower
In CBC however,
content
the
266 and 269 nm. corres-
absorption
and tryptophan.
shown in Fi-
to the maximum of
absorption.
phenylalanine
the phenylalanine
Fluorescence
of CBC is
no trypto-
so that
the
fine-
can be detected. The helix
content
Vol. 47, No. 4, 1972
BIOCHEMICAL
RESEARCH COMMUNICATIONS
content and change in fluorescence intensity 2. The helix of CBC versus Ca++ concentration at 250C. o-o ; helix content,AA; fluorescence intensity. Vertical bars represent possible errors due to line width. Protein concentrations are 0.45 and 0.12 mg/ml for the helix content and the fluorescence measurements respectively. The binding constant calculated from these curves is 5.106M-l.
Figure
and the
tyrosine
fluorescence
the Ca++ concentration distinct crease
AND BIOPHYSICAL
increase in the
The binding curves
is
5.4x106M-1 method.
intensity
are plotted
in helix
fluorescence
constant
for
5x106M-1 . This
of
CBC as a function
in Figure which
content,
2. There
is
paralleled
The increase
a very by an in-
intensity of the tyrosine residues. ++ estimated from these the Ca -CBC complex,
in good agreement with 12 by Hartshorne and Pyun using
obtained
is
of
is
in helix
content
and the
the value
of
the Chelex
increase
100
in fluores-
cence
intensity could be reversed by adding EGTA to bind any ex++ in fluorescence intensity could not have cess Ca . The increase been caused by aggregation
of CBC molecules
but
only
by an intra-
molecular
change because the UV spectrum was identical in the pre++ sence and absence of Ca . The conformational change in CBC occurs ++ concentrations in the micromolar range, i.e. at the phyat Ca siological
concentration
Fluorescence the
Perrin's
plot
where muscle
polarisation. a straight
With line
contraction changing
is regulated. temperature
in the presence
a62
shows
of Ca++ (see
Vol. 47, No. 4, 1972
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
7
a6 \
+-+++-h T/q
(OK / poise
)
Figure
3. The effect of temperature and viscosity on the fluorescence polarisation of CBC. o-o ; heating curve at pCa>8 a-0 ; heating curve at pCa=5.7.A-A; isothermal curve at 30°c and pCa>8.A-A ; isothermal curve at 30°C and bars represent the standard deviation pCa=5.7. Vertical of 3 observations. T is the absolute temperature and qis the viscosity of the solvent.
Figure
3).
straight
On the other
hand there
is a large
in the absence of Ca+*. This suggests ++ the tyrosine residues occupy sites of Ca
protein
molecule
the absence thermal
which allow only ++ of Ca , the tyrosine
activation
of motion
very
limited
residues
independent
the CBC molecule.
More accurate
tyrosine
residues
in CBC can be obtained
changing
viscosities
see Figure
of motion
is
at a constant 31, because
constant.
in that
For the
However,
overall
relaxation
times
fluorescence
thermal
of
of
plot
(isothermal
case the
in
motion
from a Perrin's
temperature
the
can undergo
of the
rotational
in the
within
motion.
easily
from a
that
line
presence
plot,
deviation
the with
Perrin's
activation
lifetimes
at 30°c we
used the values of 1.8 and 2.2 nsec in the absence and presence ++ These values were derived from a value of of Ca respectively. 2.6 nsec for at 23OC
the
fluorescence
13 and corrected
for
lifetime fluorescence
863
of
free
tyrosine
intensity
in water
changes
(Fi-
Vol. 47, No. 4, 1972
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Temperature
Figure
gure of
( “C
)
4. The temperature effect on the fluorescence intensity of CBC. o-o ; at pCa>8, m-o ; at pCa=5.7, e-8 ; the relabetween the tive difference in fluorescence intensity 2 conditions. Vertical bars represent possible errors due to line width. Using
4).
14.5
these
data
we obtained
a rotational
relaxation time ++ respecand absence of Ca
and 29.2 nsec in the presence
tively
at
30°C.
ture
variation
These values that
becomes rather
rigid
The temperature in Figure
4. Strong
observed,
while
Ca++ -free
CBC is
mational siological
support
CBC is
flexible
on the
addition
effect
on the
thermal
change in CBC is
in the of
with
of
therefore
tempera-
Ca++ and
Ca++.
the
in intensity raising
of the
absence of
fluorescence
quenching
the difference increased
the results
intensity
is
shown
fluorescence
can be
of Ca++-bound
CBC and
temperature.
The confor-
much more pronounced
at phy-
temperatures.
ACKXOWLEDGEMENTS. The authors like to thank shi for stimulating discussions. of us, JPvE, held a postdoctoral for the Promotion of Science.
professor F.Oosawa and Dr. K.MihaThis work was performed while one fellowship of the Japan Society
REFERENCES. 1. 2.
S.Ebashi and M.Endo, Progr.Biophys.Mol.Biol. D.J.Hartshorne and H.Mueller, B.B.R.C. 864
31,
18, 123, (1968). 647, (1968).
Vol. 47, No. 4, 1972
3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13.
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
T.Wakabayashi and F.Ebashi, J.Biochem. 69, 441, (1971) S.Ebashi, M.L.Greaser and J.Gergely, J.Biol.Chem. 246, 4226, (1971). M.L.Greaser and J.Gergely, Fed.Proc. 29, 463, (1970). A.Kodama and F.Ebashi, J.BiGhem. 64, 465, (1968). S.Ebashi, K.Weber and M.Osborn, J.Biol.Chem. 244, 4406,(1969). F.Perrin, J.Phys.Radium, 7, 390, (1926). N.Greenfield, B.Davidson and G.D.Fasman, Biochemistry, 5, 1630 (1967). G.Schwartsenbach, H.Senn and G.Anderegg, Helv.Chim.Acta, -'40 1886, (1957). O.H.Lowry, N.J.Rosebrough, A.L.Farr and R.J.Randall, J.Biol. Chem. 193, 265, (1951). D.J.Hartshorne and H.Y.Pyun, Biocim.Biophys.Acta, 2, 698, (1971). G.G.Vurek and N.Alexander, Science, 156, 949, (1967). R.F.Chen,
865
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
ca++ INDUCED CONFORMATIONAL CHANGES IN THE Ca++ BI"IJDING COMPONENT OF TROPONIN Jean-Paul van Eerd and Yukishige Kawasaki Institute of Molecular Biology and Department of Physics, Nagoya University, Nagoya, Japan 464.
Received April
17, 1972
The Ca++binding component of troponin undergoes reversible conformational changes in the presence or absence of micromolar amounts of Ca++. The presence of Ca++ causes an increase in the fluorescence intensity of the tyrosine residues as well as an The binding constant is 5.106M-1. increase of the helix content. Fluorescence polarisation shows that the motion of the tyrosine residues is much smaller in the presence than in the absence of Ca++. Thus the Ca++ binding component of troponin appears more rigid in the presence than in the absence of Ca++. Summary.
Muscle which
contraction
released
the nerve,
from the
bind
assumed that
troponin,
which
troponin. into
interest In three
(Greaser
Ca++. This usually
Phe/Tyr
component
conformation
induces
1972, by Academic
to myosin.
has been fractionated
only
substructure
et al. 3),
one of which identified
because of the
and 4 sub-
appears as it
absence
of
to bind
has an unof tryptophan
ratio5. whether
indeed
the conformation
on the presence
Ca++ induces
component. 859
Copyright 0
actin
and ulti-
troponin
3 (Ebashi
is
change in
in the
can be readily
(CBC) changes
of this
filaments
a conformational
of
of 1 . It
recently
and Mueller2),
to test
that
on excitation
on the thin
in the binding
ratio
amounts of Ca++,
a change in tropomyosin
laboratories
low E2So/E2b0
We have found
located
and Gergely4),
We set out ding
reticulum
has arisen
component
and the high
sarcoplasmic
resulting
2 (~Hartshorne
units
by small
Ca++ induces
in turn
in actin,
Accordingly
regulated
to troponin
generally
mately
is
Press, Inc.
of this
or absence
a striking
Ca++ binof Ca++.
change in the
Vol. 47, No. 4, 1972
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
MATERIALS AND METHODS. Preparation rabbit
of
skeletal
muscle
al. 6 . Troponin inability
in the
troponin
described
the
absence
and CBC. Troponin
according
was checked
to regulate
myosin from
troponin
for
to the
procedure
the absence
of
electrophoresis
in the presence
and showed very
little
in 6M ura as
CBC showed a single of sodium dodecyl
tryptophan
acto-
CBC was prepared
on DEAE Sephadex
and Gergely4.
et
by its
synthetic
of any added tropomyosin.
from
of Ebashi
of tropomyosin
superprecipitation
by chromatography
by Greaser
was prepared
fluorescence
band on gel
sulphate
(SDS)'
on excitation
at
290 nm. Ultraviolet with
absorption.
The UV spectrum
a Zeiss model PMQ 2 spectrophotometer. Fluorescence
cence
An Hitachi
spectroscopy.
spectrophotometer
was used for
was water-jacketed
Haake thermoregulator.
Tyrosine
after
always
rin's
less
and connected
fluorescence
a
at
306
than
at 276 nm. The OD value of the sample was 276 0.10. Polacoat ultraviolet polarising filters measuring
the degree
P, at
a number of temperatures
was used to change the viscosity Optical
Rotation
Dispersion
was a Jasco Autospectrometer ted from
with
was observed
of
fluorescence
The rotary molecular motion was calculated 8 equation , from observations of the degree of
polarisation cerol
measurements.
excitation
(105 UV) were used for risation.
model MPF-2A fluores-
fluorescence
The sample compartment
nm.,
of CBC was measured
the
[ml ;33 value was taken 9 .
specific of 14,700,
ca++ concentration.
at constant
measurements.
and for
at
+-I- concentrations Ca
860
Per-
fluorescence Gly-
temperature.
The apparatus content
233 nm. For
0% helix
using
and viscosities.
UV 5. The helix
rotations
pola-
was calcula-
100% helix
a [ml;33
used
value
a of
were adjusted
2200
using
BIOCHEMICAL
Vol. 47, No. 4, 1972
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
++ of Ca and 0.5 mM EGTA (ethylene
a Ca-buffer
tetraacetic
ethyl
ether)-N,N' 10 at pH 6.8 . Protein
acid)
bis
(n-amino-
in 10 mM cacodylate-HCl
concentration.
Protein 11 the method of Lowry .
mined using
glycol
concentrations
buffer
were deter-
.15-
d d
.I o-
.05-
I 260
I 260 WQVO
Figure
I 300 Length (n m )
1. Absorption spectrum of the Ca+' binding component of troponin. The protein concentration is 0.26 mg/ml in 0.3 mM NaHC03. The spectrum is identical in the presence and absence of Ca++.
RESULTS AND DISCUSSION. Ultraviolet gure
spectrum.
1. The maximum at
tyrosine
absorption.
The UV spectrum
275 nm. corresponds
The maxima at 259,
pond to maxima of the phenylalanine the
finestructure
served than
of the
because those
the molar
of tyrosine
phan is
present
structure
of
extinction
and the
tyrosine
intensity
In most proteins cannot
of phenylalanine
absorption and helix
861
is
low5,
easily
content.
be ob-
is much lower
In CBC however,
content
the
266 and 269 nm. corres-
absorption
and tryptophan.
shown in Fi-
to the maximum of
absorption.
phenylalanine
the phenylalanine
Fluorescence
of CBC is
no trypto-
so that
the
fine-
can be detected. The helix
content
Vol. 47, No. 4, 1972
BIOCHEMICAL
RESEARCH COMMUNICATIONS
content and change in fluorescence intensity 2. The helix of CBC versus Ca++ concentration at 250C. o-o ; helix content,AA; fluorescence intensity. Vertical bars represent possible errors due to line width. Protein concentrations are 0.45 and 0.12 mg/ml for the helix content and the fluorescence measurements respectively. The binding constant calculated from these curves is 5.106M-l.
Figure
and the
tyrosine
fluorescence
the Ca++ concentration distinct crease
AND BIOPHYSICAL
increase in the
The binding curves
is
5.4x106M-1 method.
intensity
are plotted
in helix
fluorescence
constant
for
5x106M-1 . This
of
CBC as a function
in Figure which
content,
2. There
is
paralleled
The increase
a very by an in-
intensity of the tyrosine residues. ++ estimated from these the Ca -CBC complex,
in good agreement with 12 by Hartshorne and Pyun using
obtained
is
of
is
in helix
content
and the
the value
of
the Chelex
increase
100
in fluores-
cence
intensity could be reversed by adding EGTA to bind any ex++ in fluorescence intensity could not have cess Ca . The increase been caused by aggregation
of CBC molecules
but
only
by an intra-
molecular
change because the UV spectrum was identical in the pre++ sence and absence of Ca . The conformational change in CBC occurs ++ concentrations in the micromolar range, i.e. at the phyat Ca siological
concentration
Fluorescence the
Perrin's
plot
where muscle
polarisation. a straight
With line
contraction changing
is regulated. temperature
in the presence
a62
shows
of Ca++ (see
Vol. 47, No. 4, 1972
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
7
a6 \
+-+++-h T/q
(OK / poise
)
Figure
3. The effect of temperature and viscosity on the fluorescence polarisation of CBC. o-o ; heating curve at pCa>8 a-0 ; heating curve at pCa=5.7.A-A; isothermal curve at 30°c and pCa>8.A-A ; isothermal curve at 30°C and bars represent the standard deviation pCa=5.7. Vertical of 3 observations. T is the absolute temperature and qis the viscosity of the solvent.
Figure
3).
straight
On the other
hand there
is a large
in the absence of Ca+*. This suggests ++ the tyrosine residues occupy sites of Ca
protein
molecule
the absence thermal
which allow only ++ of Ca , the tyrosine
activation
of motion
very
limited
residues
independent
the CBC molecule.
More accurate
tyrosine
residues
in CBC can be obtained
changing
viscosities
see Figure
of motion
is
at a constant 31, because
constant.
in that
For the
However,
overall
relaxation
times
fluorescence
thermal
of
of
plot
(isothermal
case the
in
motion
from a Perrin's
temperature
the
can undergo
of the
rotational
in the
within
motion.
easily
from a
that
line
presence
plot,
deviation
the with
Perrin's
activation
lifetimes
at 30°c we
used the values of 1.8 and 2.2 nsec in the absence and presence ++ These values were derived from a value of of Ca respectively. 2.6 nsec for at 23OC
the
fluorescence
13 and corrected
for
lifetime fluorescence
863
of
free
tyrosine
intensity
in water
changes
(Fi-
Vol. 47, No. 4, 1972
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Temperature
Figure
gure of
( “C
)
4. The temperature effect on the fluorescence intensity of CBC. o-o ; at pCa>8, m-o ; at pCa=5.7, e-8 ; the relabetween the tive difference in fluorescence intensity 2 conditions. Vertical bars represent possible errors due to line width. Using
4).
14.5
these
data
we obtained
a rotational
relaxation time ++ respecand absence of Ca
and 29.2 nsec in the presence
tively
at
30°C.
ture
variation
These values that
becomes rather
rigid
The temperature in Figure
4. Strong
observed,
while
Ca++ -free
CBC is
mational siological
support
CBC is
flexible
on the
addition
effect
on the
thermal
change in CBC is
in the of
with
of
therefore
tempera-
Ca++ and
Ca++.
the
in intensity raising
of the
absence of
fluorescence
quenching
the difference increased
the results
intensity
is
shown
fluorescence
can be
of Ca++-bound
CBC and
temperature.
The confor-
much more pronounced
at phy-
temperatures.
ACKXOWLEDGEMENTS. The authors like to thank shi for stimulating discussions. of us, JPvE, held a postdoctoral for the Promotion of Science.
professor F.Oosawa and Dr. K.MihaThis work was performed while one fellowship of the Japan Society
REFERENCES. 1. 2.
S.Ebashi and M.Endo, Progr.Biophys.Mol.Biol. D.J.Hartshorne and H.Mueller, B.B.R.C. 864
31,
18, 123, (1968). 647, (1968).
Vol. 47, No. 4, 1972
3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13.
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
T.Wakabayashi and F.Ebashi, J.Biochem. 69, 441, (1971) S.Ebashi, M.L.Greaser and J.Gergely, J.Biol.Chem. 246, 4226, (1971). M.L.Greaser and J.Gergely, Fed.Proc. 29, 463, (1970). A.Kodama and F.Ebashi, J.BiGhem. 64, 465, (1968). S.Ebashi, K.Weber and M.Osborn, J.Biol.Chem. 244, 4406,(1969). F.Perrin, J.Phys.Radium, 7, 390, (1926). N.Greenfield, B.Davidson and G.D.Fasman, Biochemistry, 5, 1630 (1967). G.Schwartsenbach, H.Senn and G.Anderegg, Helv.Chim.Acta, -'40 1886, (1957). O.H.Lowry, N.J.Rosebrough, A.L.Farr and R.J.Randall, J.Biol. Chem. 193, 265, (1951). D.J.Hartshorne and H.Y.Pyun, Biocim.Biophys.Acta, 2, 698, (1971). G.G.Vurek and N.Alexander, Science, 156, 949, (1967). R.F.Chen,
865