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Isolation and recombination of bovine rod outer segment cGMP phosphodiesterase and its regulators
Vol.
92, No.
Jonuory
2, 1980
29,
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
Pages 505-510
1980
ISOLATION AND RECOMBINATION OF BOVINE ROD OUTER SEGMENT cGMP PHOSPHODIESTERASE AND ITS REGULATORS J. B. Hurleyl Department
of Physiology and Biophysics, University Urbana, Illinois 61801
October
Received
26,
of Illinois
1979
SUMMARY: cGMP phosphodiesterase extracted from rod outer segments can be activated by GTP in the presence of phospholipid vesicles containing I have separated the phosphodiesterase from a phosbleached rhodopsin. phodiesterase inhibitory protein and a GTPase also present in the crude extracts from rods. The GTPase can be activated by bleached rhodopsin. However, in the absence of the GTPase and inhibitor, the phosphodiesterase was not activated by GTP in the presence of bleached rhodopsin. Recombination with these proteins partially restored the activetion by GTP and bleached rhodopsin. Rod outer cular that
contain
several
a cGMP phosphodiesterase activation
light
cidated. which
the detailed
segment tried
and a GTPase.
step
here
to play
not
aware
the visual
the isolation
from
Recent
enzymes, evidence
transduction of this
process
and recombination role
by light
such a reconstitution
activated
by the bleaching
mechanism
an essential
phosphodeisterase
were
in
molecular
I report appear
light
of the phosphodiesterase
may be an important
However,
they
segments
in
(3). components
of the presence MATERIALS
isolated
suggests
of rhodopsin process
has not been
of bovine
et al. from
by
(1,Z).
of several
the regulation Shinozawa
in parti-
(4) frog
elu-
proteins rod
outer
have previously rods,
but
of the inhibitor. AND METHODS
cGMP, GIP, trypsin, trypsin inhibitor, and snake venom (Ophiophagus hannah) were obtained from Sigma Chemical Company; Cellex D(DEAEcellulose) from Bio-Rad Laboratories; Se hadex GZOO and Se harose 6B from Pharmacia Fine Chemicals. c3H) cGMP, ( 1E C) 5'GMP and (y- 33 P) GTP were purchased from Amersham Corporation; (r3*P) GTP was also purchased from New England Nuclear. Dodecyltrimethylammonium bromide was obtained from Eastman. Protein concentration was accomplished using a single hollow fiber concentrator obtained from Bio-Med Instruments, Chicago, Illinois. 1Present Building,
Address: Stanford
Department University
of Structural Biology; Sherman Fairchild School of Medicine, Stanford, California
94305.
0006-291X/80/020505-06801.00/0 SOS
Cop.vright 8 1980 b.v Academic Press, Inc. All rights of reproduction in any form reserved.
Vol.
92, No.
2, 1980
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
cGMP phosphodiesterase was assayed as described elsewhere (5). was assayed by measuring 32P release from (y-3*P) GTP using activated charcoal to isolate the free phosphate from nucleotides (6).
GTPase
Extraction of the rod outer segment phosphodiesterase and DEAE-cellulose chromatography were carried out as described elsewhere (6). Bovine retinae obtained from Hormel Co., Austin, Minn. were isolated by flotation on 42% sucrose, followed by a 15% sucrose wash. Phosphodiesterase was extracted by homogenization of the rods under dim red light in 10 mM Tris pH 8.0 and 1 mM dithiothreitol. The extract was applied to a 1.5 x 15 cm DEAE-cellulose column at 40 mM Tris pH 8.0, 1 mM MgC12 and 1 mM dithiothreitol. Inhibitor was eluted by washing with 40 mM Tris pH 8.0, 1 mM MgCl , 1 mM dithiothreitol and 100 mM NaCl. Phosphodiesterase and GTPase were t i en eluted together with a gradient from 100 mM to 500 mM NaCl. Rhodopsin solubilized in from rod outer segment were prepared (8). Vesicles (9) to purified rhodopsin in the detergent.
ified
dodecyltrimethylammonium bromide was pur(7) by conconavalin A affinity chromatography by adding purified egg phosphotidyl choline the ratio 1OO:l and dialyzing 4 days to remove RESULTS
As reported hibitor
elsewhere
is present
be separated
a trypsin
(3),
in extracts
from
from bovine
the phosphodiesterase
by DEAE-cellulose
chromatography.
phosphodiesterase
and GTPase from
and efficiently these
separated
proteins
described
could
by gel
column
was concentrated
G200 column. is
not
recovered
below.
off
this
better
than
of purified
phosphodiesterase
independent
and ranges
GTPase.
extracts free
I isolated
recombination
is
experiments,
the DEAE-cellulose
shown in Fig.
rather
from
column. preparations
was used
GTPase yields
506
to a Sephadex GTPase activity
1.
a Sepharose
phosphodiesterase
several
6B column
from
of 1 to 2 ml and applied
20 to 100 nmoles
column.
can
can be quickly
chromatography.
the Sepharose from
from
A Sepharose
from the DEAE-cellulose
but
was used for
resolution
which
inhibitor
column
so that
in-
out.
profile
column
segments
show that
phosphodiesterase
elution
The G200 column
provided
filtration
to a volume
A typical
outer
and the GTPase in the
procedures
Pooled
phosphodiesterase
the DEAE-cellulose
be carried
Phosphodiesterase.
rod
Here I first
by the following
below,
sensitive
cGMP/min to further appear
6B column;
isolation
because
The specific is
see
activity
concentration
mg. purify
the GTPase
to be significantly
it
Vol.
92, No.
BIOCHEMICAL
2, 1980
AND
BIOPHYSICAL
40
40
RESEARCH
COMMUNICATIONS
32-
16
24
32 FRACTION
Figure
1.
on agarose
I find
that
the
based
columns
the presence
than
on dextran
of 1 mM 5' GMP causes
enhancing
column,
Nevertheless,
the
separation
as can be seen in Fig.
phosphodiesterase
activity.
is
typically
The GTPase
fractions
Tris-Cl
at pH 8.0,
1 mM MgC12 and 1 mM dithiothreitol
On SDS polyacrylamide the phosphodiesterase
39,000
daltons
cellulose tively only
The major
3b).
column
(Fig.
appears
identified rhodopsin
bands 3~).
gels,
associated
with
as a monomer
major (3d). at 39,000
507
not
recovered
to elute
very
completely
late
with
free
about against
to remove
5'GMP.
protein
and 88,000
the GTPase appear inhibitor
50 mM
bands
of
daltons at 36,000
and
of the DEAE-
bands,
none of which
is
Purified
rhodopsin
vesicles
and as a dimer
of
20%
overnight
the major
at 84,000
The phosphodiesterase as several
the GTPase
and dialyzed
as a doublet
as the inhibitor both
pooled
electrophoresis
appear
In addition,
columns.
2, the GTPase is
GTPase were
based
of GTPase from phosphodiesterase.
yield.
(Fig.
64
Typical elution profile of the phosphodiesterase on the Sephadex G200 kolumn as described in the text. The column was 2.5 x 36 cm and was run at a flow rate of 5 ml/hr at 4°C with 50 mM Tris pH 8.0, 1 mM MgC12 1 mM dithiothreitol, and 100 PM phenylmethyl sulfonyl fluoride.' Approximately 3 ml fractions were collected. Blue dextran was used to make the void volume and DNP-glycine to mark the included volume.
higher
off
56
NUMBER
at 80,000
yet
posishow
daltons
(3a)
Vol.
92, No.
BIOCHEMICAL
2, 1980
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
t 20 FRACTION
Figure
2.
NUMBER
Typical elution profile of phosphodiesterase and GTPase off the Sepharose 6B column used to isolate GTPase for recombination The column was 2.5 x 38 cm experiments as described in the text. and was run at a flow rate of 7 ml/hr at 4°C with 40 mM Tris pH 8.0, 100 mM KU, 1 mM MgC12, 1 mM dithiothreitol, 100 uM phenylmethyl sulfonyl fluoride, and 1 ti 5' GMP. 3 ml fractions were collected. GTPase was assayed in the presence of bleached purified rhodopsin vesicles (5 ug rhodopsin).
~
88,000
84,000---
.
z
.-
80,00039,000
39,000-
36,OOOT
DYE FRONT-
0
Figure
3.
C
b
d
SDS polyacrylamide gel rlectrophoresis (10) of a) purified rhodopsin vesicles (-5 ug), b) gel filtration purified phosphodiesterase c) Sepharose 68 purified GTPasr (-30 ug), d) DEAE-cellulose (2 ug), 12.52 acrylamide: inhibitor (-50 ug). a), c), d) were run with b) with 10.5%.
508
Vol.
92, No.
2, 1980
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
Table 1. RECOMBINATION OF PURIFIED ROD OUTER SEGMENT cGMP PHOSPHODIESTERASE WITH ITS REGULATORS. -5 pg purified phosphodiesterase (PDE), -6 pg purified GTPase (27 pmoles GTP/min), and -30 ug DEAE-cellulose inhibitor were added where indicated. The numbers in parentheses are activities due to added PDE corrected for residual PDE activities in the isolated GTPase. __Phosphodiesterase activity (nmoles cGMP/min) Recombination Bleached Bleached Bleached Bleached Bleached Bleached
mixture rhodopsin rhadopsin rhodopsin rhodopsin rhodopsin rhodopsin
The agarose rhodopsin not
+ + + + + +
vesicles
However,
Sephadex
by
(Table
Addition
of inhibitor
rhodopsin
vesicles
absence
and presence
cluded
in
this
terase
activity
the presence
the
purified
carried
recombination the absence
and GTPase restores
However,
mixture,
the
rhodopsin
of bleached
does not
restore
the
the GTPase is
decreases
the combination
in-
phosphodies-
not when GTP is present.
vesicles
the GTP effect
experiments.
in both
when
is
sensitivity
activity
inhibitor
of GTP but
this
the presence
alone
GTP sensitivity.
of bleached
in
inhibitor
of bleached
purified
recombination
the phosphodiesterase
of GTP; i.e.,
31 19 3.8 74 (55) 59 (55)
bleached
to restore
out
~$1 GTP
phosphodiesterase
presenceof
to the phosphodiesterase
plus
in
in
100 I:!
in the presence
In an attempt
I have
decreases
rhodopsin
GTP
1).
to the phosphodiesterase,
bleached
activated
alone.
with
61 35 14 2.6 68 (54) 29 (26)
GTPase is
significantly
rhodopsin
GTP
PDE PDE + inhibitor GTPase GTPase + inhibitor GTPase + PDE GTPase + PDF + inhibitor
purified
vesicles
activated
w/o
Thus,
in
of inhibitor
on the phosphodiesterase. DISCUSSION
Hurley hibitor
et al.,
protein
from This
chromatography.
terase
and GTPase.
filtration
have
crude
extracts
procedure Here I report
chromatography.
the phosphodiesterase phodiesterase
(3,6)
regulation
recently
of bovine
allows that
Furthermore,
inhibitor
reported
isolation
segments
of inhibitor enzymes
I provide
and GTPase
by rhodopsin
rod
recovery these
the
play
and GTP.
of an in-
by DEAE-cellulose free
phosphodies-
can be separated
evidence an essential
suggesting role
by gel that
in phos-
Vol.
92, No.
2, 1980
BIOCHEMICAL
Isolated (3)
phosphodiesterase
on SDS polyacrylamide
at 36,000
and 39,000
phospholipid a molecular
weight
appears
gels.
This
containing
for
lation These the
activated during restored
phosphodiesterase results inhibitor
GTPase appears
GTPase fraction
here
by recombination
protein
maintains
basal
state.
Activation
tiich
in the presence
occurs
bands by assigned
rhodopsin with
on activation
rhodopsin
tht
phosphodiesterase
vesicles
phosphodiesterase
1) suggesting
The results
for
as two major
are based
of bleached
way (Table
GTP and bleached
a mechanism
doublet
I have not yet
Isolated
purification.
suggest
dalton
inhibitor.
the presence
in this
COMMUNICATIONS
can be activated
rhodopsin.
successfulrecombination.
proteins
I have partially
88,000
presented
by GTP in
significantly
regulatory
as an 84,000;
to the phosphodiesterase
of phosphodiesterase
is not
RESEARCH
bleached
The recombinationexperiments
as a criterion
BIOPHYSICAL
Isolated
daltons.
vesicles
AND
in Table activation
the loss 1 show that
to the iso-
GTPase and inhibitor. regulation
in which
the phosphodiesterase
at low activity
by bleached
activating
of GTP, counteracts
rhodopsin the effects
of
in the
the GTPase,
of the inhibitor
on the
phosphodiesterase. ACKNOWLEDGEMENT I thank advice. This fellowship.
Prof. Thomas Ebrev for his support, encouragement, and work was supported by NIH EY01323 and a NIH NRSA predoctoral
REFERENCES 1. 2. 3. 4. 5. 6. 7. 8. 9. 10.
Hubbell, W.L. and Bownds, M.D. (1979) Ann. Rev. Neurosci. 2, 17-34. Keirns, J.J., Miki, N., Bitensky, M.W. and Keirns, M. (1975) Biochemistry 14, 2760-66. Hurley, J.B. and Ebrey, T.G. (1978) Biophys. J. 2, 314a. I ., Wheeler, G., and Bitensky, M. (1979) J. Supramol. %,;Zo,zawa, . lo, T&%F? Thompson, W. and Appleman, N. (1971) Biochemistry lo, 311-316. for publication. Hurley, J., Barry, B., and Ebrey, T. (1979) submitted Papermaster, D. and Dreyer W. (1979) Biochemistry 13, 2438-2444. van Breugel, P., Daemen, F., and Bonting, S. (1977) Exp. Eye Res.4, 581-585. Singleton, W., Gray, M., Brown, M., and White, J. (1965) J. Oil Chem. 42, 53-56. Laemmli, V. (1970) Nature 227, 680-685.
510
92, No.
Jonuory
2, 1980
29,
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
Pages 505-510
1980
ISOLATION AND RECOMBINATION OF BOVINE ROD OUTER SEGMENT cGMP PHOSPHODIESTERASE AND ITS REGULATORS J. B. Hurleyl Department
of Physiology and Biophysics, University Urbana, Illinois 61801
October
Received
26,
of Illinois
1979
SUMMARY: cGMP phosphodiesterase extracted from rod outer segments can be activated by GTP in the presence of phospholipid vesicles containing I have separated the phosphodiesterase from a phosbleached rhodopsin. phodiesterase inhibitory protein and a GTPase also present in the crude extracts from rods. The GTPase can be activated by bleached rhodopsin. However, in the absence of the GTPase and inhibitor, the phosphodiesterase was not activated by GTP in the presence of bleached rhodopsin. Recombination with these proteins partially restored the activetion by GTP and bleached rhodopsin. Rod outer cular that
contain
several
a cGMP phosphodiesterase activation
light
cidated. which
the detailed
segment tried
and a GTPase.
step
here
to play
not
aware
the visual
the isolation
from
Recent
enzymes, evidence
transduction of this
process
and recombination role
by light
such a reconstitution
activated
by the bleaching
mechanism
an essential
phosphodeisterase
were
in
molecular
I report appear
light
of the phosphodiesterase
may be an important
However,
they
segments
in
(3). components
of the presence MATERIALS
isolated
suggests
of rhodopsin process
has not been
of bovine
et al. from
by
(1,Z).
of several
the regulation Shinozawa
in parti-
(4) frog
elu-
proteins rod
outer
have previously rods,
but
of the inhibitor. AND METHODS
cGMP, GIP, trypsin, trypsin inhibitor, and snake venom (Ophiophagus hannah) were obtained from Sigma Chemical Company; Cellex D(DEAEcellulose) from Bio-Rad Laboratories; Se hadex GZOO and Se harose 6B from Pharmacia Fine Chemicals. c3H) cGMP, ( 1E C) 5'GMP and (y- 33 P) GTP were purchased from Amersham Corporation; (r3*P) GTP was also purchased from New England Nuclear. Dodecyltrimethylammonium bromide was obtained from Eastman. Protein concentration was accomplished using a single hollow fiber concentrator obtained from Bio-Med Instruments, Chicago, Illinois. 1Present Building,
Address: Stanford
Department University
of Structural Biology; Sherman Fairchild School of Medicine, Stanford, California
94305.
0006-291X/80/020505-06801.00/0 SOS
Cop.vright 8 1980 b.v Academic Press, Inc. All rights of reproduction in any form reserved.
Vol.
92, No.
2, 1980
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
cGMP phosphodiesterase was assayed as described elsewhere (5). was assayed by measuring 32P release from (y-3*P) GTP using activated charcoal to isolate the free phosphate from nucleotides (6).
GTPase
Extraction of the rod outer segment phosphodiesterase and DEAE-cellulose chromatography were carried out as described elsewhere (6). Bovine retinae obtained from Hormel Co., Austin, Minn. were isolated by flotation on 42% sucrose, followed by a 15% sucrose wash. Phosphodiesterase was extracted by homogenization of the rods under dim red light in 10 mM Tris pH 8.0 and 1 mM dithiothreitol. The extract was applied to a 1.5 x 15 cm DEAE-cellulose column at 40 mM Tris pH 8.0, 1 mM MgC12 and 1 mM dithiothreitol. Inhibitor was eluted by washing with 40 mM Tris pH 8.0, 1 mM MgCl , 1 mM dithiothreitol and 100 mM NaCl. Phosphodiesterase and GTPase were t i en eluted together with a gradient from 100 mM to 500 mM NaCl. Rhodopsin solubilized in from rod outer segment were prepared (8). Vesicles (9) to purified rhodopsin in the detergent.
ified
dodecyltrimethylammonium bromide was pur(7) by conconavalin A affinity chromatography by adding purified egg phosphotidyl choline the ratio 1OO:l and dialyzing 4 days to remove RESULTS
As reported hibitor
elsewhere
is present
be separated
a trypsin
(3),
in extracts
from
from bovine
the phosphodiesterase
by DEAE-cellulose
chromatography.
phosphodiesterase
and GTPase from
and efficiently these
separated
proteins
described
could
by gel
column
was concentrated
G200 column. is
not
recovered
below.
off
this
better
than
of purified
phosphodiesterase
independent
and ranges
GTPase.
extracts free
I isolated
recombination
is
experiments,
the DEAE-cellulose
shown in Fig.
rather
from
column. preparations
was used
GTPase yields
506
to a Sephadex GTPase activity
1.
a Sepharose
phosphodiesterase
several
6B column
from
of 1 to 2 ml and applied
20 to 100 nmoles
column.
can
can be quickly
chromatography.
the Sepharose from
from
A Sepharose
from the DEAE-cellulose
but
was used for
resolution
which
inhibitor
column
so that
in-
out.
profile
column
segments
show that
phosphodiesterase
elution
The G200 column
provided
filtration
to a volume
A typical
outer
and the GTPase in the
procedures
Pooled
phosphodiesterase
the DEAE-cellulose
be carried
Phosphodiesterase.
rod
Here I first
by the following
below,
sensitive
cGMP/min to further appear
6B column;
isolation
because
The specific is
see
activity
concentration
mg. purify
the GTPase
to be significantly
it
Vol.
92, No.
BIOCHEMICAL
2, 1980
AND
BIOPHYSICAL
40
40
RESEARCH
COMMUNICATIONS
32-
16
24
32 FRACTION
Figure
1.
on agarose
I find
that
the
based
columns
the presence
than
on dextran
of 1 mM 5' GMP causes
enhancing
column,
Nevertheless,
the
separation
as can be seen in Fig.
phosphodiesterase
activity.
is
typically
The GTPase
fractions
Tris-Cl
at pH 8.0,
1 mM MgC12 and 1 mM dithiothreitol
On SDS polyacrylamide the phosphodiesterase
39,000
daltons
cellulose tively only
The major
3b).
column
(Fig.
appears
identified rhodopsin
bands 3~).
gels,
associated
with
as a monomer
major (3d). at 39,000
507
not
recovered
to elute
very
completely
late
with
free
about against
to remove
5'GMP.
protein
and 88,000
the GTPase appear inhibitor
50 mM
bands
of
daltons at 36,000
and
of the DEAE-
bands,
none of which
is
Purified
rhodopsin
vesicles
and as a dimer
of
20%
overnight
the major
at 84,000
The phosphodiesterase as several
the GTPase
and dialyzed
as a doublet
as the inhibitor both
pooled
electrophoresis
appear
In addition,
columns.
2, the GTPase is
GTPase were
based
of GTPase from phosphodiesterase.
yield.
(Fig.
64
Typical elution profile of the phosphodiesterase on the Sephadex G200 kolumn as described in the text. The column was 2.5 x 36 cm and was run at a flow rate of 5 ml/hr at 4°C with 50 mM Tris pH 8.0, 1 mM MgC12 1 mM dithiothreitol, and 100 PM phenylmethyl sulfonyl fluoride.' Approximately 3 ml fractions were collected. Blue dextran was used to make the void volume and DNP-glycine to mark the included volume.
higher
off
56
NUMBER
at 80,000
yet
posishow
daltons
(3a)
Vol.
92, No.
BIOCHEMICAL
2, 1980
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
t 20 FRACTION
Figure
2.
NUMBER
Typical elution profile of phosphodiesterase and GTPase off the Sepharose 6B column used to isolate GTPase for recombination The column was 2.5 x 38 cm experiments as described in the text. and was run at a flow rate of 7 ml/hr at 4°C with 40 mM Tris pH 8.0, 100 mM KU, 1 mM MgC12, 1 mM dithiothreitol, 100 uM phenylmethyl sulfonyl fluoride, and 1 ti 5' GMP. 3 ml fractions were collected. GTPase was assayed in the presence of bleached purified rhodopsin vesicles (5 ug rhodopsin).
~
88,000
84,000---
.
z
.-
80,00039,000
39,000-
36,OOOT
DYE FRONT-
0
Figure
3.
C
b
d
SDS polyacrylamide gel rlectrophoresis (10) of a) purified rhodopsin vesicles (-5 ug), b) gel filtration purified phosphodiesterase c) Sepharose 68 purified GTPasr (-30 ug), d) DEAE-cellulose (2 ug), 12.52 acrylamide: inhibitor (-50 ug). a), c), d) were run with b) with 10.5%.
508
Vol.
92, No.
2, 1980
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
Table 1. RECOMBINATION OF PURIFIED ROD OUTER SEGMENT cGMP PHOSPHODIESTERASE WITH ITS REGULATORS. -5 pg purified phosphodiesterase (PDE), -6 pg purified GTPase (27 pmoles GTP/min), and -30 ug DEAE-cellulose inhibitor were added where indicated. The numbers in parentheses are activities due to added PDE corrected for residual PDE activities in the isolated GTPase. __Phosphodiesterase activity (nmoles cGMP/min) Recombination Bleached Bleached Bleached Bleached Bleached Bleached
mixture rhodopsin rhadopsin rhodopsin rhodopsin rhodopsin rhodopsin
The agarose rhodopsin not
+ + + + + +
vesicles
However,
Sephadex
by
(Table
Addition
of inhibitor
rhodopsin
vesicles
absence
and presence
cluded
in
this
terase
activity
the presence
the
purified
carried
recombination the absence
and GTPase restores
However,
mixture,
the
rhodopsin
of bleached
does not
restore
the
the GTPase is
decreases
the combination
in-
phosphodies-
not when GTP is present.
vesicles
the GTP effect
experiments.
in both
when
is
sensitivity
activity
inhibitor
of GTP but
this
the presence
alone
GTP sensitivity.
of bleached
in
inhibitor
of bleached
purified
recombination
the phosphodiesterase
of GTP; i.e.,
31 19 3.8 74 (55) 59 (55)
bleached
to restore
out
~$1 GTP
phosphodiesterase
presenceof
to the phosphodiesterase
plus
in
in
100 I:!
in the presence
In an attempt
I have
decreases
rhodopsin
GTP
1).
to the phosphodiesterase,
bleached
activated
alone.
with
61 35 14 2.6 68 (54) 29 (26)
GTPase is
significantly
rhodopsin
GTP
PDE PDE + inhibitor GTPase GTPase + inhibitor GTPase + PDE GTPase + PDF + inhibitor
purified
vesicles
activated
w/o
Thus,
in
of inhibitor
on the phosphodiesterase. DISCUSSION
Hurley hibitor
et al.,
protein
from This
chromatography.
terase
and GTPase.
filtration
have
crude
extracts
procedure Here I report
chromatography.
the phosphodiesterase phodiesterase
(3,6)
regulation
recently
of bovine
allows that
Furthermore,
inhibitor
reported
isolation
segments
of inhibitor enzymes
I provide
and GTPase
by rhodopsin
rod
recovery these
the
play
and GTP.
of an in-
by DEAE-cellulose free
phosphodies-
can be separated
evidence an essential
suggesting role
by gel that
in phos-
Vol.
92, No.
2, 1980
BIOCHEMICAL
Isolated (3)
phosphodiesterase
on SDS polyacrylamide
at 36,000
and 39,000
phospholipid a molecular
weight
appears
gels.
This
containing
for
lation These the
activated during restored
phosphodiesterase results inhibitor
GTPase appears
GTPase fraction
here
by recombination
protein
maintains
basal
state.
Activation
tiich
in the presence
occurs
bands by assigned
rhodopsin with
on activation
rhodopsin
tht
phosphodiesterase
vesicles
phosphodiesterase
1) suggesting
The results
for
as two major
are based
of bleached
way (Table
GTP and bleached
a mechanism
doublet
I have not yet
Isolated
purification.
suggest
dalton
inhibitor.
the presence
in this
COMMUNICATIONS
can be activated
rhodopsin.
successfulrecombination.
proteins
I have partially
88,000
presented
by GTP in
significantly
regulatory
as an 84,000;
to the phosphodiesterase
of phosphodiesterase
is not
RESEARCH
bleached
The recombinationexperiments
as a criterion
BIOPHYSICAL
Isolated
daltons.
vesicles
AND
in Table activation
the loss 1 show that
to the iso-
GTPase and inhibitor. regulation
in which
the phosphodiesterase
at low activity
by bleached
activating
of GTP, counteracts
rhodopsin the effects
of
in the
the GTPase,
of the inhibitor
on the
phosphodiesterase. ACKNOWLEDGEMENT I thank advice. This fellowship.
Prof. Thomas Ebrev for his support, encouragement, and work was supported by NIH EY01323 and a NIH NRSA predoctoral
REFERENCES 1. 2. 3. 4. 5. 6. 7. 8. 9. 10.
Hubbell, W.L. and Bownds, M.D. (1979) Ann. Rev. Neurosci. 2, 17-34. Keirns, J.J., Miki, N., Bitensky, M.W. and Keirns, M. (1975) Biochemistry 14, 2760-66. Hurley, J.B. and Ebrey, T.G. (1978) Biophys. J. 2, 314a. I ., Wheeler, G., and Bitensky, M. (1979) J. Supramol. %,;Zo,zawa, . lo, T&%F? Thompson, W. and Appleman, N. (1971) Biochemistry lo, 311-316. for publication. Hurley, J., Barry, B., and Ebrey, T. (1979) submitted Papermaster, D. and Dreyer W. (1979) Biochemistry 13, 2438-2444. van Breugel, P., Daemen, F., and Bonting, S. (1977) Exp. Eye Res.4, 581-585. Singleton, W., Gray, M., Brown, M., and White, J. (1965) J. Oil Chem. 42, 53-56. Laemmli, V. (1970) Nature 227, 680-685.
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