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Starvation results in decreased initiation factor activity in rat skeletal muscle
VoI. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
STARVATION RESULTS IN DECREASED INITIATION FACTOR ACTIVITY IN RAT SKELETAL MUSCLE BY D. Eugene Rannels, Anthony E. Pegg and Stephen R. Rannels Department of Physiology, The Milton S. Hershey Medical Center The Pennsylvania State University, Hershey, PennSylvania 17033
Received August27,1976 SUMMARY Activity of a factor forming a nitrocellulose filter-bound complex with [35S]met-tRNA~et and GTP was estimated in the postribosomal supernatant of psoas and heart muscle. Complex formation required initiator tRNA and GTP or GMP-P(CH2)P; it was inhibited by Mg 2+, GDP, aurintricarboxylic acid, spermine and spermidine. Starvation reduced complex-forming activity of supernatants from psoas but not heart muscle. Reduced activity was not due to increased dilution or deacylation of met-tRNA~ et or to increased hydrolysis of GTP by extracts from starved animals. INTRODUCTION
When rats were made alloxan-diabetic or starved for
48 hours, ribosomal subunits accumulated and polysomes were depleted in psoas muscle
(1,2).
No changes in ribosomal aggregation
were observed in hearts from these animals
(2).
Protein synthesis,
estimated in vitro, was inhibited in skeletal muscle from starved rats
(3).
These studies suggested that starvation restricted syn-
thesis of skeletal muscle proteins at the level of peptide-chain initiation. Reactions leading to formation of an initiation complex consisting of met-tRNA~ et and a 40S ribosomal subunit appeared to become rate limiting to protein synthesis in heme-deficient reticulocytes (4,5) and in the presence of low levels of double-stranded RNA or oxidized glutathione
(7).
(6)
Addition of the initiation factors
which mediate formation of this complex prevented or reversed these inhibitions
(8).
Formation of the complex may also be subject to
control by physiological factors such as substrate hormone
(Ii) availability or energy charge
Copyrtght© 1976 by A c a ~ m i c Press, Inc. All rights o] r~roduction in any [orm reserve.
1481
(12,13).
(9,10), and These ob-
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCHCOMMUNICATIONS
servations suggested the possible importance of initiation reactions as a site of regulation of protein synthesis. In ascites tumor cells, starvation for amino acids led to a loss of polysomes and a reduction in a met-tRNA~et-40S subunit complex,
the formation of which was mediated by an IF-E2-1ike
initiation factor
(9).
Thus, it appeared that the effects of
starvation on ribosomal aggregation in rat psoas could have been mediated by changes in activity of a similar factor.
This paper
describes formation of an initiation complex by post-ribosomal supernatants from heart and skeletal muscle of fed and starved rats. METHODS Heart or psoas muscle was removed from anesthetized rats, blotted, weighed and homogenized in a solution (2° ) containing 0.25 M KCI, 10 mM Tris, pH 7.4, and 3 ~ dithiothreitol. Following centrifugation of the homogenate for 70 minutes in a Beckman SW56 rotor (56,000 rpm), 50 ~i of the post-ribosomal supernatant was incubated (30 ° ) in a total volume of 300 ~i containing 90 mM KCI, 20 ~M Tris, pH 7.5, 3 r~4 dithiothreitol and 1.33 mM GTP ("complete" mixture) Reactions were started bv addition of a solution containing 4 pmoles of [35S]met-tRNA~ et (Specific Activity= 83.3 x 106 dpm/nmole). Reactions were stopped by addition of 5 ml of ice-cold buffer containing 90 ~M KCI, 20 mM Tris, pH 7.5, and 5 mM MgCI 2. This solution was poured over Millipore nitrocellulose filters (HAWP; pore size 0.45 ~m) which were then washed three times with 5 ml of the same cold buffer, dried, and counted in a toluene-based scintillator. Binding activity at 30 ° was too rapid for estimates of initial rates to be made. Values reported in this paper represent the steady state. When no supernatant was present, non-specific binding represented about 2% of that observed with the complete mixture. Rat liver tRNA, prepared by the method of Rogg et al. (14), was charged using E. Coli aminoacyl-tRNA synthetases, which charge only the initiator form of methionyl-tRNA (15). GTP and other nucleotides were estimated by high pressure liquid chromatography (16). Aminoacyl-tRNA synthetases were purchased from Miles Laboratories; [35S]-L-methionine from Amersham-Searle.
RESULTS AND DISCUSSION met-tRNA~ et to ~ l l i p o r e muscle
Activity of heart supernatants in binding filters was three times that from psoas
(Table I) when extracts were prepared in 0.25 M KCI.
In
separate experiments, muscles were homogenized in the presence of 0.25, 0.50, 0.75 and 1.00 M KCI.
1482
After centrifugation,
the
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE Characteristics of I n i t i a t o r
I
of S u p e r n a t a n t - d e p e n d e n t
Binding
tRNA to Filters.
[35S]met-tRNA~ et bound, CONDITION
OF
10 -3.
INCUBATION
EXPERIMENT
cpm/g m u s c l e
PSOAS
HEART
I
Complete
690
1316
-GTP
248
126
+GDP
270
384
88
64
602
708
273
ND
-GTP
29
ND
+ATA
6
ND
105
ND
-GTP + GDP -GTP + G M P - P ( C H 2 ) P
EXPERIMENT
II
Complete
+Bacterial
tRNA
H e a r t and psoas m u s c l e w e r e p r e p a r e d as d e s c r i b e d in methods. As indicated, GDP (1.33 mM), G M P - P ( C H 2 ) P (1.33 mM), a u r i n t r i c a r b o x y l i c acid, A T A (60 ~M), or a c y l a t e d b a c t e r i a l tRNA (0.5 mg) w e r e p r e s e n t from the start of incubation. A f t e r i0 (Experiment I) or 5 (Experiment II) m i n u t e s b i n d i n g was a s s a y e d as d e s c r i b e d in methods. ND = not determined.
post-ribosomal trifuged
supernatant
to r e m o v e
ing s u p e r n a t a n t prepared
over
was
was d i l u t e d
the a c t o m y o s i n unchanged
this range
to 0.25 M KCI and recen-
formed.
w h e n psoas
Activity or h e a r t
of KCI c o n c e n t r a t i o n s .
1483
of the r e s u l t
extracts Therefore,
were full
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Ioo
IOO
~ 6o ! ~ m
ff
4o
(z:
'
\\.,
20
i
[ P20i
~,sp~ ~
o.,
~
'l~Mg 2+
O--osp ]
I
0
I
I
j I
I
I
2 5 4 5 CONCENTRATION
| .
~;sp
ga+
,,o_osp I
I
0 I 2 5 4 ADDED, mM
I
I
I
5
Figure_!l. Effects of Magnesium or Polyamines on Binding of Met-tRNA~ et to Filters. Tissue preparation and binding assays were as described in methods. Psoas muscles were homogenized in 4 volumes of buffer; hearts, 5 volumes. Incubation time was i0 minutes; MgCI 2 (Mg2+), spermidine (Spd), or spermine (Sp) were added to the assay to give the concentration indicated. Under3~ontrol conditions (no additions), 6272 and 13,505 x 102 cpm [ S]met-tRNA met were bound per gram of psoas or heart, respectively, f
activity appeared to be released to the supernatant in the presence of 0.25 M KCI. In both tissues, binding activity required GTP and was inhibited by GDP.
Inhibition amounted to 60 to 70 percent when GTP
and GDP were present in equal-molar concentrations periment I).
(Table I, Ex-
The non-hydrolyzable GTP analog, GMP-P(CH2)P,
supported 55 to 85 percent of full activity.
Binding activity
in psoas supernatants was abolished by aurintricarboxylic acid (ATA), but not by a large excess of acylated b a c t e r i a l tRNA
(Table
I, Experiment II). Addition of increasing concentrations of MgCI 2, spermidine, or spermine to the incubation buffer reduced binding of tRNA~ et
(Figure i).
[35S]met-
Spermine and spermidine were both effective
at concentrations within the physiological range
1484
(17), with sper-
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE Effect
of S t a r v a t i o n
Supernatant
II
on F i l t e r
from Heart
Binding
or P s o a s
[35S]Met-tRNA~et
of M e t - t R N A ~ et by
Muscle.
BOUND
CONDITION OF A N I M A L
10 -3. c p m / g Muscle
TISSUE
EXPERIMENT
l0 -2- c p m / m g Protein
RNA mg/g Muscle
I Psoas
738 + 32
(5)
2 days
626 + 20
(5) a
3 days
570
+ 16
4 days
Fed
i14
+ 5
1.74
+
.07
(6)
98 + 3 a
1.34
+
.05
(7) b
(5) b
89 + 3b
1.30
+
.05
(7) b
511 + 21
(5) b
77 + 3 b
1.31
+
.05
(7) b
544 + 32
(6)
81 + 4 273 + 18
.05
(6)
.01
(7) b
Starved:
EXPERIMENT
II Psoas
Fed
ND
Heart
1508
+ 87
(3)
Psoas
419
+ 25
(6) a
51 + 5 b
Heart
1541
+ 196
(3)
255 + 32
2.50
+
Starved: 2 days
ND 2.26
+
Rats w e r e f a s t e d as i n d i c a t e d a n d b i n d i n g a c t i v i t y d e t e r m i n e d in s u p e r n a t a n t s f r o m h e a r t or p s o a s as d e s c r i b e d in m e t h o d s in 15 m i n u t e i n c u b a tions. R N A was e s t i m a t e d by a l k a l i n e h y d r o l y s i s as d e s c r i b e d p r e v i o u s l y (22). V a l u e s r e p r e s e n t the m e a n + S.E.M. of the n u m b e r of d e t e r m i n a t i o n s s h o w n in p a r e n t h e s i s . ND = not determined a = p< .05 vs f e d b = p< .01 vs fed
mine
being
about
twice
a molar
basis.
These
similar
to t h a t
of
as p o t e n t
as s p e r m i d i n e
experiments
IF-E 2
(18),
indicated
IF-I
1485
(19,20)
when
compared
on
t h a t an a c t i v i t y or I F - M P
(21), w h i c h
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
form a ternary initiation complex between factor,
initiator tRNA,
and GTP, could be estimated in the post ribosomal supernatant of psoas and heart muscle.
These factors have been reported to bind
to ribosomes and to be released by high salt concentrations. The data in Table II show that 48 hours of starvation reduced binding activity of psoas supernatants whether expressed per gram muscle or per mg supernatant protein
(Experiment I).
Activity of
psoas extracts declined as starvation continued while activity of heart supernatants was unchanged after two days
(Experiment II).
Psoas RNA content decreased after two days of starvation, but did not decline thereafter; a similar period.
heart RNA was reduced somewhat after
Details of the relationship between changes in
binding activity and content of specific RNA species remain to be investigated. Similar effects of starvation were observed when assays contained 5 mM MgCI 2.
Activity was greatly reduced under these con-
ditions, but the complex formed in the presence of Mg 2+ may be more directly related to the physiological precursor of the ribosomal initiation complex
(23).
Decreased activity in supernatants from psoas of starved rats did not appear to result from increased dilution of
[35S]met-tRNA~ et
by endogenous initiator tRNA or from accelerated rates of deacylation of substrate tRNA. fold range of
Binding activity was investigated over a 10-
[35S]met-tRNA~et concentration.
Activity was re-
duced in psoas of starved rats at all tRNA concentrations panel A).
(Figure 2,
As also shown in Figure 2 (panel B), addition of tissue
extracts from psoas of fed or fasted rats reduced the amount of [35S]met-tRNA met which remained acylated during i n c u b a ~ o n . However, f the rate of deacylation was similar with each tissue source. Walton and Gill
(12,13) recently suggested that activity of
1486
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCHCOMMUNICATIONS
E
I
=
,J°
,~ I00
E
"- 8 0
/"
/
/
FED
/
i Bo o
./
b_ 6c
I0 0 !
i • 60
~4c
•
40
,20 ¸
B
L
I
I
I
020
B0
;0
Met-tRNAf ADDED, prnoles
;
;
;
J0
INCUBATION TIME, rain
Figure 2. Effect of Availability of Met-tRNA~ et on Binding Activity in Supernatants from Fed and Starved Rats. In the experiments shown in panel A, binding activity was assayed in supernatant from psoas muscle of fed (closed symbols) or starved (48 hours, open symbols) rats, as described in methods. Assays were incubated 5 minutes. In a second experiment (panel B), samples were withdrawn at the times indicated. The fraction of met-tRNA~ et which remained acylated at each time was estimated by spo%ting the sample on filter paper discs and counting the washed discs in toluene containing 0.6% omnifluor (15). Radioactivity bound to the discs at each point was expressed as a fraction of that bound at zero time. Assays contained either no tissue extract (open squares), or extract from psoas muscle of fed (closed circles) or starved (48 hours, open cirlces) animals.
a ternary complex-forming factor, partially purified from reticulocytes,
could be modified by changes in the GTP:GDP ratio and thus
by the adenylate energy charge through the nucleotide diphosphate kinase reaction.
In the present experiments,
these factors did
not appear to account for inhibition of protein synthesis in psoas muscle in vivo.
Whole tissue levels of GDP, GTP, AMP, ADP, and
ATP were unaltered by 48-72 hours of starvation; charge
(24) also was unchanged
servations). vation,
Furthermore,
(D. E. Rannels,
adenylate energy
unpublished ob-
reduced binding activity during star-
as assayed in vitro,
did not appear to result from loss
of GTP or accumulation of GDP during incubation.
1487
Approximately
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCHCOMMUNICATIONS
TABLE E f f e c t of C r e a t i n e on A c t i v i t y
III
Phosphate
from Psoas
and C r e a t i n e
Phosphokinase
of F e d and S t a r v e d
Rats.
CONDITION
CP+
[ 3 5 S ] M e t - t R N A ~ et bound,
Nucleotide Concentration ~moles/ml GTP GDP
OF A N I M A L
CPK
10 -2.
Fed
-
(5) 45 ± 2
.99 ± .04
.27 ± .05
Starved
-
(5) 32 ± 2 a
.86 ± .06
.34 ± .03
Fed
+
(5) 67 ± 2 b
1.09
± .07
.14 ± .03 c
Starved
+
(5) 45 ± i a'b
i.i0
± .03 b
.18 ± .04 c
cpm/mg protein
Rats were s t a r v e d for 96 hours and b i n d i n g a c t i v i t y of psoas extracts a s s a y e d in 5 m i n u t e i n c u b a t i o n s as d e s c r i b e d in methods. The c o n c e n t r a t i o n s of GTP and GDP in the assay m i x t u r e at zero time w e r e 1.16 ± .06 and 0.04 ± .01 ~ m o l e s / m l , r e s p e c t i v e l y . Creatine phosphate (CP) and c r e a t i n e p h o s p h o k i n a s e (CPK) w e r e a d d e d to the assay m i x t u r e at c o n c e n t r a t i o n s of 3.33 n ~ and 0.07 mg/ml, r e s p e c t i v e l y . Similar changes in n u c l e o t i d e c o n c e n t r a t i o n s w e r e o b t a i n e d f o l l o w i n g a 15 minute incubation. V a l u e s r e p r e s e n t the m e a n ± S.E.M. of the n u m b e r of d e t e r m i n a t i o n s s h o w n in p a r e n t h e s i s . a = p < .01 vs F e d b = p < .01 vs - (CP + CPK) c = p < .05 vs - (CP + CPK)
20% of the GTP i n i t i a l l y lyzed d u r i n g or s t a r v e d
a 5 minute
rats
phosphokinase
ferences
in b i n d i n g
from both
regenerated.
Reduced
maintained
of this
of s t a r v e d
mechanism
activity
rats.
IF-E2-1ike
Further
is m o d i f i e d
of the factor.
1488
and
b u t dif-
Activity
of
45% h i g h e r w h e n GTP was
for the i n h i b i t i o n
in s k e l e t a l m u s c l e
purification
(Table III).
from fed
phosphate
GTP in b o t h extracts,
remained
activity
supernatants
of c r e a t i n e
sources was a b o u t
at least in part,
by w h i c h
of psaos
Addition
activity
supernatants
in the assay m i x t u r e was h y d r o -
incubation
(Table III).
creatine
account,
present
factor may
of p r o t e i n definition
during
synthesis of the
starvation
requires
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCHCOMMUNICATIONS
ACKNOWLEDGEMENTS The authors are grateful to Dr. L. S. Jefferson and Dr. H. E. Morgan for their encouragement and financial support. This work was supported by grants HLI1534, AM15658 and CA18138 from the National Institutes of Health. REFERENCES i. 2. 3. 4. 5. 6. 7. 8. 9. i0. ii. 12. 13. 14. 15. 16. 17. 18. 19. 20. 21. 22. 23. 24.
Jefferson, L. S., Koehler, J. O. and Morgan, H. E. (1972) Proc. Nat. Acad. Sci. (U.S.) 69____C816-820. Rannels, D. E., Hjalmarson, and Morgan, H. E. (1974) Amer. J. Physiol., 226, 528-539. Rannels, S. R., Li, J. B. and Jefferson, L. S. (1976). Diabetes 25, Suppl. i, 333. Balkow, K., Mizuno, S., Fisher, J. M. and Rabinovitz, M. (1973) Biochem. Biophys. Acta., 324, 397-409. Legon, S., Jackson, R. J. and Hunt, T. (1973) Nature New Biol., 241, 150-152. Ehrenfeld, E. and Hunt, T. (1971) Proc. Nat. Acad. Sci. (U.S.), 68, 1075-1078. K-~sower, N.S., Vanderhoff, G. A. and Kosower, E. M. (1972) Biochim. Biophys. Acta., 272, 623-637. Beuzard, Y. and London, I. M. (1974) Proc. Nat. Acad. Sci., (U.S.) 71, 2863-2866. Pain, V. M. and Henshaw, E. C. (1975) Eur. J. Biochem., 57 335-342. Smith, K. E. and Henshaw, E. C. (1975) Biochemistry i_44, 10601067. Liang, T. and Liao, S. (1975) Proc. Nat. Acad. Sci. (U.S.) 72, 706-709. Walton, G. M. and Gill, G. N. (1975) Biochim. Biophys. Acta 390, 231-245. Walton, G. M. and Gill, G. N. (1976) Biochim. Biophys. Acta, 418, 195-203. Rogg, H., Wehrli, W. and Staehelin, M. (1969) Biochim. Biophys. Acta, 195, 13-15. Stanley, W. M., Jr. (1974) In: Methods in Enzymology, Vol. XXIX (L. Grossman and K. Moldave, eds.) pp. 530-546, Academic Press New York. Whitfield, C. F., and Morgan, H. E. (1973) Biochim. Biophys. Acta 307, 181-196. Raina, A., and J~nne, J. (1975) Medical Biology 5_33, 121-147. Schreier, M. H. and Staehelin, T. (1973) Nature New Biol., 242, 35-38. Dettman, G. L. and Stanley, W. M., Jr. (1973) Biochim. Biophys, Acta 299, 142-147. Gupta, N° K., Woodley, C. L., Chen, Y. C. and Bose, K. K. (1973) J. Biol. Chem. 248, 4500-4511. Safer, B., Anderson, W. F. and Merrick, W. C. (1975) J. Biol. Chem. 250, 9067-9075. Morgan, H. E., Jefferson, L. S., Wolpert, E. B. and Rannels, D. E. (1971) J. Biol. Chem. 246, 2163-2170. Gupta, N. K., Chatterjee, B., Chen, Y. C. and Majumdar, A. (1975) J. Biol. Chem. 250, 853-862. Atkinson, D. E. and Walton, G. M. (1967) J. Biol. Chem. 242, 3239-3241.
1489
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
STARVATION RESULTS IN DECREASED INITIATION FACTOR ACTIVITY IN RAT SKELETAL MUSCLE BY D. Eugene Rannels, Anthony E. Pegg and Stephen R. Rannels Department of Physiology, The Milton S. Hershey Medical Center The Pennsylvania State University, Hershey, PennSylvania 17033
Received August27,1976 SUMMARY Activity of a factor forming a nitrocellulose filter-bound complex with [35S]met-tRNA~et and GTP was estimated in the postribosomal supernatant of psoas and heart muscle. Complex formation required initiator tRNA and GTP or GMP-P(CH2)P; it was inhibited by Mg 2+, GDP, aurintricarboxylic acid, spermine and spermidine. Starvation reduced complex-forming activity of supernatants from psoas but not heart muscle. Reduced activity was not due to increased dilution or deacylation of met-tRNA~ et or to increased hydrolysis of GTP by extracts from starved animals. INTRODUCTION
When rats were made alloxan-diabetic or starved for
48 hours, ribosomal subunits accumulated and polysomes were depleted in psoas muscle
(1,2).
No changes in ribosomal aggregation
were observed in hearts from these animals
(2).
Protein synthesis,
estimated in vitro, was inhibited in skeletal muscle from starved rats
(3).
These studies suggested that starvation restricted syn-
thesis of skeletal muscle proteins at the level of peptide-chain initiation. Reactions leading to formation of an initiation complex consisting of met-tRNA~ et and a 40S ribosomal subunit appeared to become rate limiting to protein synthesis in heme-deficient reticulocytes (4,5) and in the presence of low levels of double-stranded RNA or oxidized glutathione
(7).
(6)
Addition of the initiation factors
which mediate formation of this complex prevented or reversed these inhibitions
(8).
Formation of the complex may also be subject to
control by physiological factors such as substrate hormone
(Ii) availability or energy charge
Copyrtght© 1976 by A c a ~ m i c Press, Inc. All rights o] r~roduction in any [orm reserve.
1481
(12,13).
(9,10), and These ob-
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCHCOMMUNICATIONS
servations suggested the possible importance of initiation reactions as a site of regulation of protein synthesis. In ascites tumor cells, starvation for amino acids led to a loss of polysomes and a reduction in a met-tRNA~et-40S subunit complex,
the formation of which was mediated by an IF-E2-1ike
initiation factor
(9).
Thus, it appeared that the effects of
starvation on ribosomal aggregation in rat psoas could have been mediated by changes in activity of a similar factor.
This paper
describes formation of an initiation complex by post-ribosomal supernatants from heart and skeletal muscle of fed and starved rats. METHODS Heart or psoas muscle was removed from anesthetized rats, blotted, weighed and homogenized in a solution (2° ) containing 0.25 M KCI, 10 mM Tris, pH 7.4, and 3 ~ dithiothreitol. Following centrifugation of the homogenate for 70 minutes in a Beckman SW56 rotor (56,000 rpm), 50 ~i of the post-ribosomal supernatant was incubated (30 ° ) in a total volume of 300 ~i containing 90 mM KCI, 20 ~M Tris, pH 7.5, 3 r~4 dithiothreitol and 1.33 mM GTP ("complete" mixture) Reactions were started bv addition of a solution containing 4 pmoles of [35S]met-tRNA~ et (Specific Activity= 83.3 x 106 dpm/nmole). Reactions were stopped by addition of 5 ml of ice-cold buffer containing 90 ~M KCI, 20 mM Tris, pH 7.5, and 5 mM MgCI 2. This solution was poured over Millipore nitrocellulose filters (HAWP; pore size 0.45 ~m) which were then washed three times with 5 ml of the same cold buffer, dried, and counted in a toluene-based scintillator. Binding activity at 30 ° was too rapid for estimates of initial rates to be made. Values reported in this paper represent the steady state. When no supernatant was present, non-specific binding represented about 2% of that observed with the complete mixture. Rat liver tRNA, prepared by the method of Rogg et al. (14), was charged using E. Coli aminoacyl-tRNA synthetases, which charge only the initiator form of methionyl-tRNA (15). GTP and other nucleotides were estimated by high pressure liquid chromatography (16). Aminoacyl-tRNA synthetases were purchased from Miles Laboratories; [35S]-L-methionine from Amersham-Searle.
RESULTS AND DISCUSSION met-tRNA~ et to ~ l l i p o r e muscle
Activity of heart supernatants in binding filters was three times that from psoas
(Table I) when extracts were prepared in 0.25 M KCI.
In
separate experiments, muscles were homogenized in the presence of 0.25, 0.50, 0.75 and 1.00 M KCI.
1482
After centrifugation,
the
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE Characteristics of I n i t i a t o r
I
of S u p e r n a t a n t - d e p e n d e n t
Binding
tRNA to Filters.
[35S]met-tRNA~ et bound, CONDITION
OF
10 -3.
INCUBATION
EXPERIMENT
cpm/g m u s c l e
PSOAS
HEART
I
Complete
690
1316
-GTP
248
126
+GDP
270
384
88
64
602
708
273
ND
-GTP
29
ND
+ATA
6
ND
105
ND
-GTP + GDP -GTP + G M P - P ( C H 2 ) P
EXPERIMENT
II
Complete
+Bacterial
tRNA
H e a r t and psoas m u s c l e w e r e p r e p a r e d as d e s c r i b e d in methods. As indicated, GDP (1.33 mM), G M P - P ( C H 2 ) P (1.33 mM), a u r i n t r i c a r b o x y l i c acid, A T A (60 ~M), or a c y l a t e d b a c t e r i a l tRNA (0.5 mg) w e r e p r e s e n t from the start of incubation. A f t e r i0 (Experiment I) or 5 (Experiment II) m i n u t e s b i n d i n g was a s s a y e d as d e s c r i b e d in methods. ND = not determined.
post-ribosomal trifuged
supernatant
to r e m o v e
ing s u p e r n a t a n t prepared
over
was
was d i l u t e d
the a c t o m y o s i n unchanged
this range
to 0.25 M KCI and recen-
formed.
w h e n psoas
Activity or h e a r t
of KCI c o n c e n t r a t i o n s .
1483
of the r e s u l t
extracts Therefore,
were full
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Ioo
IOO
~ 6o ! ~ m
ff
4o
(z:
'
\\.,
20
i
[ P20i
~,sp~ ~
o.,
~
'l~Mg 2+
O--osp ]
I
0
I
I
j I
I
I
2 5 4 5 CONCENTRATION
| .
~;sp
ga+
,,o_osp I
I
0 I 2 5 4 ADDED, mM
I
I
I
5
Figure_!l. Effects of Magnesium or Polyamines on Binding of Met-tRNA~ et to Filters. Tissue preparation and binding assays were as described in methods. Psoas muscles were homogenized in 4 volumes of buffer; hearts, 5 volumes. Incubation time was i0 minutes; MgCI 2 (Mg2+), spermidine (Spd), or spermine (Sp) were added to the assay to give the concentration indicated. Under3~ontrol conditions (no additions), 6272 and 13,505 x 102 cpm [ S]met-tRNA met were bound per gram of psoas or heart, respectively, f
activity appeared to be released to the supernatant in the presence of 0.25 M KCI. In both tissues, binding activity required GTP and was inhibited by GDP.
Inhibition amounted to 60 to 70 percent when GTP
and GDP were present in equal-molar concentrations periment I).
(Table I, Ex-
The non-hydrolyzable GTP analog, GMP-P(CH2)P,
supported 55 to 85 percent of full activity.
Binding activity
in psoas supernatants was abolished by aurintricarboxylic acid (ATA), but not by a large excess of acylated b a c t e r i a l tRNA
(Table
I, Experiment II). Addition of increasing concentrations of MgCI 2, spermidine, or spermine to the incubation buffer reduced binding of tRNA~ et
(Figure i).
[35S]met-
Spermine and spermidine were both effective
at concentrations within the physiological range
1484
(17), with sper-
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE Effect
of S t a r v a t i o n
Supernatant
II
on F i l t e r
from Heart
Binding
or P s o a s
[35S]Met-tRNA~et
of M e t - t R N A ~ et by
Muscle.
BOUND
CONDITION OF A N I M A L
10 -3. c p m / g Muscle
TISSUE
EXPERIMENT
l0 -2- c p m / m g Protein
RNA mg/g Muscle
I Psoas
738 + 32
(5)
2 days
626 + 20
(5) a
3 days
570
+ 16
4 days
Fed
i14
+ 5
1.74
+
.07
(6)
98 + 3 a
1.34
+
.05
(7) b
(5) b
89 + 3b
1.30
+
.05
(7) b
511 + 21
(5) b
77 + 3 b
1.31
+
.05
(7) b
544 + 32
(6)
81 + 4 273 + 18
.05
(6)
.01
(7) b
Starved:
EXPERIMENT
II Psoas
Fed
ND
Heart
1508
+ 87
(3)
Psoas
419
+ 25
(6) a
51 + 5 b
Heart
1541
+ 196
(3)
255 + 32
2.50
+
Starved: 2 days
ND 2.26
+
Rats w e r e f a s t e d as i n d i c a t e d a n d b i n d i n g a c t i v i t y d e t e r m i n e d in s u p e r n a t a n t s f r o m h e a r t or p s o a s as d e s c r i b e d in m e t h o d s in 15 m i n u t e i n c u b a tions. R N A was e s t i m a t e d by a l k a l i n e h y d r o l y s i s as d e s c r i b e d p r e v i o u s l y (22). V a l u e s r e p r e s e n t the m e a n + S.E.M. of the n u m b e r of d e t e r m i n a t i o n s s h o w n in p a r e n t h e s i s . ND = not determined a = p< .05 vs f e d b = p< .01 vs fed
mine
being
about
twice
a molar
basis.
These
similar
to t h a t
of
as p o t e n t
as s p e r m i d i n e
experiments
IF-E 2
(18),
indicated
IF-I
1485
(19,20)
when
compared
on
t h a t an a c t i v i t y or I F - M P
(21), w h i c h
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
form a ternary initiation complex between factor,
initiator tRNA,
and GTP, could be estimated in the post ribosomal supernatant of psoas and heart muscle.
These factors have been reported to bind
to ribosomes and to be released by high salt concentrations. The data in Table II show that 48 hours of starvation reduced binding activity of psoas supernatants whether expressed per gram muscle or per mg supernatant protein
(Experiment I).
Activity of
psoas extracts declined as starvation continued while activity of heart supernatants was unchanged after two days
(Experiment II).
Psoas RNA content decreased after two days of starvation, but did not decline thereafter; a similar period.
heart RNA was reduced somewhat after
Details of the relationship between changes in
binding activity and content of specific RNA species remain to be investigated. Similar effects of starvation were observed when assays contained 5 mM MgCI 2.
Activity was greatly reduced under these con-
ditions, but the complex formed in the presence of Mg 2+ may be more directly related to the physiological precursor of the ribosomal initiation complex
(23).
Decreased activity in supernatants from psoas of starved rats did not appear to result from increased dilution of
[35S]met-tRNA~ et
by endogenous initiator tRNA or from accelerated rates of deacylation of substrate tRNA. fold range of
Binding activity was investigated over a 10-
[35S]met-tRNA~et concentration.
Activity was re-
duced in psoas of starved rats at all tRNA concentrations panel A).
(Figure 2,
As also shown in Figure 2 (panel B), addition of tissue
extracts from psoas of fed or fasted rats reduced the amount of [35S]met-tRNA met which remained acylated during i n c u b a ~ o n . However, f the rate of deacylation was similar with each tissue source. Walton and Gill
(12,13) recently suggested that activity of
1486
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCHCOMMUNICATIONS
E
I
=
,J°
,~ I00
E
"- 8 0
/"
/
/
FED
/
i Bo o
./
b_ 6c
I0 0 !
i • 60
~4c
•
40
,20 ¸
B
L
I
I
I
020
B0
;0
Met-tRNAf ADDED, prnoles
;
;
;
J0
INCUBATION TIME, rain
Figure 2. Effect of Availability of Met-tRNA~ et on Binding Activity in Supernatants from Fed and Starved Rats. In the experiments shown in panel A, binding activity was assayed in supernatant from psoas muscle of fed (closed symbols) or starved (48 hours, open symbols) rats, as described in methods. Assays were incubated 5 minutes. In a second experiment (panel B), samples were withdrawn at the times indicated. The fraction of met-tRNA~ et which remained acylated at each time was estimated by spo%ting the sample on filter paper discs and counting the washed discs in toluene containing 0.6% omnifluor (15). Radioactivity bound to the discs at each point was expressed as a fraction of that bound at zero time. Assays contained either no tissue extract (open squares), or extract from psoas muscle of fed (closed circles) or starved (48 hours, open cirlces) animals.
a ternary complex-forming factor, partially purified from reticulocytes,
could be modified by changes in the GTP:GDP ratio and thus
by the adenylate energy charge through the nucleotide diphosphate kinase reaction.
In the present experiments,
these factors did
not appear to account for inhibition of protein synthesis in psoas muscle in vivo.
Whole tissue levels of GDP, GTP, AMP, ADP, and
ATP were unaltered by 48-72 hours of starvation; charge
(24) also was unchanged
servations). vation,
Furthermore,
(D. E. Rannels,
adenylate energy
unpublished ob-
reduced binding activity during star-
as assayed in vitro,
did not appear to result from loss
of GTP or accumulation of GDP during incubation.
1487
Approximately
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCHCOMMUNICATIONS
TABLE E f f e c t of C r e a t i n e on A c t i v i t y
III
Phosphate
from Psoas
and C r e a t i n e
Phosphokinase
of F e d and S t a r v e d
Rats.
CONDITION
CP+
[ 3 5 S ] M e t - t R N A ~ et bound,
Nucleotide Concentration ~moles/ml GTP GDP
OF A N I M A L
CPK
10 -2.
Fed
-
(5) 45 ± 2
.99 ± .04
.27 ± .05
Starved
-
(5) 32 ± 2 a
.86 ± .06
.34 ± .03
Fed
+
(5) 67 ± 2 b
1.09
± .07
.14 ± .03 c
Starved
+
(5) 45 ± i a'b
i.i0
± .03 b
.18 ± .04 c
cpm/mg protein
Rats were s t a r v e d for 96 hours and b i n d i n g a c t i v i t y of psoas extracts a s s a y e d in 5 m i n u t e i n c u b a t i o n s as d e s c r i b e d in methods. The c o n c e n t r a t i o n s of GTP and GDP in the assay m i x t u r e at zero time w e r e 1.16 ± .06 and 0.04 ± .01 ~ m o l e s / m l , r e s p e c t i v e l y . Creatine phosphate (CP) and c r e a t i n e p h o s p h o k i n a s e (CPK) w e r e a d d e d to the assay m i x t u r e at c o n c e n t r a t i o n s of 3.33 n ~ and 0.07 mg/ml, r e s p e c t i v e l y . Similar changes in n u c l e o t i d e c o n c e n t r a t i o n s w e r e o b t a i n e d f o l l o w i n g a 15 minute incubation. V a l u e s r e p r e s e n t the m e a n ± S.E.M. of the n u m b e r of d e t e r m i n a t i o n s s h o w n in p a r e n t h e s i s . a = p < .01 vs F e d b = p < .01 vs - (CP + CPK) c = p < .05 vs - (CP + CPK)
20% of the GTP i n i t i a l l y lyzed d u r i n g or s t a r v e d
a 5 minute
rats
phosphokinase
ferences
in b i n d i n g
from both
regenerated.
Reduced
maintained
of this
of s t a r v e d
mechanism
activity
rats.
IF-E2-1ike
Further
is m o d i f i e d
of the factor.
1488
and
b u t dif-
Activity
of
45% h i g h e r w h e n GTP was
for the i n h i b i t i o n
in s k e l e t a l m u s c l e
purification
(Table III).
from fed
phosphate
GTP in b o t h extracts,
remained
activity
supernatants
of c r e a t i n e
sources was a b o u t
at least in part,
by w h i c h
of psaos
Addition
activity
supernatants
in the assay m i x t u r e was h y d r o -
incubation
(Table III).
creatine
account,
present
factor may
of p r o t e i n definition
during
synthesis of the
starvation
requires
Vol. 72, No. 4, 1976
BIOCHEMICAL AND BIOPHYSICAL RESEARCHCOMMUNICATIONS
ACKNOWLEDGEMENTS The authors are grateful to Dr. L. S. Jefferson and Dr. H. E. Morgan for their encouragement and financial support. This work was supported by grants HLI1534, AM15658 and CA18138 from the National Institutes of Health. REFERENCES i. 2. 3. 4. 5. 6. 7. 8. 9. i0. ii. 12. 13. 14. 15. 16. 17. 18. 19. 20. 21. 22. 23. 24.
Jefferson, L. S., Koehler, J. O. and Morgan, H. E. (1972) Proc. Nat. Acad. Sci. (U.S.) 69____C816-820. Rannels, D. E., Hjalmarson, and Morgan, H. E. (1974) Amer. J. Physiol., 226, 528-539. Rannels, S. R., Li, J. B. and Jefferson, L. S. (1976). Diabetes 25, Suppl. i, 333. Balkow, K., Mizuno, S., Fisher, J. M. and Rabinovitz, M. (1973) Biochem. Biophys. Acta., 324, 397-409. Legon, S., Jackson, R. J. and Hunt, T. (1973) Nature New Biol., 241, 150-152. Ehrenfeld, E. and Hunt, T. (1971) Proc. Nat. Acad. Sci. (U.S.), 68, 1075-1078. K-~sower, N.S., Vanderhoff, G. A. and Kosower, E. M. (1972) Biochim. Biophys. Acta., 272, 623-637. Beuzard, Y. and London, I. M. (1974) Proc. Nat. Acad. Sci., (U.S.) 71, 2863-2866. Pain, V. M. and Henshaw, E. C. (1975) Eur. J. Biochem., 57 335-342. Smith, K. E. and Henshaw, E. C. (1975) Biochemistry i_44, 10601067. Liang, T. and Liao, S. (1975) Proc. Nat. Acad. Sci. (U.S.) 72, 706-709. Walton, G. M. and Gill, G. N. (1975) Biochim. Biophys. Acta 390, 231-245. Walton, G. M. and Gill, G. N. (1976) Biochim. Biophys. Acta, 418, 195-203. Rogg, H., Wehrli, W. and Staehelin, M. (1969) Biochim. Biophys. Acta, 195, 13-15. Stanley, W. M., Jr. (1974) In: Methods in Enzymology, Vol. XXIX (L. Grossman and K. Moldave, eds.) pp. 530-546, Academic Press New York. Whitfield, C. F., and Morgan, H. E. (1973) Biochim. Biophys. Acta 307, 181-196. Raina, A., and J~nne, J. (1975) Medical Biology 5_33, 121-147. Schreier, M. H. and Staehelin, T. (1973) Nature New Biol., 242, 35-38. Dettman, G. L. and Stanley, W. M., Jr. (1973) Biochim. Biophys, Acta 299, 142-147. Gupta, N° K., Woodley, C. L., Chen, Y. C. and Bose, K. K. (1973) J. Biol. Chem. 248, 4500-4511. Safer, B., Anderson, W. F. and Merrick, W. C. (1975) J. Biol. Chem. 250, 9067-9075. Morgan, H. E., Jefferson, L. S., Wolpert, E. B. and Rannels, D. E. (1971) J. Biol. Chem. 246, 2163-2170. Gupta, N. K., Chatterjee, B., Chen, Y. C. and Majumdar, A. (1975) J. Biol. Chem. 250, 853-862. Atkinson, D. E. and Walton, G. M. (1967) J. Biol. Chem. 242, 3239-3241.
1489