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Inhibition of the peptidyl transferase A-site function by 2′-O-aminoacyloligonucleotides
Vol.56,No.3,
1974
BIOCHEMICAL
INHIBITION
AND BIOPHYSICAL
OF THE PEPTIDYL
RESEARCH COMMUNICATIONS
TRANSFERASE A-SITE
FUNCTION
BY 2’-O-AMINOACYLOLIGONUCLEOTIDES David Michigan
Received
December
Ringer
Cancer
and Stanislav
Foundation,
Chla/dek*
Detroit,
Michigan
48201
11,1973 SUMMARY
New "non-isomerizable" analogs of the 3'-terminus of AA-tRNA, C-A(2'Phe)H, C-A(P'Phe)Me, C-A(2'H)Phe and C-A(2'Me)Phe, were tested as acceptor substrates of ribosomal peptidyl transferase and inhibitors of the peptidyl transferase A-site function. The 3'-O-AA-derivatives were active acceptors of Ac-Phe in while the PI-O-AA-derivatives were completely the peptidyl transferase reaction, inactive. Both 2'- and 3'-O-AA-derivatives were potent inhibitors of peptidyl transferase catalyzed Ac-Phe transfer to puromycin. The results indicate that although peptidyl transferase exclusively utilizes 3'-O-esters of tRNA as acceptor substrates, its A-site can also recognize the 3'-terminus of 2'-OAA-tRNA. INTRODUCTION Since
the discovery
in protein
biosynthesis,
terminal
adenosine
Because the
of the
cis-diol
the
Moreover,
tRNA that
is
unit
the
employed
* To whom reprint 110 E. Warren Avenue,
direct
exact
involvement
location
has been the rapid
terminal
exact it
the
the
extremely
of
to determine tRNA.
of
2'
subject
z 3'
of
now appears
that
throughout
the
the
of
unit
the
of
(2,3),
aminoacyl it
is
various
requests should Detroit, Michigan
amfnoacyl
considerable
migration
adenosine
position
of
of 2'(3')-U-aminoacyl-tRNA
not
the it
is
residue a single
stages
be sent: 48201.
on the
interest
(1).
aminoacyl
group
almost
impossible
in native isomer
of protein Michigan
residue
of
of
aminoacylaminoacyl-
biosynthesis.
Cancer
Foundation,
Abbreviations: C-APhe, cytidyly1(3'-5')-2'(3')-O-L-phenylalanyladenosine (I); C-A(2'Phe)H, cytidyly1(3'-5')-3'-deoxy-2'-O-L-phenylalanyladenosine (IIa); C-A(2'Phe)Me, cytidyly1(3'-5')-3'-O-methyl-2'-u-~-phenylalanyladenosine (IIb); C-A(2'H)Phe, cytidyly1(3'-5')-2'-deoxy-3'-O-L-phenylalanyladenosine (IIIa); C-A(2'Me)Phe, cytidyly1(3'-5')-2'-&methyl-3'-O-L-phenylalanyladenosine (IIIb); tRNAox-red, tRNA w ich has been oxidized with periodate, reduced with borohydride (6); A#,;'" !4 , L-phenylalanyl derivative of oxidizedreduced adenosine, either "2"' or "3"' -isomer (for correct nomenclature of the latter, see ref. 5). 760
Vol.
56, No.
On the
3, 1974
basis
BIOCHEMICAL
of the
amtnoacyl-tRNA inhibiting
structure
and its
AND
and activity
2'-analog
polypeptide
BIOPHYSICAL
(the
synthesis),
of puromycin
latter
it
RESEARCH
COMMUNICATIONS
as a 3'-analog
was found
of
to be inactive
has been suggested
that
in
3'-O-aminoacyl-
C
HOCHz
0
1cs; 0 7 HO-P=0
0
OH
I HO-P=0
OH
OH
HO-P=0
I A
&HZ
6Cl-l~
A
0 w
ii
bPhe
PheO
R
v Phe.H
I
n
o;R=H
IItO,R=H
b,R=OCHa
tRNA is
the
active
we have
recently
analog
of
ferase
reaction
reported
is
3'-isomer
PI-isomer
is
formed
by the
(4).
acceptor
must occur
peptidyl
inactive (7)
have
synthetase after
a "non-isomerizable" in the
virtually
and Cramer
AA-tRNA
More specifically,
of AFi,red,
an active
and Sprinzl
transacylation
(5).
shown
reaction,
enzymic
transStudies
that
thus
2'-Oindicating
aminoacylation
and before
bond formation. As part
various
whether
several the
(ITb), substrates
of our stages
or not
ribosomal
at
biosynthesis
the is
its
and Chen (6)
2' + 3'
the
that
and that
aminoacyl-tRNA
peptide
in protein
3'-U-aminoacyl-tRNA,
by Ofengand
that
isomer
bj R=OCHa
study
of
of protein
a 2'
+ 3'
or 3'-hydroxyl.
C-A(2'H)Phe for
(IIIa) peptidyl
this
in which compounds,
and C-A(2'Me)Phe transferase
3'-terminus
is a required
to study
These
of the
we have been
transacylation
aminoacyloligonucleotides 2'-
involvement
biosynthesis,
In order
mechanism.
the
the
and as inhibitors
761
residue
(IIa),
C-A(2'Phe)H
(IIIb),
in the
we have
aminoacyl
were
tested of
tRNA in
interested
step
question,
of
peptidyl
to learn overall
synthesized is
"fixed"
C-A(2'Phe)Me as acceptor transferase
Vol.
56,
No.
3, 1974
catalyzed
BIOCHEMICAL
Ac-Phe
3'-0-aminoacyl
to
center,
of
both
peptidyl
aminoacyl-tRNA
BlOPHYSlCAi
puromycin.
(IIIa,
derivatives
transferase bitors
transfer
AND
2'-
Our results
IIIb)
can act
show that
that
by the
peptidyl
the
although at
derivatives
indicating
can be recognized
COMMUNICATIONS
as acceptors
and 3'-U-aminoacyl
transferase,
RESEARCH
the
peptidyl
are potent
3'-terminus
of
transferase
only
inhi-
2'-O-
A-site.
MATERIALS AND METHODS Three
times
Biochemicals)
NHqCl-washed
and Ac-(3H)Phe-tRNA,
alanine/mg
tRNA, were
The chemical phosphates
the
in this
assay
study
2'-
will
0.44
described
cells
nmoles
(General
phenyl-
(5).
and 3'-O-aminoacyldinucleoside elsewhere.
was measured
are given
MRE-600
activity
be described
activity
conditions
E. coZi
as previously of the
transferase
from
specific
prepared
synthesis
used
Peptidyl of
ribosomes
in the
as before
figure
(5).
Details
legends.
RESULTS AND DISCUSSION As can be seen
(IIIa)
C-A(2'H)Phe
from
Fig.
1, only
peptidyl
transferase
reaction
system.
No activity
has been observed
range
adenosine
derivatives
acceptor
of
1 X 10m5 M less
than
report
by the of
peptidyl
transferase
proved
that
prepared 3'-A$red
reaction, by chemical indeed
These
whereas
active
762
over
a wide
with
the
analogous
The decreased
to C-APhe
(I)
may be attributed results
a mixture
synthesis
P'-O-amino-
(IIb)
same trend
relative
are
that
(8) (at to
consistent
2'-A$red,
was active. acceptor
the
2'-
with
in the
and 3'-isomers
Our recent (5).
steric
prepared
was inactive of
in the S ribosome
corresponding
and digestion,
the
of Ac-Phe
elsewhere).
(9) who showed
aminoacylation
is
the
the
of C-APhe)
group.
acceptors
and C-A(2'Phe)Me
(IIIb)
that
and Ofengand
by enzymic
ox-red Of APhe
50% of
with
observed
C-A(2'Me)Phe
derivatives
Ac-Phe-tRNA*poly(U)*70
to be published
2'-O-methyl
Hussain
tRNAoXmred
We have
are
the
(IIa)
(results
activity
hindrance
using
C-A(2'Phe)H
of concentration.
3'-O-aminoacyl
(IIIb)
and C-A(2'Me)Phe
acyloligonucleotides
the
report
We therefore
the from
Vol.56,No.3,
1974
BIOCHEMICAL
100
AND BIOPHYSICAL
r
ACCEPTOR
Figure
1
conclude of
the
that
peptidyl
transferase
although
this
fact
of AA-tRNA
is
required
ribosomal Binding
peptidyl
CONC.
(M)
2’- and 3'-O-L-Phenylalanyldinucleoside phosphate dependent release of the Ac-(3H)Phe residue from Ac-(3H)Phe-tRNA in the peptidyl transferase reaction. Each reaction mixture contained in 0.10 ml: 50 mM Tris-HCl (pH 7.4), 100 mM NH4C1, 10 mM MgC12, 3.7 A2 0 units of ribosomes, 10 pg poly(U), and 0.12 A260 units of AC-(3H P Phe-tRNA (2000 cpm) . The reaction was initiated by addition of the acceptor compounds at the concentrations indicated. Following incubation at 37' for 30 min, the reaction was terminated by the addition of 2.0 ml of 2.5% CC13COOH at 4'. After 15 min at 4", the entire reaction mixture was filtered through a HAWP-Millipore membrane which was then washed with three 2.0 ml portions of cold 2.5% CC13COOH. After the membranes were dried, the radioactivity was determined in a 4.5 g PPO/lOO mg dimethyl-POPOP/l liter toluene scintillation mixture. The amount of Ac-(3H)Phe residue transferred from Ac-(3H)PhetRNA to the acceptor was determined as the difference between radioactivity retained on the filter after incubation without acceptor and that retained after incubation with an acceptor. It was expressed as the percentage of the radioactivity of Ac(3H)Phe-tRNA added to the experimental mixture. Symbols: 0, C-APhe (I); A, C-A(2'Phe)H IIa); 0, C-A(2'Phe)Me (IIb); A, C-A(2'H)Phe (IIIa); m, 2'Me)Phe (IIIb).
AA-tRNA,
3'-isomer
RESEARCH COMMUNICATIONS
possesses per
se does for
all
specificity
for
the
3'-isomer
not
necessarily
mean that
steps
of protein
biosynthesis
the at
stage.l of
transferase
the
acceptor A-site
terminu-s should
of AA-tRNA
precede
the
peptide
1 Recently, Fraser and Rich (10) speculated newly-formed peptidyl-tRNA (which is the 3'-isomer) Psite may be associated with 3' + 2' transacylation.
763
(e.g.,
CCA-AA) bond forming
that translocation from the A-site
to
the step
of to
(ll),
Vol.
56,
No.
3, 1974
INHIBITOR
BIOCHEMICAL
CONC.
Figure
2.
and if
2'-O-aminoacyl-tRNA
competition aminoacyl indeed
between
case.
inhibitors
of
the
containing
system
BlOPHYSlCAi
aw
(Ml
RESEARCH
INHIBITOR
COMMUNICATIONS
CONC.
(M)
Ac-(3H)Phe-puromycin formation as a function of 2'- and 3'-O-Lphenylalanyldinucleoside phosphate concentrations. The reaction mixtures were identical to those described in Figure 1 except that 1.0 X 10-4 M puromycin was also present. Compounds IIa, IIb, IIIa and IIIb were present at the concentrations indicated on the abscissa and ribosomes were added last to initiate the reactions. After 30 min at 37' the reactions were terminated (with 0.1 ml of 0.1 M Be(NO3)2 and 0.3 M NaOAc (pH 5.5) saturated with MgS04) and Ac-(3H)Phe-puromycin was extracted with 1.5 ml of ethyl acetate, as described by Monro et al. (14). The radioactivity of 1.0 ml aliquots of the ethyl acetate extract was measured in 10 ml of 4.5gPPO/lOO mg dimethyl-POPOP/0.25 liters 2-methoxyethanol/l liter Control experiments, in which toluene scintillation mixture. puromycin was omitted, indicated that little or no radioactivity Percent of Ac-(3H)Phe-puromycin was extracted to ethyl acetate. formed represents the amount of Ac-(3H)Phe-puromycin formed in the presence of aminoacyldinucleoside phosphate relative to the 100% Ac-(3H)Phe-puromycin formed amount formed in its absence. was equal to 1525 cpm. [;',I--, C-APhe (I); A, C-A(2'Phe)H (IIa); 0, C-A(2'H)Phe (IIIa). --, C-APhe (I); q , C-A(2'Phe)Me (IIb); D, C-A(2'Me)Phe (IIIb).
can be bound
puromycin,
derivatives, the
AND
the
peptidyl
P'-O-aminoacyl transferase
that
be able
acceptor
Ac-Phe
transfer
poly(U),
764
2'-o-
This
was
were
excellent
to puromycin
and 70 S ribosomes
2'(3')-0-aminoacylnucleosides compete with puromycin
the
and the
(IIb).*
IIa and IIb,
derivatives,
as donor,
to demonstrate
substrate,
and C-A(2'Phe)Me
mediated
Ac-Phe-tRNA
2 We had previously shown 2'(3')-O-aminoacyloli onucleotides transferase activity 9 12).
standard
(IIa)
C-A(2'Phe)H Both
we should
and in peptidyl
in
Vol.
56,
No.
3. 1974
BIOCHEMICAL
AN5
BlOPHYSlCAi
PUROMYCIN
Figure
Their
2).
that the
2'-
activity,
(IIIa)
C-A(2'H)Phe
good acceptor
can be seen inhibitory
from
be recognized
binding
2.5
X 10-5
the
inhibitory
(50% inhibition
In addition,
Fig. effect
The above by the
at
3, increasing of
up to the
IIa and IIb,
1.4
results peptidyl
3 Recently, C-A was found to ribosomes (13).
indicate
that
transferase
was similar
probably
as either
of the
3'-isomers
X 10m4 M) and C-A(2'Me)Phe these
compounds
to be completely
of
not
that act
inac-
at the
As
overcomes
puromycin
and the
same ribo-
derivatives
We therefore
are
shown).3
puromycin
2'-O-aminoacyl
to be a weak inhibitor
to
can exist
10m3 M (data
A-site.
765
IIb,
although
indicating
IIa and IIb,
Ac-Phe-puromycin
activity
concentration thus
of
M) which
C-A was found
at a concentration
2'-O-aminoacyloligonucleotides, site.
at
at 8 X 10 -5 M), was lower
substrates.
as an inhibitor
50% inhibition
Significantly,
(50% inhibition
somal
CONC. (M)
and 3.3 X 10m5 M for
IIa
(50% inhibition
or 3'-isomer. 2),
(IIIb)
the
(I)
of C-APhe
(Fig.
tive
inhibitory
at 4 X 10V5 M for
formation
COMMUNKATIONS
Reversal of C-A(2'Phe)H (IIa) and C-A(P'Phe)Me (IIb) inhibition of Ac-(3H)Phe-puromycin formation in the peptidyl transferase reaction. Reactions were executed as in Figure 2 except that the concentrations of IIa and IIb were held constant (4.0 X ,lO-5 and 3.4 X 10-5 M respectively) and the concentration of puromycin varied as indicated in the figure. Percent inhibition represents the difference in counts between reaction mixtures with both puromycin and the aminoacyldinucleoside phosphate present and that containing just puromycin. 0, C-A(2'Phe)H (IIa); A, C-A(P'Phe)Me (IIb).
3.
(Fig.
RESEARCH
would
of chloramphenicol
may like
M
BIOCHEMICAL
Vol.56,No.3,1974
to suggest
that
the
same may hold
AND BlOPHYSlCAi
true
for
the
here
do not
they
do show that
RESEARCH COMMUNICATIONS
3'-terminus
of
2'-O-aminoacyl-
tRNA. Although ribosomal
2'
the + 3'
data
transacylation,
can bind
to ribosomes,
however,
that
EF-T,
the
dependent
presented
presumably
isomer
binding
to the
integrity
of
establish
A-site.
the
presence
of
2'-O-aminoacyl-tRNA It
remains
2'-O-aminoacyl-tRNA
to be proven,
is retained
during
to ribosomes.
ACKNOWLEDGEMENTS This Research
investigation
was supported
Grant
No. GM-19111-02
Medical
Sciences
and in part
Cancer
Foundation
grateful
to Dr.
evaluation
of
from
the
from
in part the
by U.S.
National
by an institutional United
Harmon McAllister
Foundation
Institute grant
of Greater
(Wayne State
University)
Public
Health of
to the Detroit. for
Service
General Michigan We are a critical
the manuscript.
REFERENCES 1. 2. 3. 4. :: 7. i: 10. 11. 12. 13. 14.
Zachau, H. G. and Feldman, H. In "Progress in Nucleic Acid Research and Molecular Biology", 4, 217 (196u. Wolfenden, R., Ranmler, D. H. and Lipmann, F. Biochemistry, 3, 329 (1964). Griffin, B. E., Jarman, M., Reese, C. B., Sulston, J. E. and Trentham, D. R. Biochemistry, 2, 3638 (1966). Nathans, D. and Neidle, A. Nature, 197, 1076 (1963). Chlidek, S., Ringer, D. and femliEka, J. Biochemistry, in ress. Ofengand, J. and Chen, C.-M. J. Biol. Chem., 247, 2049 -972 e-r . Sprinzl, M. and Cramer, F. Nature New Biol., 245, 3 (1973). Ringer, D. and Chla'dek, S. FEBS Letters, in press. Hussain, Z. and Ofengand, J. Biochem. Biophys. Res. Cornnun., a, 1143 (1973). Fraser, T. H. and Rich, A. Proc. Natl. Acad. Sci. U.S.A., 70, 2671 (1973). T. and Lessard, J. L. J. Biol. Chem., 245, 6208 Pestka, S., Hishizawa, (1970). Rychlfk, I., Cernd, J., Chla'dek, S., Pulkrabek, J., Zemlizka, J. and Haladovd, Z. FEBS Symposium, 2l-, 47 (1970). Nierhaus, D. and Nierhaus, K. H. Proc. Natl. Acad. Sci. U.S.A., 70, 2224 (1973). J. and Marcker, K. A. Proc. Natl. Acad. Sci. U.S.A., Monro, R. E., terni, 6J, 1042 (1968).
766
1974
BIOCHEMICAL
INHIBITION
AND BIOPHYSICAL
OF THE PEPTIDYL
RESEARCH COMMUNICATIONS
TRANSFERASE A-SITE
FUNCTION
BY 2’-O-AMINOACYLOLIGONUCLEOTIDES David Michigan
Received
December
Ringer
Cancer
and Stanislav
Foundation,
Chla/dek*
Detroit,
Michigan
48201
11,1973 SUMMARY
New "non-isomerizable" analogs of the 3'-terminus of AA-tRNA, C-A(2'Phe)H, C-A(P'Phe)Me, C-A(2'H)Phe and C-A(2'Me)Phe, were tested as acceptor substrates of ribosomal peptidyl transferase and inhibitors of the peptidyl transferase A-site function. The 3'-O-AA-derivatives were active acceptors of Ac-Phe in while the PI-O-AA-derivatives were completely the peptidyl transferase reaction, inactive. Both 2'- and 3'-O-AA-derivatives were potent inhibitors of peptidyl transferase catalyzed Ac-Phe transfer to puromycin. The results indicate that although peptidyl transferase exclusively utilizes 3'-O-esters of tRNA as acceptor substrates, its A-site can also recognize the 3'-terminus of 2'-OAA-tRNA. INTRODUCTION Since
the discovery
in protein
biosynthesis,
terminal
adenosine
Because the
of the
cis-diol
the
Moreover,
tRNA that
is
unit
the
employed
* To whom reprint 110 E. Warren Avenue,
direct
exact
involvement
location
has been the rapid
terminal
exact it
the
the
extremely
of
to determine tRNA.
of
2'
subject
z 3'
of
now appears
that
throughout
the
the
of
unit
the
of
(2,3),
aminoacyl it
is
various
requests should Detroit, Michigan
amfnoacyl
considerable
migration
adenosine
position
of
of 2'(3')-U-aminoacyl-tRNA
not
the it
is
residue a single
stages
be sent: 48201.
on the
interest
(1).
aminoacyl
group
almost
impossible
in native isomer
of protein Michigan
residue
of
of
aminoacylaminoacyl-
biosynthesis.
Cancer
Foundation,
Abbreviations: C-APhe, cytidyly1(3'-5')-2'(3')-O-L-phenylalanyladenosine (I); C-A(2'Phe)H, cytidyly1(3'-5')-3'-deoxy-2'-O-L-phenylalanyladenosine (IIa); C-A(2'Phe)Me, cytidyly1(3'-5')-3'-O-methyl-2'-u-~-phenylalanyladenosine (IIb); C-A(2'H)Phe, cytidyly1(3'-5')-2'-deoxy-3'-O-L-phenylalanyladenosine (IIIa); C-A(2'Me)Phe, cytidyly1(3'-5')-2'-&methyl-3'-O-L-phenylalanyladenosine (IIIb); tRNAox-red, tRNA w ich has been oxidized with periodate, reduced with borohydride (6); A#,;'" !4 , L-phenylalanyl derivative of oxidizedreduced adenosine, either "2"' or "3"' -isomer (for correct nomenclature of the latter, see ref. 5). 760
Vol.
56, No.
On the
3, 1974
basis
BIOCHEMICAL
of the
amtnoacyl-tRNA inhibiting
structure
and its
AND
and activity
2'-analog
polypeptide
BIOPHYSICAL
(the
synthesis),
of puromycin
latter
it
RESEARCH
COMMUNICATIONS
as a 3'-analog
was found
of
to be inactive
has been suggested
that
in
3'-O-aminoacyl-
C
HOCHz
0
1cs; 0 7 HO-P=0
0
OH
I HO-P=0
OH
OH
HO-P=0
I A
&HZ
6Cl-l~
A
0 w
ii
bPhe
PheO
R
v Phe.H
I
n
o;R=H
IItO,R=H
b,R=OCHa
tRNA is
the
active
we have
recently
analog
of
ferase
reaction
reported
is
3'-isomer
PI-isomer
is
formed
by the
(4).
acceptor
must occur
peptidyl
inactive (7)
have
synthetase after
a "non-isomerizable" in the
virtually
and Cramer
AA-tRNA
More specifically,
of AFi,red,
an active
and Sprinzl
transacylation
(5).
shown
reaction,
enzymic
transStudies
that
thus
2'-Oindicating
aminoacylation
and before
bond formation. As part
various
whether
several the
(ITb), substrates
of our stages
or not
ribosomal
at
biosynthesis
the is
its
and Chen (6)
2' + 3'
the
that
and that
aminoacyl-tRNA
peptide
in protein
3'-U-aminoacyl-tRNA,
by Ofengand
that
isomer
bj R=OCHa
study
of
of protein
a 2'
+ 3'
or 3'-hydroxyl.
C-A(2'H)Phe for
(IIIa) peptidyl
this
in which compounds,
and C-A(2'Me)Phe transferase
3'-terminus
is a required
to study
These
of the
we have been
transacylation
aminoacyloligonucleotides 2'-
involvement
biosynthesis,
In order
mechanism.
the
the
and as inhibitors
761
residue
(IIa),
C-A(2'Phe)H
(IIIb),
in the
we have
aminoacyl
were
tested of
tRNA in
interested
step
question,
of
peptidyl
to learn overall
synthesized is
"fixed"
C-A(2'Phe)Me as acceptor transferase
Vol.
56,
No.
3, 1974
catalyzed
BIOCHEMICAL
Ac-Phe
3'-0-aminoacyl
to
center,
of
both
peptidyl
aminoacyl-tRNA
BlOPHYSlCAi
puromycin.
(IIIa,
derivatives
transferase bitors
transfer
AND
2'-
Our results
IIIb)
can act
show that
that
by the
peptidyl
the
although at
derivatives
indicating
can be recognized
COMMUNICATIONS
as acceptors
and 3'-U-aminoacyl
transferase,
RESEARCH
the
peptidyl
are potent
3'-terminus
of
transferase
only
inhi-
2'-O-
A-site.
MATERIALS AND METHODS Three
times
Biochemicals)
NHqCl-washed
and Ac-(3H)Phe-tRNA,
alanine/mg
tRNA, were
The chemical phosphates
the
in this
assay
study
2'-
will
0.44
described
cells
nmoles
(General
phenyl-
(5).
and 3'-O-aminoacyldinucleoside elsewhere.
was measured
are given
MRE-600
activity
be described
activity
conditions
E. coZi
as previously of the
transferase
from
specific
prepared
synthesis
used
Peptidyl of
ribosomes
in the
as before
figure
(5).
Details
legends.
RESULTS AND DISCUSSION As can be seen
(IIIa)
C-A(2'H)Phe
from
Fig.
1, only
peptidyl
transferase
reaction
system.
No activity
has been observed
range
adenosine
derivatives
acceptor
of
1 X 10m5 M less
than
report
by the of
peptidyl
transferase
proved
that
prepared 3'-A$red
reaction, by chemical indeed
These
whereas
active
762
over
a wide
with
the
analogous
The decreased
to C-APhe
(I)
may be attributed results
a mixture
synthesis
P'-O-amino-
(IIb)
same trend
relative
are
that
(8) (at to
consistent
2'-A$red,
was active. acceptor
the
2'-
with
in the
and 3'-isomers
Our recent (5).
steric
prepared
was inactive of
in the S ribosome
corresponding
and digestion,
the
of Ac-Phe
elsewhere).
(9) who showed
aminoacylation
is
the
the
of C-APhe)
group.
acceptors
and C-A(2'Phe)Me
(IIIb)
that
and Ofengand
by enzymic
ox-red Of APhe
50% of
with
observed
C-A(2'Me)Phe
derivatives
Ac-Phe-tRNA*poly(U)*70
to be published
2'-O-methyl
Hussain
tRNAoXmred
We have
are
the
(IIa)
(results
activity
hindrance
using
C-A(2'Phe)H
of concentration.
3'-O-aminoacyl
(IIIb)
and C-A(2'Me)Phe
acyloligonucleotides
the
report
We therefore
the from
Vol.56,No.3,
1974
BIOCHEMICAL
100
AND BIOPHYSICAL
r
ACCEPTOR
Figure
1
conclude of
the
that
peptidyl
transferase
although
this
fact
of AA-tRNA
is
required
ribosomal Binding
peptidyl
CONC.
(M)
2’- and 3'-O-L-Phenylalanyldinucleoside phosphate dependent release of the Ac-(3H)Phe residue from Ac-(3H)Phe-tRNA in the peptidyl transferase reaction. Each reaction mixture contained in 0.10 ml: 50 mM Tris-HCl (pH 7.4), 100 mM NH4C1, 10 mM MgC12, 3.7 A2 0 units of ribosomes, 10 pg poly(U), and 0.12 A260 units of AC-(3H P Phe-tRNA (2000 cpm) . The reaction was initiated by addition of the acceptor compounds at the concentrations indicated. Following incubation at 37' for 30 min, the reaction was terminated by the addition of 2.0 ml of 2.5% CC13COOH at 4'. After 15 min at 4", the entire reaction mixture was filtered through a HAWP-Millipore membrane which was then washed with three 2.0 ml portions of cold 2.5% CC13COOH. After the membranes were dried, the radioactivity was determined in a 4.5 g PPO/lOO mg dimethyl-POPOP/l liter toluene scintillation mixture. The amount of Ac-(3H)Phe residue transferred from Ac-(3H)PhetRNA to the acceptor was determined as the difference between radioactivity retained on the filter after incubation without acceptor and that retained after incubation with an acceptor. It was expressed as the percentage of the radioactivity of Ac(3H)Phe-tRNA added to the experimental mixture. Symbols: 0, C-APhe (I); A, C-A(2'Phe)H IIa); 0, C-A(2'Phe)Me (IIb); A, C-A(2'H)Phe (IIIa); m, 2'Me)Phe (IIIb).
AA-tRNA,
3'-isomer
RESEARCH COMMUNICATIONS
possesses per
se does for
all
specificity
for
the
3'-isomer
not
necessarily
mean that
steps
of protein
biosynthesis
the at
stage.l of
transferase
the
acceptor A-site
terminu-s should
of AA-tRNA
precede
the
peptide
1 Recently, Fraser and Rich (10) speculated newly-formed peptidyl-tRNA (which is the 3'-isomer) Psite may be associated with 3' + 2' transacylation.
763
(e.g.,
CCA-AA) bond forming
that translocation from the A-site
to
the step
of to
(ll),
Vol.
56,
No.
3, 1974
INHIBITOR
BIOCHEMICAL
CONC.
Figure
2.
and if
2'-O-aminoacyl-tRNA
competition aminoacyl indeed
between
case.
inhibitors
of
the
containing
system
BlOPHYSlCAi
aw
(Ml
RESEARCH
INHIBITOR
COMMUNICATIONS
CONC.
(M)
Ac-(3H)Phe-puromycin formation as a function of 2'- and 3'-O-Lphenylalanyldinucleoside phosphate concentrations. The reaction mixtures were identical to those described in Figure 1 except that 1.0 X 10-4 M puromycin was also present. Compounds IIa, IIb, IIIa and IIIb were present at the concentrations indicated on the abscissa and ribosomes were added last to initiate the reactions. After 30 min at 37' the reactions were terminated (with 0.1 ml of 0.1 M Be(NO3)2 and 0.3 M NaOAc (pH 5.5) saturated with MgS04) and Ac-(3H)Phe-puromycin was extracted with 1.5 ml of ethyl acetate, as described by Monro et al. (14). The radioactivity of 1.0 ml aliquots of the ethyl acetate extract was measured in 10 ml of 4.5gPPO/lOO mg dimethyl-POPOP/0.25 liters 2-methoxyethanol/l liter Control experiments, in which toluene scintillation mixture. puromycin was omitted, indicated that little or no radioactivity Percent of Ac-(3H)Phe-puromycin was extracted to ethyl acetate. formed represents the amount of Ac-(3H)Phe-puromycin formed in the presence of aminoacyldinucleoside phosphate relative to the 100% Ac-(3H)Phe-puromycin formed amount formed in its absence. was equal to 1525 cpm. [;',I--, C-APhe (I); A, C-A(2'Phe)H (IIa); 0, C-A(2'H)Phe (IIIa). --, C-APhe (I); q , C-A(2'Phe)Me (IIb); D, C-A(2'Me)Phe (IIIb).
can be bound
puromycin,
derivatives, the
AND
the
peptidyl
P'-O-aminoacyl transferase
that
be able
acceptor
Ac-Phe
transfer
poly(U),
764
2'-o-
This
was
were
excellent
to puromycin
and 70 S ribosomes
2'(3')-0-aminoacylnucleosides compete with puromycin
the
and the
(IIb).*
IIa and IIb,
derivatives,
as donor,
to demonstrate
substrate,
and C-A(2'Phe)Me
mediated
Ac-Phe-tRNA
2 We had previously shown 2'(3')-O-aminoacyloli onucleotides transferase activity 9 12).
standard
(IIa)
C-A(2'Phe)H Both
we should
and in peptidyl
in
Vol.
56,
No.
3. 1974
BIOCHEMICAL
AN5
BlOPHYSlCAi
PUROMYCIN
Figure
Their
2).
that the
2'-
activity,
(IIIa)
C-A(2'H)Phe
good acceptor
can be seen inhibitory
from
be recognized
binding
2.5
X 10-5
the
inhibitory
(50% inhibition
In addition,
Fig. effect
The above by the
at
3, increasing of
up to the
IIa and IIb,
1.4
results peptidyl
3 Recently, C-A was found to ribosomes (13).
indicate
that
transferase
was similar
probably
as either
of the
3'-isomers
X 10m4 M) and C-A(2'Me)Phe these
compounds
to be completely
of
not
that act
inac-
at the
As
overcomes
puromycin
and the
same ribo-
derivatives
We therefore
are
shown).3
puromycin
2'-O-aminoacyl
to be a weak inhibitor
to
can exist
10m3 M (data
A-site.
765
IIb,
although
indicating
IIa and IIb,
Ac-Phe-puromycin
activity
concentration thus
of
M) which
C-A was found
at a concentration
2'-O-aminoacyloligonucleotides, site.
at
at 8 X 10 -5 M), was lower
substrates.
as an inhibitor
50% inhibition
Significantly,
(50% inhibition
somal
CONC. (M)
and 3.3 X 10m5 M for
IIa
(50% inhibition
or 3'-isomer. 2),
(IIIb)
the
(I)
of C-APhe
(Fig.
tive
inhibitory
at 4 X 10V5 M for
formation
COMMUNKATIONS
Reversal of C-A(2'Phe)H (IIa) and C-A(P'Phe)Me (IIb) inhibition of Ac-(3H)Phe-puromycin formation in the peptidyl transferase reaction. Reactions were executed as in Figure 2 except that the concentrations of IIa and IIb were held constant (4.0 X ,lO-5 and 3.4 X 10-5 M respectively) and the concentration of puromycin varied as indicated in the figure. Percent inhibition represents the difference in counts between reaction mixtures with both puromycin and the aminoacyldinucleoside phosphate present and that containing just puromycin. 0, C-A(2'Phe)H (IIa); A, C-A(P'Phe)Me (IIb).
3.
(Fig.
RESEARCH
would
of chloramphenicol
may like
M
BIOCHEMICAL
Vol.56,No.3,1974
to suggest
that
the
same may hold
AND BlOPHYSlCAi
true
for
the
here
do not
they
do show that
RESEARCH COMMUNICATIONS
3'-terminus
of
2'-O-aminoacyl-
tRNA. Although ribosomal
2'
the + 3'
data
transacylation,
can bind
to ribosomes,
however,
that
EF-T,
the
dependent
presented
presumably
isomer
binding
to the
integrity
of
establish
A-site.
the
presence
of
2'-O-aminoacyl-tRNA It
remains
2'-O-aminoacyl-tRNA
to be proven,
is retained
during
to ribosomes.
ACKNOWLEDGEMENTS This Research
investigation
was supported
Grant
No. GM-19111-02
Medical
Sciences
and in part
Cancer
Foundation
grateful
to Dr.
evaluation
of
from
the
from
in part the
by U.S.
National
by an institutional United
Harmon McAllister
Foundation
Institute grant
of Greater
(Wayne State
University)
Public
Health of
to the Detroit. for
Service
General Michigan We are a critical
the manuscript.
REFERENCES 1. 2. 3. 4. :: 7. i: 10. 11. 12. 13. 14.
Zachau, H. G. and Feldman, H. In "Progress in Nucleic Acid Research and Molecular Biology", 4, 217 (196u. Wolfenden, R., Ranmler, D. H. and Lipmann, F. Biochemistry, 3, 329 (1964). Griffin, B. E., Jarman, M., Reese, C. B., Sulston, J. E. and Trentham, D. R. Biochemistry, 2, 3638 (1966). Nathans, D. and Neidle, A. Nature, 197, 1076 (1963). Chlidek, S., Ringer, D. and femliEka, J. Biochemistry, in ress. Ofengand, J. and Chen, C.-M. J. Biol. Chem., 247, 2049 -972 e-r . Sprinzl, M. and Cramer, F. Nature New Biol., 245, 3 (1973). Ringer, D. and Chla'dek, S. FEBS Letters, in press. Hussain, Z. and Ofengand, J. Biochem. Biophys. Res. Cornnun., a, 1143 (1973). Fraser, T. H. and Rich, A. Proc. Natl. Acad. Sci. U.S.A., 70, 2671 (1973). T. and Lessard, J. L. J. Biol. Chem., 245, 6208 Pestka, S., Hishizawa, (1970). Rychlfk, I., Cernd, J., Chla'dek, S., Pulkrabek, J., Zemlizka, J. and Haladovd, Z. FEBS Symposium, 2l-, 47 (1970). Nierhaus, D. and Nierhaus, K. H. Proc. Natl. Acad. Sci. U.S.A., 70, 2224 (1973). J. and Marcker, K. A. Proc. Natl. Acad. Sci. U.S.A., Monro, R. E., terni, 6J, 1042 (1968).
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