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Role of modified nucleoside adjacent to 3t́-end of anticodon in codon-anticodon interaction
Vol. 40, No. 1, 1970
ROLE
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
OF MODIFIED
NUCLEOSIDE
ADJACENT
CODON-ANTICODON Kakoli
Ghosh
Department McMaster
Received
OF ANTICODON
IN
INTERACTION
and of
University,
TO 3'-END
H.
P.
Ghosh
Biochemistry
Hamilton,
Ontario,
Canada.
May 26, 1970
Summary: Removal of the base Y adjacent to the anticodon o yeast tRNAPhe changes its coding properties. Modified tRNA 6 he The codon UUU responds to the codon UUC better than the +5 odon UUU. can be read efficiently only at higher Mg cont. or in the presence of streptomycin. Binding studies show that the unmodified and the modified tRNAPhe can not occur next to each other on the two binding sites of a ribosome. Removal of Y changes the configuration of the anticodon loop of tRNAPhe such that the base (G) involved in "Wobble" changes its relative orientation to the other bases in the anticodon. The
phenylalanine
contain end
a flourescent of
the
adenosine case
of
tRNA
action.
of
any
and in
the
of
conformational
or
removal
nucleoside it
is
structure
(1,2).
Occurrence
a modified
nucleoside
a possible
role
(5)
have
position
is
the
than
is
needed
codons
the
Previous
base
to
essential
for
binding for
been
of
prevent
charging
anticodon
of 135
the
this
the
U or
A
in
reading may
also
has
the
(6,7,8).
the
the
increase
anticodon
suggest
of by
the
involving
the
inter-
function
ribosome-mRNA tRNA
3'-
in
position
the
It of
to
the
a modified
with
the
studies
tRNA
to
observed
that
anticodon
the
germ
codon-anticodon
anticodon.
flexibility. adjacent
of
the
conformation of
wheat
adjacent
at
in
to
and
beginning
proposed
the
stacked
yeast
have
of
("Wobble@'base)
the
anticodon to
other
of
not
unknown
of
) of
corresponding
this
of
5'-base
Y of
Hodgson
triplet
stabilization
that
(tRNAPhe
3'-end
suggests
purine
codon
the
presence
Fuller
alkylated
but
to
loop
RNA
2'-OMeGAA
species
The
anticodon
base
anticodon, next
(3,4).
the
transfer
such
maximal
degree
modification that
this
complex
Vol. 40, No. 1, 1970
The
results
the
presented
base
cont.
in
the
removal the
of
anticodon
the not
Yeast
acid
coated
with
The for
1.2
rations
of
pH
buffer,
described
isolated by
1.1
the
T and
G were
a procedure separation
Mg +2
a higher
the
suggest
that
configuration
loop.
The
conformation
tRNAFhe
and
5'-base, and
and
2'-OMeG
therefore
from
aminoacids --et
were
using
al.
described
Nishimura
2.
___ coli
MRE600
either
of
Erbe
--et
(16).
involving followed
al.
from the by
both
--et by The
E.
-coli
separation
partial
tRNAGhe
per
A260
as
assayed
separation
136
0.05M
of
flourescence
cacodylate
tRNA
species
synthetase
as
was
purified
Gordon
E.
acids the
prepa-
were (15)
polymerizing and
nucleic
could
Ribosomes
aminoacid
of
the
synthetase
method
two
260 pH 2.9,
The
by
(14).
the
at
isolated
aminoacyl-tRNA
al.
A
the
chromatography
The
MRE600 of
acid
unit.
in
Aminoacyl-tRNA
(13). by
purified
The
(11,12).
yeast
silicic of
per
with
BD-cellulose
determined
MgC12
on
phenylalanine
by
tRNAPhe
(BD-
activities
tRNAPhe
phenylalanine
0.015M
acceptor of
(7).
spectra
containing
The
isolated
- cellulose
chromatography
treating
Zachau
free
DEAE
further
nmoles
by was
were
Ghosh
benzoylated by
1.3
removed
Thiebe
with
method
by
to
tRNA;he
from
its
preferentially
results
changes
rigid
(9,lO).
of
as
a more
followed
and
7.0
yeast
anticodon
isolated
nmoles
by
of
the
at
of
U.
1.5
charged
from
was
Flourescence
spectra.
only
removal
affects
UUC is
These loop
with
Y was
by to
recognized
anticodon
have
were
4 hours
accept
codon
streptomycin.
BD-cellulose
base
described
be
the
the
tRNA Phe
yeast
cont.
that
Methods:
isolated
unit.
were
now
chromatography
tRNAPhels
as
the
pair
tRNAPhe
cellulose)
of
show
of
Mg +2
pattern
"Wobble"
and
anticodon
UUU can
Y from
may
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
communication
low
codon
stacking
Materials
the
presence
of
hence,
this
At The
or
37O
to
properties.
recognized.
can
in
Y adjacent
coding
the
BIOCHEMICAL
coli by factors
or factor
B cells polymer
by phase
T and
G
Vol. 40, No. 1, 1970
by
(NH4j2
on
Polypeptide
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
(15).
The
a DEAE-Sephadex
column
synthesis
ribopolynucleotides
sequences
were
ribosomes
in
was
fractionation
SO4
purified
BIOCHEMICAL
followed
using
followed
as
as
before
the
peptidyl
site
as
described
by
two
described
(13).
--et
were
and
al.
further
by
Erbe
of
repeating
Binding
(P site) Ono
factors
of
--et
al.
(16).
aminoacyl-tRNA
aminoacyl
site
to
(A site)
(17).
Results: It
was
previously
transfer both
shown
phenylalanine poly
r-U
and
Results
(18). Phe-tRNAihe
that into
poly
to
transfer
tRNAPhe
charged
polyphenylalanine
r-(U-U-C),
presented
fails
yeast
in
under
using Figure
homologously the
a ribosomal
1 show
phenylalanine
that into
direction
system at
can
a Mg+2
from cont.
polyphenylalanine
of --E.
coli
of
1OmM as
A A-
-C-OMe
A G-Ok U C -0Me
/A ,G ,A ,C ,c
G
ll
G A. Fig.
1.
G Phe tRNA
B.
c-
I Phe tRNAp
Kinetics of incorporation of phenylalanine. The reaction mixture contained per ml: Tris-Cl. pH 7.5, 10 nmoles; NH4C1-160 nmoles: DTT-10 pmoles; GTP-1 washed ribosome-21 A260 units; umole; T and G factor C14-Phe-tRNAPhe-350 pmoles or C14-Phe-tRNAThe-362 - 48Oug; 'nmoles and Mg acetate as indicated. The template cont. was 1.0 A260 units of poly U or 5.8 pmoles of poly r-(U-U-C) Phenylalanine polymerized was assayed as described per ml. earlier (13). 137
Vol. 40, No. 1, 1970
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
i
c 8 N
138
BIOCHEMICAL
Vol. 40, No. 1, 1970
directed
by
poly
Phe-tRNAPhe triplet
and
the
these
by
75
of
poly
of
fold.
is, that
of
in
1.
Table
effect
on
cont.
from
Presence
of
of cont. that
anticodon
loop
longer
pair
A steric
enzymatic
P site.
of
with
of
between
on
thus the
binding
C14-Phe-tRNAPhe
the
occur
Phe-tRNA
N-acetyl
results Y
changed
can
are not
they
shown has
1OmM and
20mM Mg
no
poly
r-U
by
25-fold.
At
The
+2
results
loop
relative
in
above
anticodon
tRNA
molecule
higher
tRNA Phe
of
loop,.
The
orientation base
occupy
the
complex.
Phe at the Y Phe-tRNAPhe
to
are
by
"Wobble"
modified when
Phe-tRNA;he
10 ug/ml
anticodon the
the
in
(2'-OMeG)
can
the no
cont.
presented bind
the
its
the
UUC are
Polyphenlalanine
observed.
of
ribosome-mRNA
of
containing The
have
both
stimulated
configuration
presence
studied
results
r-(U-U-C).
Y from
tRNA Phe so that Y U at lower Mg+2
may
sites
the
base
we
of
at
is
r-U
UUU and
from
directed
however,
poly
These
(19),
a cont.
poly
stimulates
in
codons
The
at
by
tRNA;he
tRNA;he.
r-(U-U-C).
Phe-tRNAFe
the
might
hindrance
molecule
binding
from
by
Z-fold.
the
phenylalanine
directed
20mM
incorporation
stimulation
in
2'-OMeGAA
miscoding
poly
is,
removal
anticodon
induce
streptomycin
significant
a change
of
of
streptomycin no
produces
and
by
both
phenylalanine
incorporation
Phe-tRNAPhe, Y at 1OmM Mg +2
presence
suggest
r-U
cont.
anticodon to
on poly
the
synthesis
+2
both
the
known
streptomycin by
complex
by is
Mg +2
to
Phe-tRNA;he
only
the
of
directed
from
both
Clearly
cont.
Phe-tRNAGhe
increased
by
(2'-OMeGAA)
Mg+2
synthesis
higher
efficiently
directed
tRNA
at
recognized
condition.
the
from
however,
is
anticodon
Increasing
streptomycin
effect
the
Polyphenylalanine
recognized
however,
identical
by
phenylalanine
suggest
Since
recognized
r-(U-U.-C)
results
Mg
not
under
conditions.
transfer
r-(U-U-C),
Phe-tRNAGhe
UUU is
under
Poly
r-U.
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
in poly
or
the
therefore,
of
r-U-ribosome
2.
The
normal
consecutive
poly
tested
at
results complex
the
r-U-ribosome
N-Ac-Phe-tRNAGhe
Table
139
two
We,
A site
and
the
show at
both
that 1OmM
20 mM
10 mM
+2 % cont.
Ac-H3-Phe-tRNA
bound
of
Phe Y
(p
to
22.0
11.0
14.0
5.4
moles/ml)
cl4 -p;;:;;NA;e
C 14-Phe-tRNA
2
bound
A site
20.3
< .05
7.8
< .05
Ac-H3-Phe-C14-Phe formed
The two step reaction as described by Ono --et al. (17) was followed. In step I the reaction mixture contained per ml. of ribosome 4 A260 units of poly U, 126 31 A260 units Phe or 135 pmoles pmoles of Ac-H3-Phe-tRNAp of Ac-H3-PhetRNAPhe and Mg acetate as indicated. Step II reaction mixt 8 re contained per ml.0.05 pmoles of GTP, 1 pmoles of Fusidic acid, 150 l.lg of T, 435 pmoles of C14-Phe-tRNAshe and Mg acetate as indicated. Both reaction mixture contained 0.04M Tris-Cl, pH 7.4, 0.01M DTT and 0.16M NH4Cl.
23.6
72.0
Ac-H3-Phe-tRNAPhe
71.2 7.0
Phe v
Phe
Total Ac-H3-Phe-tRNA
-Phe-tRNAye
Ac-H3
Ac-H3-Phe-tRNA
Ac-Phe-tRNA in the P site
'Binding
TABLE
s.-
BIOCHEMICAL AND BIOPHYSICAL
Vol. 40, No. 1, 1970
(Mg++)
(M9 ++)
= 1OmM
RESEARCH COMMUNICATIONS
=2OmM I
k“? _ c+Pdv
15
30
Phe-1RNAPPs u v
60
90
1
Time [min] Fig.
2.
Schematic diagram of the model for tRNA anticodon arm. (a) Fuller and Hodg son model for tRNAPhe. (b) Proposed alternate model for tRNA:he. The alternate model proposes a change in the stacking pattern of the anticodon only. The helical character of the structure is considered to be the same as postulated by Fuller and Hodgson (5).
20mM Mg +2 when the Phe tRNA . On the other and
P site
the
ribosome
when
the
P site
is
occupied
by
ribosome-poly Phe Phe , C 14 -Phe-tRNA can bind is occupied by N-Ac-H3-Phe-tRNA Y Y 14 -Phe site and the dipeptide N-Ac-H3-Phe-C is synthesized. strongly of
suggest
the
loops
anticodon of
tRNA
hand
of
tRNA Phe
that loops.
Phe
and
and
tRNAye
is
of
have
tRNAthe
A possible
different
schematic
diagram
in
2.
shown
N-Ac-H3-Phe-
Figure
r-U
complex
to
the
These
A results
configuration of
the
anticodon
Discussion Previous to
the
workers
anticodon
reported or
modification
that
removal of
the
141
of
the
side-chain
modified of
base this
base
adjacent affects
Vol. 40, No. 1, 1970
its
binding
to
transfe.r
BIOCHEMICAL
capacity
to
aminoacids
however,
show
of
codon
recognition
of
the
by
anticodon
are
now
no
longer
the
flexibility
the
Mg
of
the
known
to
tRNA
molecule
Y however, Also GTP
and
base
and
Phe
the
(unpublished
Fuller
and
more, is
our
results
possible
and
alternate
to
as
streptomycin
the
known
of
codon
as
the
is
so
of
that
5' -base
show
that
the
alternate
active.
anticodon
conformation
stacking
an
functionally
studies
in of
loop of
of
is
loop,
base
anticodon
Phe
of of
have
Y the
> with modified
recognized
and
may
model
pairing.
support
the
is
anticodon
not
structure of
cont.
The
that
lend
Results tRNAiet
+2
(12,21).
normal
loop
loop
the
the
the
, indicating
anticodon
involved
tightens
(T-GTP-Phe-tRNA-
anticodon Our
stability
loop
involves
Phe
Increasing
Mg
of
has
the
Also
anticodon
nature
the
base
increase
configuration
Phe-tRNA
and
pairing.
(20).
the
conformation
"Wobble"
streptomycin
ability
finding,
only
the
The
complex
its
pyrimidines
may
UUC which
of
affects
"Wobble"
the
tertiary
well
model
its
miscoding
changed
the
two 2).
that
observation).
base loop
binding
forms
Hodgson
modified
anticodon
of
configuration
factor
the
the
that
for
allow
the
base
(Fig.
conformation
with
TT T equally
such
hence, Our
Presumably,
needed
is
and
(6,7,8).
modified
together
and
recognizes Phe-tRNA
changed
It
the
this
chain
anticodon.
presence
ribosome
change
Phe
is
pair.
of
the
stacked
or
"Wobble"
structure
of
RESEARCH COMMUNICATIONS
complex
polypeptide
removal
loop
cont.
mRNA-ribosome
into
that
anticodon
+2
the
AND BIOPHYSICAL
by
to
the
suggest
bases
in
that the
"Wobble".
Further-
anticodon
loop
conformatio
oligonucleotide
already
suggested
the
an
anticodon loop (22). for his interest and critical We thank Dr. R. H. Hall Acknowledgment: This work has been supported by a grant from the Medical discussion. is a Medical MA 3514 ). H.P.G. Research Council of Canada (grant no. Research Council Scholar. References 1. 2.
u. L. RajBhandary, S. H. Chang, A. Stuart, and H. G. Khorana, Proc. R. M. Hoskinson, U.S., 57 751 (i967). B. S. Kdock, G. Katz, E. D. Taylor, and Natl. Acad. Sci., U. S., 62, 941 (1969) 142
R. D. Faulkner, Natl. Acad. Sci., R.
W.
Holley,
T
Proc.
Vol. 40, No. 1, 1970
3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16. 17. 18. 19. 20. 21. 22.
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
W. J. Burrows, F. Skoog, K. L. Roy, and D. J,., Armstrong, D. Soll, Proc. Natl. Acad. Sci., 63, 834 (1969) H. Ishikura, Y. Yamada, K. Murao, M. Saneyoshi, and S. Nishimura, Biochem. Biophys. Res. Cmmun., 37, 990 (1969). W. Fuller, and A. Hodgson, Nature, 215, 277 (1967). Fittler, and R. H. Hall, Biochem, Biophys. Res. Commun., 25, :;l (1966). R. Thiebe, and H. G. Zachau, European J. Biochem., 5, 546, (1968). M. L. Gefter, and R. L. Russell, J. Mol, Biol., 2, l&5 (1969). I. Gillam, S. Millward, D. Blew, M. von Tigerstrom, E. Wimmer, and G. M. Tenner, Biochemistry, 6, 3043 (1967). E. Wimmer, I. H. Maxwell, and G. M. Tenner, Biochemistry, 1, 2623 (1968). D. Yoshikami, G. Katz, E. B. Keller, and B. S. Dudock, Biochem. Biophys. Acta, 166, 714 (1968). 3. Eisinger, B. Fener, and T. Yamane, Proc. Natl. Acad. Sci., U. S., 638 (1970). .g., H. P. Ghosh, D. Sull, and H. G. Khorana, J. Mol. Biol. 25, 275 (1967) F. Harada, U. Narushima, and T. Seno, Biochim, S. Nishimura, Biophys. Acta 142, 133 (1967). J. Biol. Chem., z, 5680 (1969). J. Gordon, R. W. Erbe, M. M. Nau, and P. Leder, J. Mol. Biol., 38, 441 (1969). J. Waterson, and P. Lengyel, Nature, 222, 645 Y. Ono, A. Skoultchi, (1969). D. S811, and U. L. RajBhandary, J. Mol. Biol., 29, 113 (1967). J. Davies,. W. Gilbert, and L. Gorini, Proc. Natl. Acad. Sci., U. S., 883 (1964). 51, M. I. Sherman, and M. V. Simpson, Proc. Natl. Acad. Sci., U. S. 2, 1338 (1969). K. Beardsley, and C. R. Cantor, Fred. Proc., 2, 672 (1970). 0. c. Uhlenbeck, J. Baller, and P. Doty, Nature 25, 508 (1970).
143
ROLE
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
OF MODIFIED
NUCLEOSIDE
ADJACENT
CODON-ANTICODON Kakoli
Ghosh
Department McMaster
Received
OF ANTICODON
IN
INTERACTION
and of
University,
TO 3'-END
H.
P.
Ghosh
Biochemistry
Hamilton,
Ontario,
Canada.
May 26, 1970
Summary: Removal of the base Y adjacent to the anticodon o yeast tRNAPhe changes its coding properties. Modified tRNA 6 he The codon UUU responds to the codon UUC better than the +5 odon UUU. can be read efficiently only at higher Mg cont. or in the presence of streptomycin. Binding studies show that the unmodified and the modified tRNAPhe can not occur next to each other on the two binding sites of a ribosome. Removal of Y changes the configuration of the anticodon loop of tRNAPhe such that the base (G) involved in "Wobble" changes its relative orientation to the other bases in the anticodon. The
phenylalanine
contain end
a flourescent of
the
adenosine case
of
tRNA
action.
of
any
and in
the
of
conformational
or
removal
nucleoside it
is
structure
(1,2).
Occurrence
a modified
nucleoside
a possible
role
(5)
have
position
is
the
than
is
needed
codons
the
Previous
base
to
essential
for
binding for
been
of
prevent
charging
anticodon
of 135
the
this
the
U or
A
in
reading may
also
has
the
(6,7,8).
the
the
increase
anticodon
suggest
of by
the
involving
the
inter-
function
ribosome-mRNA tRNA
3'-
in
position
the
It of
to
the
a modified
with
the
studies
tRNA
to
observed
that
anticodon
the
germ
codon-anticodon
anticodon.
flexibility. adjacent
of
the
conformation of
wheat
adjacent
at
in
to
and
beginning
proposed
the
stacked
yeast
have
of
("Wobble@'base)
the
anticodon to
other
of
not
unknown
of
) of
corresponding
this
of
5'-base
Y of
Hodgson
triplet
stabilization
that
(tRNAPhe
3'-end
suggests
purine
codon
the
presence
Fuller
alkylated
but
to
loop
RNA
2'-OMeGAA
species
The
anticodon
base
anticodon, next
(3,4).
the
transfer
such
maximal
degree
modification that
this
complex
Vol. 40, No. 1, 1970
The
results
the
presented
base
cont.
in
the
removal the
of
anticodon
the not
Yeast
acid
coated
with
The for
1.2
rations
of
pH
buffer,
described
isolated by
1.1
the
T and
G were
a procedure separation
Mg +2
a higher
the
suggest
that
configuration
loop.
The
conformation
tRNAFhe
and
5'-base, and
and
2'-OMeG
therefore
from
aminoacids --et
were
using
al.
described
Nishimura
2.
___ coli
MRE600
either
of
Erbe
--et
(16).
involving followed
al.
from the by
both
--et by The
E.
-coli
separation
partial
tRNAGhe
per
A260
as
assayed
separation
136
0.05M
of
flourescence
cacodylate
tRNA
species
synthetase
as
was
purified
Gordon
E.
acids the
prepa-
were (15)
polymerizing and
nucleic
could
Ribosomes
aminoacid
of
the
synthetase
method
two
260 pH 2.9,
The
by
(14).
the
at
isolated
aminoacyl-tRNA
al.
A
the
chromatography
The
MRE600 of
acid
unit.
in
Aminoacyl-tRNA
(13). by
purified
The
(11,12).
yeast
silicic of
per
with
BD-cellulose
determined
MgC12
on
phenylalanine
by
tRNAPhe
(BD-
activities
tRNAPhe
phenylalanine
0.015M
acceptor of
(7).
spectra
containing
The
isolated
- cellulose
chromatography
treating
Zachau
free
DEAE
further
nmoles
by was
were
Ghosh
benzoylated by
1.3
removed
Thiebe
with
method
by
to
tRNA;he
from
its
preferentially
results
changes
rigid
(9,lO).
of
as
a more
followed
and
7.0
yeast
anticodon
isolated
nmoles
by
of
the
at
of
U.
1.5
charged
from
was
Flourescence
spectra.
only
removal
affects
UUC is
These loop
with
Y was
by to
recognized
anticodon
have
were
4 hours
accept
codon
streptomycin.
BD-cellulose
base
described
be
the
the
tRNA Phe
yeast
cont.
that
Methods:
isolated
unit.
were
now
chromatography
tRNAPhels
as
the
pair
tRNAPhe
cellulose)
of
show
of
Mg +2
pattern
"Wobble"
and
anticodon
UUU can
Y from
may
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
communication
low
codon
stacking
Materials
the
presence
of
hence,
this
At The
or
37O
to
properties.
recognized.
can
in
Y adjacent
coding
the
BIOCHEMICAL
coli by factors
or factor
B cells polymer
by phase
T and
G
Vol. 40, No. 1, 1970
by
(NH4j2
on
Polypeptide
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
(15).
The
a DEAE-Sephadex
column
synthesis
ribopolynucleotides
sequences
were
ribosomes
in
was
fractionation
SO4
purified
BIOCHEMICAL
followed
using
followed
as
as
before
the
peptidyl
site
as
described
by
two
described
(13).
--et
were
and
al.
further
by
Erbe
of
repeating
Binding
(P site) Ono
factors
of
--et
al.
(16).
aminoacyl-tRNA
aminoacyl
site
to
(A site)
(17).
Results: It
was
previously
transfer both
shown
phenylalanine poly
r-U
and
Results
(18). Phe-tRNAihe
that into
poly
to
transfer
tRNAPhe
charged
polyphenylalanine
r-(U-U-C),
presented
fails
yeast
in
under
using Figure
homologously the
a ribosomal
1 show
phenylalanine
that into
direction
system at
can
a Mg+2
from cont.
polyphenylalanine
of --E.
coli
of
1OmM as
A A-
-C-OMe
A G-Ok U C -0Me
/A ,G ,A ,C ,c
G
ll
G A. Fig.
1.
G Phe tRNA
B.
c-
I Phe tRNAp
Kinetics of incorporation of phenylalanine. The reaction mixture contained per ml: Tris-Cl. pH 7.5, 10 nmoles; NH4C1-160 nmoles: DTT-10 pmoles; GTP-1 washed ribosome-21 A260 units; umole; T and G factor C14-Phe-tRNAPhe-350 pmoles or C14-Phe-tRNAThe-362 - 48Oug; 'nmoles and Mg acetate as indicated. The template cont. was 1.0 A260 units of poly U or 5.8 pmoles of poly r-(U-U-C) Phenylalanine polymerized was assayed as described per ml. earlier (13). 137
Vol. 40, No. 1, 1970
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
i
c 8 N
138
BIOCHEMICAL
Vol. 40, No. 1, 1970
directed
by
poly
Phe-tRNAPhe triplet
and
the
these
by
75
of
poly
of
fold.
is, that
of
in
1.
Table
effect
on
cont.
from
Presence
of
of cont. that
anticodon
loop
longer
pair
A steric
enzymatic
P site.
of
with
of
between
on
thus the
binding
C14-Phe-tRNAPhe
the
occur
Phe-tRNA
N-acetyl
results Y
changed
can
are not
they
shown has
1OmM and
20mM Mg
no
poly
r-U
by
25-fold.
At
The
+2
results
loop
relative
in
above
anticodon
tRNA
molecule
higher
tRNA Phe
of
loop,.
The
orientation base
occupy
the
complex.
Phe at the Y Phe-tRNAPhe
to
are
by
"Wobble"
modified when
Phe-tRNA;he
10 ug/ml
anticodon the
the
in
(2'-OMeG)
can
the no
cont.
presented bind
the
its
the
UUC are
Polyphenlalanine
observed.
of
ribosome-mRNA
of
containing The
have
both
stimulated
configuration
presence
studied
results
r-(U-U-C).
Y from
tRNA Phe so that Y U at lower Mg+2
may
sites
the
base
we
of
at
is
r-U
UUU and
from
directed
however,
poly
These
(19),
a cont.
poly
stimulates
in
codons
The
at
by
tRNA;he
tRNA;he.
r-(U-U-C).
Phe-tRNAFe
the
might
hindrance
molecule
binding
from
by
Z-fold.
the
phenylalanine
directed
20mM
incorporation
stimulation
in
2'-OMeGAA
miscoding
poly
is,
removal
anticodon
induce
streptomycin
significant
a change
of
of
streptomycin no
produces
and
by
both
phenylalanine
incorporation
Phe-tRNAPhe, Y at 1OmM Mg +2
presence
suggest
r-U
cont.
anticodon to
on poly
the
synthesis
+2
both
the
known
streptomycin by
complex
by is
Mg +2
to
Phe-tRNA;he
only
the
of
directed
from
both
Clearly
cont.
Phe-tRNAGhe
increased
by
(2'-OMeGAA)
Mg+2
synthesis
higher
efficiently
directed
tRNA
at
recognized
condition.
the
from
however,
is
anticodon
Increasing
streptomycin
effect
the
Polyphenylalanine
recognized
however,
identical
by
phenylalanine
suggest
Since
recognized
r-(U-U.-C)
results
Mg
not
under
conditions.
transfer
r-(U-U-C),
Phe-tRNAGhe
UUU is
under
Poly
r-U.
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
in poly
or
the
therefore,
of
r-U-ribosome
2.
The
normal
consecutive
poly
tested
at
results complex
the
r-U-ribosome
N-Ac-Phe-tRNAGhe
Table
139
two
We,
A site
and
the
show at
both
that 1OmM
20 mM
10 mM
+2 % cont.
Ac-H3-Phe-tRNA
bound
of
Phe Y
(p
to
22.0
11.0
14.0
5.4
moles/ml)
cl4 -p;;:;;NA;e
C 14-Phe-tRNA
2
bound
A site
20.3
< .05
7.8
< .05
Ac-H3-Phe-C14-Phe formed
The two step reaction as described by Ono --et al. (17) was followed. In step I the reaction mixture contained per ml. of ribosome 4 A260 units of poly U, 126 31 A260 units Phe or 135 pmoles pmoles of Ac-H3-Phe-tRNAp of Ac-H3-PhetRNAPhe and Mg acetate as indicated. Step II reaction mixt 8 re contained per ml.0.05 pmoles of GTP, 1 pmoles of Fusidic acid, 150 l.lg of T, 435 pmoles of C14-Phe-tRNAshe and Mg acetate as indicated. Both reaction mixture contained 0.04M Tris-Cl, pH 7.4, 0.01M DTT and 0.16M NH4Cl.
23.6
72.0
Ac-H3-Phe-tRNAPhe
71.2 7.0
Phe v
Phe
Total Ac-H3-Phe-tRNA
-Phe-tRNAye
Ac-H3
Ac-H3-Phe-tRNA
Ac-Phe-tRNA in the P site
'Binding
TABLE
s.-
BIOCHEMICAL AND BIOPHYSICAL
Vol. 40, No. 1, 1970
(Mg++)
(M9 ++)
= 1OmM
RESEARCH COMMUNICATIONS
=2OmM I
k“? _ c+Pdv
15
30
Phe-1RNAPPs u v
60
90
1
Time [min] Fig.
2.
Schematic diagram of the model for tRNA anticodon arm. (a) Fuller and Hodg son model for tRNAPhe. (b) Proposed alternate model for tRNA:he. The alternate model proposes a change in the stacking pattern of the anticodon only. The helical character of the structure is considered to be the same as postulated by Fuller and Hodgson (5).
20mM Mg +2 when the Phe tRNA . On the other and
P site
the
ribosome
when
the
P site
is
occupied
by
ribosome-poly Phe Phe , C 14 -Phe-tRNA can bind is occupied by N-Ac-H3-Phe-tRNA Y Y 14 -Phe site and the dipeptide N-Ac-H3-Phe-C is synthesized. strongly of
suggest
the
loops
anticodon of
tRNA
hand
of
tRNA Phe
that loops.
Phe
and
and
tRNAye
is
of
have
tRNAthe
A possible
different
schematic
diagram
in
2.
shown
N-Ac-H3-Phe-
Figure
r-U
complex
to
the
These
A results
configuration of
the
anticodon
Discussion Previous to
the
workers
anticodon
reported or
modification
that
removal of
the
141
of
the
side-chain
modified of
base this
base
adjacent affects
Vol. 40, No. 1, 1970
its
binding
to
transfe.r
BIOCHEMICAL
capacity
to
aminoacids
however,
show
of
codon
recognition
of
the
by
anticodon
are
now
no
longer
the
flexibility
the
Mg
of
the
known
to
tRNA
molecule
Y however, Also GTP
and
base
and
Phe
the
(unpublished
Fuller
and
more, is
our
results
possible
and
alternate
to
as
streptomycin
the
known
of
codon
as
the
is
so
of
that
5' -base
show
that
the
alternate
active.
anticodon
conformation
stacking
an
functionally
studies
in of
loop of
of
is
loop,
base
anticodon
Phe
of of
have
Y the
> with modified
recognized
and
may
model
pairing.
support
the
is
anticodon
not
structure of
cont.
The
that
lend
Results tRNAiet
+2
(12,21).
normal
loop
loop
the
the
the
, indicating
anticodon
involved
tightens
(T-GTP-Phe-tRNA-
anticodon Our
stability
loop
involves
Phe
Increasing
Mg
of
has
the
Also
anticodon
nature
the
base
increase
configuration
Phe-tRNA
and
pairing.
(20).
the
conformation
"Wobble"
streptomycin
ability
finding,
only
the
The
complex
its
pyrimidines
may
UUC which
of
affects
"Wobble"
the
tertiary
well
model
its
miscoding
changed
the
two 2).
that
observation).
base loop
binding
forms
Hodgson
modified
anticodon
of
configuration
factor
the
the
that
for
allow
the
base
(Fig.
conformation
with
TT T equally
such
hence, Our
Presumably,
needed
is
and
(6,7,8).
modified
together
and
recognizes Phe-tRNA
changed
It
the
this
chain
anticodon.
presence
ribosome
change
Phe
is
pair.
of
the
stacked
or
"Wobble"
structure
of
RESEARCH COMMUNICATIONS
complex
polypeptide
removal
loop
cont.
mRNA-ribosome
into
that
anticodon
+2
the
AND BIOPHYSICAL
by
to
the
suggest
bases
in
that the
"Wobble".
Further-
anticodon
loop
conformatio
oligonucleotide
already
suggested
the
an
anticodon loop (22). for his interest and critical We thank Dr. R. H. Hall Acknowledgment: This work has been supported by a grant from the Medical discussion. is a Medical MA 3514 ). H.P.G. Research Council of Canada (grant no. Research Council Scholar. References 1. 2.
u. L. RajBhandary, S. H. Chang, A. Stuart, and H. G. Khorana, Proc. R. M. Hoskinson, U.S., 57 751 (i967). B. S. Kdock, G. Katz, E. D. Taylor, and Natl. Acad. Sci., U. S., 62, 941 (1969) 142
R. D. Faulkner, Natl. Acad. Sci., R.
W.
Holley,
T
Proc.
Vol. 40, No. 1, 1970
3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16. 17. 18. 19. 20. 21. 22.
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
W. J. Burrows, F. Skoog, K. L. Roy, and D. J,., Armstrong, D. Soll, Proc. Natl. Acad. Sci., 63, 834 (1969) H. Ishikura, Y. Yamada, K. Murao, M. Saneyoshi, and S. Nishimura, Biochem. Biophys. Res. Cmmun., 37, 990 (1969). W. Fuller, and A. Hodgson, Nature, 215, 277 (1967). Fittler, and R. H. Hall, Biochem, Biophys. Res. Commun., 25, :;l (1966). R. Thiebe, and H. G. Zachau, European J. Biochem., 5, 546, (1968). M. L. Gefter, and R. L. Russell, J. Mol, Biol., 2, l&5 (1969). I. Gillam, S. Millward, D. Blew, M. von Tigerstrom, E. Wimmer, and G. M. Tenner, Biochemistry, 6, 3043 (1967). E. Wimmer, I. H. Maxwell, and G. M. Tenner, Biochemistry, 1, 2623 (1968). D. Yoshikami, G. Katz, E. B. Keller, and B. S. Dudock, Biochem. Biophys. Acta, 166, 714 (1968). 3. Eisinger, B. Fener, and T. Yamane, Proc. Natl. Acad. Sci., U. S., 638 (1970). .g., H. P. Ghosh, D. Sull, and H. G. Khorana, J. Mol. Biol. 25, 275 (1967) F. Harada, U. Narushima, and T. Seno, Biochim, S. Nishimura, Biophys. Acta 142, 133 (1967). J. Biol. Chem., z, 5680 (1969). J. Gordon, R. W. Erbe, M. M. Nau, and P. Leder, J. Mol. Biol., 38, 441 (1969). J. Waterson, and P. Lengyel, Nature, 222, 645 Y. Ono, A. Skoultchi, (1969). D. S811, and U. L. RajBhandary, J. Mol. Biol., 29, 113 (1967). J. Davies,. W. Gilbert, and L. Gorini, Proc. Natl. Acad. Sci., U. S., 883 (1964). 51, M. I. Sherman, and M. V. Simpson, Proc. Natl. Acad. Sci., U. S. 2, 1338 (1969). K. Beardsley, and C. R. Cantor, Fred. Proc., 2, 672 (1970). 0. c. Uhlenbeck, J. Baller, and P. Doty, Nature 25, 508 (1970).
143