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Genetic recombination of phage S13 in a recombination-deficient mutant of Escherichiacoli K12
Vol. 22, No. 2, 1966
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
GENETIC RECOMBINATION OF PHAGE S13 IN A RECOMBINATION-DEFICIENT
MUTANT OF ESCHERICHIA COLI K12
Irwin
Tessman
Department of Biological Sciences Purdue University, Lafayette, Indiana
Received
that
recombination
in Escherichia
reduces
the frequency
of recombinants
and Margulies,
1965).
the recombination
mechanism bination
used
recombination 2. phage
genetic
material;
To determine
whether
the
under
protein
likely
the
species;
close
S13 presumably stranded
of the
contains
DNA (Tessman,
reduction
implies
must be the major
on phage
for
S13 recom-
I,
simple
II,
IIIa,
genetically
mutants
in group
1.7 x lo6
1958 and 1959;
daltons Sinsheimer,
169
genetic
IIIb,
II,
E.S.
in
of
or of the host
Tessman
(Sinsheimer, 1959).
communication) were
more than
linearity were
cell.
constitution.
and IV)
specify
frequencies 1958;
involved
1965 and personal
does not
to p)X174 (Zahler,
is
in recombination
phage
Tessman,
recombination
only
involved
of the
(labelled
the virus
and except
steps
relatively
(E.S.
groups
relation
here
same mechanism
control
of its
investigation
map and additivity of its
genetic
because
that
of 1000
objectives:
of the phage
5 complementation is
reported
this
are
large
by a mutation
a factor
by the mutation
whether
In a comprehensive
so it
of this
affected
The study
can be blocked
by more than
To determine
S13 was studied
only
cell.
has two specific
coli
The finding
mechanism
by the
1.
this
14, 1965
Genetic
(Clark that
December
of the
demonstrated. and Shleser, 1959)
found, about
5
genetic Because 1963),
of single-
Vol. 22, No. 2, 1966
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
METHODS A recombination-deficient isolated Both
by Clark
F- strains
resistant
and Margulies were
kindly
were
S13 were
labelled
-Ret+ and -Ret Because of these
of the mutagenic
respects.
medium with acids.
confirming also strains; (Clark
and Margulies,
phage.
Therefore,
strains
will
are the
sensitive
to
strains
used
be referred
was necessary
to as
still
and also
parent
grew
to ultraviolet
in (leu-)
as the only (try-)
Hfr
Trisadded
strain
than
of -Ret-. light
to be related
strain
on a synthetic
recombinants
property
each
leucine-requiring
and methionine
more u+trp+
to show that
to its
a tryptophan-requiring
is known
(KlO),
did &-,
The derived
strains
(IJV) as the original
to their
abilities
to recombine
1965).
recombination
was compared &)
Q')
recombinants
Cl22
or -Rec- and incubating
type
can form plaques.
-Ret
in tryptone
broth
mutants
were
in TB plus
+
in -Ret
of S13 that by plating
at 43',
a temperature
Crosses
were
(13 g of Bacto
performed tryptone of 4-8
1 x 10 -2 M CaC12.
at a multiplicity
of 5.
170
and -Retcannot
selected
of H20; TB) to a concentration
each mutant
it
at 43'
histidine
same sensitivities
type
added,
these
were
with
W sensitivity
to 2 x 108/m1
K12 strains
and colonies
Both derivatives
1000 times
temperature-sensitive
liter
These
JC-411.
N-methyl-N'-nitro-N-
was similar
the recombination-deficient
Phage
with
derivatives
leucine,
at least
had the
was strain
The two S13-sensitive
treatment
grew
In crosses
showed
the
1960),
and JC-1553.1;
and streptomycin-resistant,
&+
JC-1553,
respectively.
the following
amino
Clark.
to adsorb
plating.
two S13-sensitive
glucose
K12,
the non-deficient
by Dr.
and Greenberg,
by replica
JC-411.5
from
by treatment
(Mandell
isolated
(1965)
of a failure
mutagenized
nitrosoguanidine
of E. coli
supplied
to S13 because
two strains
were
mutant
by crossing grow
progeny
phage
at which by growing plus
Wild-
on _. E &
only the wild + Ret and
7 g of NaCl per
x lo7 cells/ml A pair
above 41'.
and concentrating
of phage mutants
The phage-cell
mixtures
was were
Vol. 22, No. 2, 1966
shaken
for
mixtures
5 min,
were
incubated
diluted
of the
X ~266,
that
at 42'
mixedly
infected;
infection
which
for
took
additional
day to day.
In part,
state
indicator,
sizes
were
this
plates,
the effect
of these
measured
is known
to stimulate
and Doermann,
1958;
Tomizawa
and Anraku,
Tessman,
at 42',
cannot
and Tessman,
by mixed For
of about
in -Ret
errors, +
2 from
such as the
and the exact
1964),
1959;
were
phage/cell.
temperature
for
of
each pair
of
and -Rec- at the same time.
recombination
be compared
cells
only
conditions,
which
E.S.
the
may be due to the assay
was always
(Tessman
that
a cross
of complementation.
30-50
age of the
one cross,
of performing
lethal
fluctuate
for
a factor
To minimize
experiments
except
as a result
between
The
Adsorption
within
the
frequencies
at 37'
assurance
Cyanide,
bination
to burst.
The purpose
growth
frequencies
recombination
the cells
are
adsorbed.
2 x 10 -3 M CaC12 and
TB plus
the t mutations be phage
of the phage
place
was to provide
The recombination
mutants
time
at 42'.
there
the incubator.
into
was performed
the burst
of the
85-95%
loo-fold
always
since
could
crosses,
phage
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
time
40 min to allow
entirely
all
during
then
for
and growth t76
BIOCHEMICAL
in phage
was not
with
those
E.S.
Tessman
used,
found
T4 (Chase
so the
recom-
in previous
and Shleser,
1963;
1965).
RESULTS Table pairwise the L"
1 shows the in
-RecR&c-,
6 different
recombinant
frequencies
of crosses. recombination
the
frequencies
for
5 mutants
crossed
ways in Ret+ and -Ret-.
Since
apparently
only
was observed,
in order
In each cross + than in -Ret . but
recombination
the frequencies
to account
for
the reciprocal
the recombination Not only
reduction
factors
For one class, frequencies
are
frequency
suggest
reduced
that only
was significantly
there group
by a factor
171
shown as twice
the t
+
recombinants.
the recombination
involving are
are
lower
frequencies are at I and IIIb
reduced
least
in
two classes
mutants,
of approximately
in
the 20 to 40
Vol. 22, No. 2, 1966
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE I RECOMBINATION OF S13 MUTANTS IN -REC+ AND -REC CrOSSeSa Mutants
groupsk
Frequency
units -I-Ret
of 10W5)
ratio
-Rec-
--Rec+/Rec-
2.5
0.13
19
IXI
t43
x
frequency
(in
Complementation
crossed t39
Recombination
t39
X ~266
I X IIIb
15
0.61
25
t39
x y11
I X IIIb
42
42
t39
x t11
I X IIIb
92
1.0 2.2
x I
30
3.9
~76 X t39
II
42 7.7
t76
X tll
II
X IIIb
30
4.7
6.4
t76
X ~266
II
X IIIb
50
12.4
4.0
~76 X t2661
II
X IIIb
32
8.4
3.8
a All crosses were performed at 37' which was performed at 42O.
except
for
the last
t76 X ~266
cross,
b The complementation groups are functional units determined by complementation tests. The mutants were classified by E.S. Tessman (1965) with the exception of tll, which I classified by its failure to complement ~266.
in -Ret
.
For the other
by a factor ratio
each class
Bacterial
one of these
involved
in
step
are
is
under
genetically In g-,
recombination
appears
steps,
cellular
phage is.
of phage
by the phage
or by the cell.
that
reduced
be because activity there
is
172
far
the phage very
also S13.
one cannot and whether
might
many steps.
must
recombination
recombinational
much more likely
in &-,
control,
is
is
of the --Rec+/Rec-
K12 may involve
mechanism
genetic
recombination
This
the reduction
significant.)
one blocked
recombination
in phage controlled
be considered
the
t76,
(The variation
in E. coli
bacterial
are involved
residual
cannot
the primary
mutant
4 to 8.
recombination
At loast
steps
involving
of approximately
within
this
class,
than
utilizes
effectively.
an important
Although
say what
these
less
be
secondary
other
other steps
bacterial the slight But it mechanism
only
Vol. 22, No. 2, 1966
BIOCHEMICAL
of recombination
that
conceivable
one mechanism
other
that
operates
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
only
for
could
the
phage.
involve
For example,
breakage
it
is
and rejoining,
the
copy choice. The secondary
effective mutants
crosses
in groups
group
II
from
all
crosses group
for
mutants the
be crossed
involving
behave
A fact
anomalously
roughly
Tessman,
characteristic
of mutants
In a cross
of 8.5% and 8.0% were data).
Thus phage
primary
recombination
found
mutant
than
set
whether
more
for
the
be related
is
experiments;
that
S13 mutants ordered
map, except
to determine
for
by two-factor
mutants
from
of 513 mutants
the behavior
must
of ~76 is
II.
mutants
of phage +
T4 is different mechanism
~76
may possibly
A more complete
in -Ret
relatively
can be consistently
in group
of two -rI1
that
additive
1965).
in -Ret+ and -Ret-
II
apparently
in mapping
groups
and
is
the group
complementation
(E.S.
mechanism
I and IIIb.
on a linear II
recombination
T4,
recombination
and -Rec- respectively from both 5. coli
does not utilize
frequencies (Tessman,
unpublished
and S13 in that
the step
blocked
its
in -Ret-.
SUMMARY The primary
recombination
recombination-deficient is eliminated, into
the primary the
mutant
a secondary
at least
is
on the basis
and secondary
mechanisms
depends
for
of E. coli
mechanism
two classes
classification
mechanism
phage
K12.
When the primary
revealed. of the
to the
on the mutants
S13 is.blocked
Crosses
relative
in a mechanism
can be grouped
contributions
recombination
frequencies;
crossed.
ACKNOWLEDGMENTS This
research
was supported,
in part,
by NSF research
173
grant
GB-2748.
of
Vol. 22, No. 2, 1966
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
REFERENCES Chase, M., and Doermann, A. H. Genetics 43, 332 (1958). A. D. Proc. Natl. --Acad. Sci. u. 2. 53, 451 (1965). Clark, A. J., and Margulies, 2. BiochKBizs. Res. Corm. 3, 575 (1960). Mandell, J., and Greenberg, Sinsheimer, R. L. 2. Mol. Biol. I., 43 (1959). Tessman, E. S. ViroloFgx3 (1965). Tessman, E. S., and Shleser, R. Virology l-9, 239 (1963). Tessman, E. S., and Tessman, I. Virow1, 465 (1959). Tessman, I. Program and Abstracts of the Biophysical Society p. 42 (1958). Tessman, I. Virology7 263 (1959). Tomizawa, J., and Anraku, N. 2. Mol. Biol. 2, 508 (1964). Zahler, S. A. J. Bacterial. 75,310 (1958).
174
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
GENETIC RECOMBINATION OF PHAGE S13 IN A RECOMBINATION-DEFICIENT
MUTANT OF ESCHERICHIA COLI K12
Irwin
Tessman
Department of Biological Sciences Purdue University, Lafayette, Indiana
Received
that
recombination
in Escherichia
reduces
the frequency
of recombinants
and Margulies,
1965).
the recombination
mechanism bination
used
recombination 2. phage
genetic
material;
To determine
whether
the
under
protein
likely
the
species;
close
S13 presumably stranded
of the
contains
DNA (Tessman,
reduction
implies
must be the major
on phage
for
S13 recom-
I,
simple
II,
IIIa,
genetically
mutants
in group
1.7 x lo6
1958 and 1959;
daltons Sinsheimer,
169
genetic
IIIb,
II,
E.S.
in
of
or of the host
Tessman
(Sinsheimer, 1959).
communication) were
more than
linearity were
cell.
constitution.
and IV)
specify
frequencies 1958;
involved
1965 and personal
does not
to p)X174 (Zahler,
is
in recombination
phage
Tessman,
recombination
only
involved
of the
(labelled
the virus
and except
steps
relatively
(E.S.
groups
relation
here
same mechanism
control
of its
investigation
map and additivity of its
genetic
because
that
of 1000
objectives:
of the phage
5 complementation is
reported
this
are
large
by a mutation
a factor
by the mutation
whether
In a comprehensive
so it
of this
affected
The study
can be blocked
by more than
To determine
S13 was studied
only
cell.
has two specific
coli
The finding
mechanism
by the
1.
this
14, 1965
Genetic
(Clark that
December
of the
demonstrated. and Shleser, 1959)
found, about
5
genetic Because 1963),
of single-
Vol. 22, No. 2, 1966
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
METHODS A recombination-deficient isolated Both
by Clark
F- strains
resistant
and Margulies were
kindly
were
S13 were
labelled
-Ret+ and -Ret Because of these
of the mutagenic
respects.
medium with acids.
confirming also strains; (Clark
and Margulies,
phage.
Therefore,
strains
will
are the
sensitive
to
strains
used
be referred
was necessary
to as
still
and also
parent
grew
to ultraviolet
in (leu-)
as the only (try-)
Hfr
Trisadded
strain
than
of -Ret-. light
to be related
strain
on a synthetic
recombinants
property
each
leucine-requiring
and methionine
more u+trp+
to show that
to its
a tryptophan-requiring
is known
(KlO),
did &-,
The derived
strains
(IJV) as the original
to their
abilities
to recombine
1965).
recombination
was compared &)
Q')
recombinants
Cl22
or -Rec- and incubating
type
can form plaques.
-Ret
in tryptone
broth
mutants
were
in TB plus
+
in -Ret
of S13 that by plating
at 43',
a temperature
Crosses
were
(13 g of Bacto
performed tryptone of 4-8
1 x 10 -2 M CaC12.
at a multiplicity
of 5.
170
and -Retcannot
selected
of H20; TB) to a concentration
each mutant
it
at 43'
histidine
same sensitivities
type
added,
these
were
with
W sensitivity
to 2 x 108/m1
K12 strains
and colonies
Both derivatives
1000 times
temperature-sensitive
liter
These
JC-411.
N-methyl-N'-nitro-N-
was similar
the recombination-deficient
Phage
with
derivatives
leucine,
at least
had the
was strain
The two S13-sensitive
treatment
grew
In crosses
showed
the
1960),
and JC-1553.1;
and streptomycin-resistant,
&+
JC-1553,
respectively.
the following
amino
Clark.
to adsorb
plating.
two S13-sensitive
glucose
K12,
the non-deficient
by Dr.
and Greenberg,
by replica
JC-411.5
from
by treatment
(Mandell
isolated
(1965)
of a failure
mutagenized
nitrosoguanidine
of E. coli
supplied
to S13 because
two strains
were
mutant
by crossing grow
progeny
phage
at which by growing plus
Wild-
on _. E &
only the wild + Ret and
7 g of NaCl per
x lo7 cells/ml A pair
above 41'.
and concentrating
of phage mutants
The phage-cell
mixtures
was were
Vol. 22, No. 2, 1966
shaken
for
mixtures
5 min,
were
incubated
diluted
of the
X ~266,
that
at 42'
mixedly
infected;
infection
which
for
took
additional
day to day.
In part,
state
indicator,
sizes
were
this
plates,
the effect
of these
measured
is known
to stimulate
and Doermann,
1958;
Tomizawa
and Anraku,
Tessman,
at 42',
cannot
and Tessman,
by mixed For
of about
in -Ret
errors, +
2 from
such as the
and the exact
1964),
1959;
were
phage/cell.
temperature
for
of
each pair
of
and -Rec- at the same time.
recombination
be compared
cells
only
conditions,
which
E.S.
the
may be due to the assay
was always
(Tessman
that
a cross
of complementation.
30-50
age of the
one cross,
of performing
lethal
fluctuate
for
a factor
To minimize
experiments
except
as a result
between
The
Adsorption
within
the
frequencies
at 37'
assurance
Cyanide,
bination
to burst.
The purpose
growth
frequencies
recombination
the cells
are
adsorbed.
2 x 10 -3 M CaC12 and
TB plus
the t mutations be phage
of the phage
place
was to provide
The recombination
mutants
time
at 42'.
there
the incubator.
into
was performed
the burst
of the
85-95%
loo-fold
always
since
could
crosses,
phage
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
time
40 min to allow
entirely
all
during
then
for
and growth t76
BIOCHEMICAL
in phage
was not
with
those
E.S.
Tessman
used,
found
T4 (Chase
so the
recom-
in previous
and Shleser,
1963;
1965).
RESULTS Table pairwise the L"
1 shows the in
-RecR&c-,
6 different
recombinant
frequencies
of crosses. recombination
the
frequencies
for
5 mutants
crossed
ways in Ret+ and -Ret-.
Since
apparently
only
was observed,
in order
In each cross + than in -Ret . but
recombination
the frequencies
to account
for
the reciprocal
the recombination Not only
reduction
factors
For one class, frequencies
are
frequency
suggest
reduced
that only
was significantly
there group
by a factor
171
shown as twice
the t
+
recombinants.
the recombination
involving are
are
lower
frequencies are at I and IIIb
reduced
least
in
two classes
mutants,
of approximately
in
the 20 to 40
Vol. 22, No. 2, 1966
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE I RECOMBINATION OF S13 MUTANTS IN -REC+ AND -REC CrOSSeSa Mutants
groupsk
Frequency
units -I-Ret
of 10W5)
ratio
-Rec-
--Rec+/Rec-
2.5
0.13
19
IXI
t43
x
frequency
(in
Complementation
crossed t39
Recombination
t39
X ~266
I X IIIb
15
0.61
25
t39
x y11
I X IIIb
42
42
t39
x t11
I X IIIb
92
1.0 2.2
x I
30
3.9
~76 X t39
II
42 7.7
t76
X tll
II
X IIIb
30
4.7
6.4
t76
X ~266
II
X IIIb
50
12.4
4.0
~76 X t2661
II
X IIIb
32
8.4
3.8
a All crosses were performed at 37' which was performed at 42O.
except
for
the last
t76 X ~266
cross,
b The complementation groups are functional units determined by complementation tests. The mutants were classified by E.S. Tessman (1965) with the exception of tll, which I classified by its failure to complement ~266.
in -Ret
.
For the other
by a factor ratio
each class
Bacterial
one of these
involved
in
step
are
is
under
genetically In g-,
recombination
appears
steps,
cellular
phage is.
of phage
by the phage
or by the cell.
that
reduced
be because activity there
is
172
far
the phage very
also S13.
one cannot and whether
might
many steps.
must
recombination
recombinational
much more likely
in &-,
control,
is
is
of the --Rec+/Rec-
K12 may involve
mechanism
genetic
recombination
This
the reduction
significant.)
one blocked
recombination
in phage controlled
be considered
the
t76,
(The variation
in E. coli
bacterial
are involved
residual
cannot
the primary
mutant
4 to 8.
recombination
At loast
steps
involving
of approximately
within
this
class,
than
utilizes
effectively.
an important
Although
say what
these
less
be
secondary
other
other steps
bacterial the slight But it mechanism
only
Vol. 22, No. 2, 1966
BIOCHEMICAL
of recombination
that
conceivable
one mechanism
other
that
operates
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
only
for
could
the
phage.
involve
For example,
breakage
it
is
and rejoining,
the
copy choice. The secondary
effective mutants
crosses
in groups
group
II
from
all
crosses group
for
mutants the
be crossed
involving
behave
A fact
anomalously
roughly
Tessman,
characteristic
of mutants
In a cross
of 8.5% and 8.0% were data).
Thus phage
primary
recombination
found
mutant
than
set
whether
more
for
the
be related
is
experiments;
that
S13 mutants ordered
map, except
to determine
for
by two-factor
mutants
from
of 513 mutants
the behavior
must
of ~76 is
II.
mutants
of phage +
T4 is different mechanism
~76
may possibly
A more complete
in -Ret
relatively
can be consistently
in group
of two -rI1
that
additive
1965).
in -Ret+ and -Ret-
II
apparently
in mapping
groups
and
is
the group
complementation
(E.S.
mechanism
I and IIIb.
on a linear II
recombination
T4,
recombination
and -Rec- respectively from both 5. coli
does not utilize
frequencies (Tessman,
unpublished
and S13 in that
the step
blocked
its
in -Ret-.
SUMMARY The primary
recombination
recombination-deficient is eliminated, into
the primary the
mutant
a secondary
at least
is
on the basis
and secondary
mechanisms
depends
for
of E. coli
mechanism
two classes
classification
mechanism
phage
K12.
When the primary
revealed. of the
to the
on the mutants
S13 is.blocked
Crosses
relative
in a mechanism
can be grouped
contributions
recombination
frequencies;
crossed.
ACKNOWLEDGMENTS This
research
was supported,
in part,
by NSF research
173
grant
GB-2748.
of
Vol. 22, No. 2, 1966
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
REFERENCES Chase, M., and Doermann, A. H. Genetics 43, 332 (1958). A. D. Proc. Natl. --Acad. Sci. u. 2. 53, 451 (1965). Clark, A. J., and Margulies, 2. BiochKBizs. Res. Corm. 3, 575 (1960). Mandell, J., and Greenberg, Sinsheimer, R. L. 2. Mol. Biol. I., 43 (1959). Tessman, E. S. ViroloFgx3 (1965). Tessman, E. S., and Shleser, R. Virology l-9, 239 (1963). Tessman, E. S., and Tessman, I. Virow1, 465 (1959). Tessman, I. Program and Abstracts of the Biophysical Society p. 42 (1958). Tessman, I. Virology7 263 (1959). Tomizawa, J., and Anraku, N. 2. Mol. Biol. 2, 508 (1964). Zahler, S. A. J. Bacterial. 75,310 (1958).
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