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Cloning and characterization of the Schizosaccharomyces pombe DNA ligase gene CDC17
GHW. 41 (19X6) 321-325
321
Elscvier GENE
1518
Cloning and characterization (Recombinant
DNA;
L.H. Johnstona*,
of the Schizosacchavumyces
fission yeast;
suppressor;
promoter;
pombe DNA iigase gene CDCZ7 with Sacckarnm_vces cereviskre)
complementation
D.G. Barkera and Paul Nurseb
‘ILaboratrw.vof CeN Propagation, National Institute for Medicat Resecrrch, The Ridgewq. Mill Hill, London NW7 IAA, Tel. (01) 9593666, and ’ CeN Cj’cle Control Laborator?,. Imperial Cancer Research Fund, Lincoln k Iun Fields. Loudon WCZA 3PX (Ci~k’.J Tei. {01)2420200 (Received
July jth,
(Revision
received
(Accepted
1985) October
November
21st, 1985)
25th, 1985)
SUMMARY
The Sc~iz(~sacc~aromyces pombe CDCI 7 gene has been cloned by complementation of the cdel7 mutant coding for temperature-sensitive DNA ligase. An allele-specific suppressor active only in the presence of a high osmotic pressure was also isolated. The cloned CDCI 7 gene failed to complement the analogous DNA ligase mutation, cd&, in Saccharomyces cerevisiae, although the reverse complementation was successful [Barker and Johnston, Eur. J. Biochem. 134 (1983) 315-3191. The CDCl7 gene specifies a 2%kb transcript. __
Johnston,
INTRODUCTION
1983), and the analogous
gene CDCl7
from the fission yeast S. pombe (Nasmyth, 1977). The availability of ts mutants in these genes and of
The ubiquitous enzyme DNA ligase is required principally during DNA synthesis for the joining of Okazaki fragments and also for the repair of damaged DNA. A study of the control of expression of DNA ligase in different organisms might reveal features of cellular regulation which have been conserved during evolution. With this in mind we have initiated parallel studies into the regulation of the DNA ligase gene CDC9 from budding yeast, S. cerevisiae (Johnston and Nasmyth, 1978; Barker and
plasmid vector transformation systems for both organisms together provide a convenient approach both to cloning the genes and also to examining their heterologous expression and regulation. Following the isolation of the S. cerevisiae CDC9 gene (Barker and Johnston, 1983) we now describe the cloning and preliminary characterisation of the S. pombe CDCl7 gent.
* To whom correspondence
EXPERIMENTAL
and
reprint
requests
should
be
AND
DISCUSSION
addressed. Abbreviations:
bp, base pair(s);
types; kb, kilobase reading
plasmid-carrier
037X-I 119:X6/503.50
, S. pombe mating
or 1000 bp; nt. nucieotide(s);
frame; ss. single-stranded;
designates
h + and h
0
ORF, open
ts, temperature-sensitive:
state.
19X6 Elsevier
Science
Publishers
[ ],
(a) Cloning of CLlCZ7 A cdcf 7-K42 leui-32 strain of S. pombe was transformed (Beach et al., 1982a) with DNA from two
B.V. (Biomedical
Division)
322
clone banks, one in vector YEpl3 (Russell and Hall, 1983) and one constructed by inserting a partial Hind111 digest of chromosomal pDB262
(a positive selection
DNA
37°C after replication from the original sorbitol-agar plates. S5 tr~sformants also behaved similarly when first replicated onto minimal agar plates and
into vector
vector based upon the
bacteriophage
1. ci gene). Plates were incubated
the permissive
temperature
transformants
were replicated
grown at 25°C before transfer to YE-phloxin at 37°C. Only when replicated onto another sorbitol-
at
agar plate, which contains
of 25 “C and the resulting to yeast-extract
transformants
agar
plates containing 20 [kg phloxin B/ml YE-phloxin for further incubation at the restrictive temperature of 37°C. The phloxin stains dead cells a deep red colour
and therefore
aids the selection
did all
grow at 37 ‘C. The SS complementing
activity therefore differed from that of SlO and H2 in appearing to require high osmotic pressure for full effect; moreover,
of transfor-
it alone was alleIe-speci~c,
allele c&I 7-M75 being unaffected
mants that are able to grow at 37’ C and have a paler colour. A total of 1.5 colonies were obtained
1.2 M sorbitol,
another
by S5. Clone 55
therefore appears to be a suppressor and may be a protein which normally interacts with DNA ligase
at 37 “C
by this means, all of which showed the instability characteristic of plasmid-borne genes in yeast. Recombinant plasmid DNA extracted from three of these colonies and designated S5 and S 10 (vector Y Ep 13) and H2 (vector pDB262) was used to transform E. coli (as in Barker and Johnston, 1983). When re-isolated, each plasmid transformed S. pombe cdcl7 to growth on sorbitol-agar plates (Beach et al., 1982a) at the restrictive temperature with high frequency (about 4-6 x lO’/iig DNA). However, unlike SIO and H2 transformants, S5 transformants required some 44 h preincubation at 25’ C before the maximum number of colonies was observed at 37 ’ C, and only 2-3 T<,of these transformants were able to grow on YE-phloxin plates at
and which can partially overcome the cdc17-K42 mutation when its gene is present on a multi-copy plasmid. (b) Mapping of the CLXl7
gene
Restriction analysis (Fig. 1) and sub-cloning showed that S 10 and H2 had some 4.5 kb in common and that the CDC17 gene, possibly together with the information necessary for its expression, lies between the leftmost EcnRI site and the left BgtII site. Southern hybridisation (Southern, 1975) studies with the two probes shown in Fig. 1 confirmed that neither of these two clones had any sequence in common with S5 and that they were unrearranged
+.---+
lkb
2.4 kb Probe I
I
SSEAP I I
E
EACE
Bg
E
II
6.7 kb Probe I
I
HE I
H2
SSEAP I I III
E I
EAC E I II I
Bg
E
I
I
Bg I
C
H
I
t I
1
L
I
5’ SI Probe Fig. 1. Restriction used in Southern indicate
map ofclones hybridisation
complementing experiments
the ends of the c‘DCI7 transcript
U~irri; Bg, B@II; B, Ba/rtHi.
3’SI
cdc17.The hatched
areas represent
are shown. The two S 1mapping as determined
bq Sl nuclease
probes described mapping.
Probe
vector sequences
and the 2.4-kb and h.7-kb probes
rn Fig. 3 are also indicated.
H. HitzdIII;
E, EcoRI;
The two :~rows
S. Suil; A, Awl;
P. Purl: C.
323
compared (which
with
their
chromosomal
in S. pombe
are present
(c) Ligase synthesis
homologues
DNA
as single
copies) (not shown).
nation strain
into a cdcl7-K42
transformed
leul-32
the unrelated
h
comparative
and a stable clone from each was isolated.
These putative
integrants,
which could both grow at
plasmids,
not do so. For
the entire Hind111 fragment into YEpl3
(here-
so that all the cloned DNAs
in the same vector.
S5, SlO and HZ-YEp13,
The three
were each trans-
formed into cdcl7 and the crude extracts prepared from these transformants were assayed for levels of DNA ligase. S5 transformants possessed only the same low levels of a ts activity found with cdcl7 alone (Table I), confirming that S5 is probably a suppressor of cdcl7. In contrast, H2-Y Ep 13 directed the synthesis of a temperature-stable ligase that was present at levels some lo-fold above that of the wild type, presumably reflecting the plasmid copy number. The remaining plasmid, SlO, also specified a temperature-stable enzyme, but in this case the activity was present at only 80% of the wild-type level, possibly reflecting the lower stability of this plasmid as compared with H2-YEp13 (94”/, loss
in both crosses while no ts clones
served out of 500 spores analysed for each integrant, so LEU + was very closely linked to CDC17 and the S 10 and H2 plasmids had integrated at the site of the CDC17 gene.
Assays
in S5 should
after called H2-YEp13), could be compared
were detected in 300 spores from each cross. Thus the marker allowing growth at 36’ C in the integrants was closely linked to CDCI 7. To prove that the plasmid sequences were associated with the CDC17 site the original integrants were crossed to a cdcZ7-K42 leul-32 h’ strain. No recombinants were ob-
TABLE
insert purposes
from H2 (Fig. 1) was subcloned
36°C were crossed to an ade6-704 h’ strain. Random spore analysis showed that the ade6 marker freely recombined
to code for a DNA
ligase (Nasmyth, 1977), plasmids H2 and SlO should both direct the synthesis of this enzyme, while
should occur at the CDC17 locus. They were
therefore
as CDC17 is known
Finally,
If plasmids H2 and S 10 do carry the CDC17 gene, integration into the genome by homologous recombi-
I of DNA ligase in crude extracts
(A) Cells grown
at 25’C
and switched
from cdcl7 to 37’C
transformants
2 h before harvestmg
and assay
at 25’C
Ligase activity” cdcl7
Wild type
cdcl7
cdcl7
25’C
0.10
0.03
0.04
0.085
0.95
37’C
0.30
0
0
0.12
2.17
(B) Crude
extracts
prepared
from cells grown
cdcl7
[S5]
[SlO]
at 25’C
were incubated
[St01
cdcl7
[H2-YEpI
at either 25’C
or 34°C for 5 min before assaying
at 25-C
Ligase activity il Wild type
I
25’C
0.1 -
34°C
0.07
3 The assay measures with ‘*P, annealed
0.08
0.64
0
0.05
0.44
the ligation of two short oligodeoxynucleotides
[HZ-YEp13]
(15-mer and 17.mer Ml3 sequencing
on M 13 ss DNA (Barker et al., 1985). The product
The position
band and determining
1.5~mer, 0.6 ng labelled
cdcl7
0.03
contiguously
and gel electrophoresis. appropriate
cdcl7
of the product
the amount
is located
by autoradiography
of label. In this experiment
17-mer and 1.O )_tgcrude cell extract
is separated
was assayed
primers),
from unreacted
and the assay
each assay contained
one 5’ end-labelled
substrate
is quantified
by denaturation
by cutting
out the
400 ng M 13 ss DNA, 2 ng unlabelled
for 4 min and results are expressed
as fmol of substrate
ligated.
324
compared
with 60”/
non-selective
loss after ten generations
a
of
growth),
In summary,
b
c
we have cloned a gene which comple-
ments cdcl7, integrates back into the genome at the CDCI 7 locus and which directs the synthesis of a DNA ligase. It is therefore and S 10 do contain (d) Identification
clear that plasmids
H2
the CDC17 gene.
and mapping of the CDCl7
Total RNA extracted
from exponentially
to Northern
hybridisation
1.23
tran-
O-84
growing
O-57
script
cells was subjected
1.65
anal-
ysis (Fig. 2). The ~~~zdIII-~g~II fragment, common to both SlO and H2, hybridised to two RNA species of 1.6 kb and 2.8 kb (Fig. 2, lane a), Subcloning experiments (see above) had shown that CDCI 7 spans the DNA between the leftmost EcoRI and &$I1 sites (Fig. 1) and since the PstI-CIaI fragment from within this region only hybridised to the 2.8-kb transcript (Fig. 2, lane b) then this must correspond to the CDCl7 mRNA. A probe prepared from part of the 880 bp of DNA to the left of the Hind111 site in SlO (Fig. 1) only hybridised to the 1.6-kb transcript (Fig. 1, lane c) which must therefore be derived from an adjacent gene. S 1 nuclease mapping of the CDCf 7 transcript was carried out by cloning into the polylinker site of
Oe36 Fig. 3. S I
nucloasemappingofthe
5’ end and 3’ polyadenylation
site of the CDCI7 gene. Appropriate ning the 5’ and 3’ ends ofCDCI7 cloned
into the bacteriophage
restriction
fragments
vector
hll3mpl
1 (Norrander
ct al.. 1983). Total S. porn/x RNA WDSthen hybridised with an excess of ss preparations M”,,
forrnanidc.
nt&xc:ml
for
The hybrid
was digested
1 h at 30-C under standard
a neutral
blotting.
l.anc c shwvs
agarox the
at 42‘C
of this RNA in the presence with 200 units conditions
et al., 19X2), and the protected DNA fragments through
span-
(see section d and Fig. 1) wcrc
gel and single
identified 5’-protected
of SI
(Mamatis
electrophoresed by
Southern
fragment
of
550 _t 50 nt and lane b shows the sin& 3’-protecrcd fragment of 600 + 50 nt. DNA fragments of known M, arc shown in lane a, the values given being in kb.
abed M 13mpl1, the 1.6-kb EcoRI fragment and the 2.6kb CIUI fragment, which should span the termini of thegene (see section b above, and Fig. 1). Total yeast
l-65
c
le23 Fig. 2. Identification extracted
of the CDCl7
from S. porn/w. subjected
transcript.
and then trnnsferrcd
to a nitroccllulose
198).
this membrane
After cutting
hybridised
with different
Total
‘*P-labeiled
membrane into strips,
(Aves et al., each lane was
DNA probes from the S 10
clone (Fig. 1) as follows: (a) the 4.2-kb NindIII-Bg/II (b) the l.Mb
Psrl-Cl01
(c) an internal
fragment
Hi~dlll
fragment
RNA was
to agarose gel electrophoresis
fragment;
from within the CDC17 gene;
from the 880-bp DNA to the left of the
site: (d) DNA f’ragmenrs of known /M,, the values given
hcing in kb,
RNA was hybridised to ss DNA fragments of appropriate orientations, and after nuclease digestion the protected fragment of the EcoRI subclone was found to be 550 + 50 bp and that of the ClaI subclone was 600 2 50 bp (Fig. 3, .lane c and b). The orientation of the inserts in these two phage DNAs, taken together with preliminary DNA sequence analysis of part of the CDCI 7 coding region indicated that transcription initiates within the EcoRI fragment and terminates within the C/u1 fragment (Fig. 1). This would give a total transcript size [without poly(A)] of 2700 nt, which is in good agreement with the value of2800 nt obtained by Northern hybridisation analysis and consistent with a M, of 90000, which has been determined for the S. ~(~~7be ligasc subunit (G. Banks, manuscript in preparation).
325
(e) CDCl7
does not complement
We have previously
S. cerevisiae
shown that the cloned gene for
DNA ligase CDC9, from the budding siae, is expressed cdcl7 mutations
cdc9
in S. pombe
and
yeast S. cerevicomplements
(Barker and Johnston,
1983). How-
ever, neither the H2 nor S 10 clones of CDCZ 7 were able to complement
cdc9. The most
ation for this is lack of transcription transcripts Northern
could not be detected analysis.
likely explansince CDCI 7
in S. cerevisiae by
A similar situation
exists between
the S. pombe CDC2 and S. cerevisiae CDC28 genes (Beach et al., 1982b) and these failures
of comple-
mentations may simply reflect differences between the promoters of the two organisms. The identification of the CDC17 gene and its transcript should now form the basis for further studies on the regulation of CDCI 7 both in the mitotic cell cycle and in response to DNA damage.
REFERENCES Aves,
S.J., Durkacz,
quencing
A. and Nurse, control
cdcl0 “start”
mycespombe
Barker,
B., Carr,
and transcriptional
D.G. and Johnston,
a structural
P.: Cloning,
gene. EMBO J. 4
( 1985)457-463.
L.H.: Succharomtws
wreviritre
gene for DNA ligase which complcmenta
succharomJ~ce.v pomhe
Eur. J. Biochcm.
cdc17.
be-
of the Schi~[-ovtrc,~hclro49. Schko-
134 (1983)
315-319. Barker,
D.G., Johnson,
A.L. and Johnston,
assay for DNA ligase revcala in cdc9 mutants Gcnct.
L.H.: An improved
temperature-sensitive
of Scrcchawnws
activit) Mol. Gen.
cerrvivicw.
200 (1985) 458-462.
Beach, D., Durkacz,
B. and Nurse.
P.: ConstructIon
pombe gene bank
of a S&i:+
in a yeast bacterial
shuttle
vector and its use to isolate genes by complemcntation.
Mol.
sacchuromwes
Gen. Genet.
187 (1982a)
Beach, D. Durkacz, cell cycle control 300 (1982b) Johnston,
326-329.
B. and Nurse. P.: Functionally genes in budding
homologous
and fission yeast. Nature
706-709.
L.H. and Nasmyth,
cycle mutant
cwevititrr
cdl
ligaae. Nature
274
K.A.: Succharomycrr
cdc9 is defective
in DNA
(1978) 891-893. Maniatis,
T., Fritsch,
A Laboratory Spring Harbor, Nasmyth,
ACKNOWLEDGEMENTS
K.A.:
structural
We would like to thank Don Williamson cal reading of the manuscript.
for criti-
E.F. and Sambrook,
Manual.
Cloning.
Laboratory.
Cold
NY, 1982. Temperature-sensitive
lethal
mutants
in the
gene for DNA ligase in the yeast S~hi-r,srr~~lttrro-
myres pombe. Cell 12 (1977)
Norrander,
J.: Molecular
Cold Spring Harbor
J., Kempe.
11OY-I 120.
‘T. and Messing,
J.: Construction
of im-
proved M 13 vectors using ohgodeoxyribontxlcotide-directed mutagenesis. Russell,
Gene 26 (1083)
dehydrogenase ,,l~w.v /x&w. Southern,
101-106.
P. and Hall. B.D.: The primary gent
separated
of specific
sequcnccs
by gel electrophoresis.
(1Y75) 503-517. Communicated
of the alcohol Scl,i-o.st/cchrrrt,-
J. Biol. Chcm. 258 (1983) 143-149.
E.M.: Detection
fragments
structure
from the fission yeast
by K.F. Chater.
among
DNA
J. Mol. Biol. YX
321
Elscvier GENE
1518
Cloning and characterization (Recombinant
DNA;
L.H. Johnstona*,
of the Schizosacchavumyces
fission yeast;
suppressor;
promoter;
pombe DNA iigase gene CDCZ7 with Sacckarnm_vces cereviskre)
complementation
D.G. Barkera and Paul Nurseb
‘ILaboratrw.vof CeN Propagation, National Institute for Medicat Resecrrch, The Ridgewq. Mill Hill, London NW7 IAA, Tel. (01) 9593666, and ’ CeN Cj’cle Control Laborator?,. Imperial Cancer Research Fund, Lincoln k Iun Fields. Loudon WCZA 3PX (Ci~k’.J Tei. {01)2420200 (Received
July jth,
(Revision
received
(Accepted
1985) October
November
21st, 1985)
25th, 1985)
SUMMARY
The Sc~iz(~sacc~aromyces pombe CDCI 7 gene has been cloned by complementation of the cdel7 mutant coding for temperature-sensitive DNA ligase. An allele-specific suppressor active only in the presence of a high osmotic pressure was also isolated. The cloned CDCI 7 gene failed to complement the analogous DNA ligase mutation, cd&, in Saccharomyces cerevisiae, although the reverse complementation was successful [Barker and Johnston, Eur. J. Biochem. 134 (1983) 315-3191. The CDCl7 gene specifies a 2%kb transcript. __
Johnston,
INTRODUCTION
1983), and the analogous
gene CDCl7
from the fission yeast S. pombe (Nasmyth, 1977). The availability of ts mutants in these genes and of
The ubiquitous enzyme DNA ligase is required principally during DNA synthesis for the joining of Okazaki fragments and also for the repair of damaged DNA. A study of the control of expression of DNA ligase in different organisms might reveal features of cellular regulation which have been conserved during evolution. With this in mind we have initiated parallel studies into the regulation of the DNA ligase gene CDC9 from budding yeast, S. cerevisiae (Johnston and Nasmyth, 1978; Barker and
plasmid vector transformation systems for both organisms together provide a convenient approach both to cloning the genes and also to examining their heterologous expression and regulation. Following the isolation of the S. cerevisiae CDC9 gene (Barker and Johnston, 1983) we now describe the cloning and preliminary characterisation of the S. pombe CDCl7 gent.
* To whom correspondence
EXPERIMENTAL
and
reprint
requests
should
be
AND
DISCUSSION
addressed. Abbreviations:
bp, base pair(s);
types; kb, kilobase reading
plasmid-carrier
037X-I 119:X6/503.50
, S. pombe mating
or 1000 bp; nt. nucieotide(s);
frame; ss. single-stranded;
designates
h + and h
0
ORF, open
ts, temperature-sensitive:
state.
19X6 Elsevier
Science
Publishers
[ ],
(a) Cloning of CLlCZ7 A cdcf 7-K42 leui-32 strain of S. pombe was transformed (Beach et al., 1982a) with DNA from two
B.V. (Biomedical
Division)
322
clone banks, one in vector YEpl3 (Russell and Hall, 1983) and one constructed by inserting a partial Hind111 digest of chromosomal pDB262
(a positive selection
DNA
37°C after replication from the original sorbitol-agar plates. S5 tr~sformants also behaved similarly when first replicated onto minimal agar plates and
into vector
vector based upon the
bacteriophage
1. ci gene). Plates were incubated
the permissive
temperature
transformants
were replicated
grown at 25°C before transfer to YE-phloxin at 37°C. Only when replicated onto another sorbitol-
at
agar plate, which contains
of 25 “C and the resulting to yeast-extract
transformants
agar
plates containing 20 [kg phloxin B/ml YE-phloxin for further incubation at the restrictive temperature of 37°C. The phloxin stains dead cells a deep red colour
and therefore
aids the selection
did all
grow at 37 ‘C. The SS complementing
activity therefore differed from that of SlO and H2 in appearing to require high osmotic pressure for full effect; moreover,
of transfor-
it alone was alleIe-speci~c,
allele c&I 7-M75 being unaffected
mants that are able to grow at 37’ C and have a paler colour. A total of 1.5 colonies were obtained
1.2 M sorbitol,
another
by S5. Clone 55
therefore appears to be a suppressor and may be a protein which normally interacts with DNA ligase
at 37 “C
by this means, all of which showed the instability characteristic of plasmid-borne genes in yeast. Recombinant plasmid DNA extracted from three of these colonies and designated S5 and S 10 (vector Y Ep 13) and H2 (vector pDB262) was used to transform E. coli (as in Barker and Johnston, 1983). When re-isolated, each plasmid transformed S. pombe cdcl7 to growth on sorbitol-agar plates (Beach et al., 1982a) at the restrictive temperature with high frequency (about 4-6 x lO’/iig DNA). However, unlike SIO and H2 transformants, S5 transformants required some 44 h preincubation at 25’ C before the maximum number of colonies was observed at 37 ’ C, and only 2-3 T<,of these transformants were able to grow on YE-phloxin plates at
and which can partially overcome the cdc17-K42 mutation when its gene is present on a multi-copy plasmid. (b) Mapping of the CLXl7
gene
Restriction analysis (Fig. 1) and sub-cloning showed that S 10 and H2 had some 4.5 kb in common and that the CDC17 gene, possibly together with the information necessary for its expression, lies between the leftmost EcnRI site and the left BgtII site. Southern hybridisation (Southern, 1975) studies with the two probes shown in Fig. 1 confirmed that neither of these two clones had any sequence in common with S5 and that they were unrearranged
+.---+
lkb
2.4 kb Probe I
I
SSEAP I I
E
EACE
Bg
E
II
6.7 kb Probe I
I
HE I
H2
SSEAP I I III
E I
EAC E I II I
Bg
E
I
I
Bg I
C
H
I
t I
1
L
I
5’ SI Probe Fig. 1. Restriction used in Southern indicate
map ofclones hybridisation
complementing experiments
the ends of the c‘DCI7 transcript
U~irri; Bg, B@II; B, Ba/rtHi.
3’SI
cdc17.The hatched
areas represent
are shown. The two S 1mapping as determined
bq Sl nuclease
probes described mapping.
Probe
vector sequences
and the 2.4-kb and h.7-kb probes
rn Fig. 3 are also indicated.
H. HitzdIII;
E, EcoRI;
The two :~rows
S. Suil; A, Awl;
P. Purl: C.
323
compared (which
with
their
chromosomal
in S. pombe
are present
(c) Ligase synthesis
homologues
DNA
as single
copies) (not shown).
nation strain
into a cdcl7-K42
transformed
leul-32
the unrelated
h
comparative
and a stable clone from each was isolated.
These putative
integrants,
which could both grow at
plasmids,
not do so. For
the entire Hind111 fragment into YEpl3
(here-
so that all the cloned DNAs
in the same vector.
S5, SlO and HZ-YEp13,
The three
were each trans-
formed into cdcl7 and the crude extracts prepared from these transformants were assayed for levels of DNA ligase. S5 transformants possessed only the same low levels of a ts activity found with cdcl7 alone (Table I), confirming that S5 is probably a suppressor of cdcl7. In contrast, H2-Y Ep 13 directed the synthesis of a temperature-stable ligase that was present at levels some lo-fold above that of the wild type, presumably reflecting the plasmid copy number. The remaining plasmid, SlO, also specified a temperature-stable enzyme, but in this case the activity was present at only 80% of the wild-type level, possibly reflecting the lower stability of this plasmid as compared with H2-YEp13 (94”/, loss
in both crosses while no ts clones
served out of 500 spores analysed for each integrant, so LEU + was very closely linked to CDC17 and the S 10 and H2 plasmids had integrated at the site of the CDC17 gene.
Assays
in S5 should
after called H2-YEp13), could be compared
were detected in 300 spores from each cross. Thus the marker allowing growth at 36’ C in the integrants was closely linked to CDCI 7. To prove that the plasmid sequences were associated with the CDC17 site the original integrants were crossed to a cdcZ7-K42 leul-32 h’ strain. No recombinants were ob-
TABLE
insert purposes
from H2 (Fig. 1) was subcloned
36°C were crossed to an ade6-704 h’ strain. Random spore analysis showed that the ade6 marker freely recombined
to code for a DNA
ligase (Nasmyth, 1977), plasmids H2 and SlO should both direct the synthesis of this enzyme, while
should occur at the CDC17 locus. They were
therefore
as CDC17 is known
Finally,
If plasmids H2 and S 10 do carry the CDC17 gene, integration into the genome by homologous recombi-
I of DNA ligase in crude extracts
(A) Cells grown
at 25’C
and switched
from cdcl7 to 37’C
transformants
2 h before harvestmg
and assay
at 25’C
Ligase activity” cdcl7
Wild type
cdcl7
cdcl7
25’C
0.10
0.03
0.04
0.085
0.95
37’C
0.30
0
0
0.12
2.17
(B) Crude
extracts
prepared
from cells grown
cdcl7
[S5]
[SlO]
at 25’C
were incubated
[St01
cdcl7
[H2-YEpI
at either 25’C
or 34°C for 5 min before assaying
at 25-C
Ligase activity il Wild type
I
25’C
0.1 -
34°C
0.07
3 The assay measures with ‘*P, annealed
0.08
0.64
0
0.05
0.44
the ligation of two short oligodeoxynucleotides
[HZ-YEp13]
(15-mer and 17.mer Ml3 sequencing
on M 13 ss DNA (Barker et al., 1985). The product
The position
band and determining
1.5~mer, 0.6 ng labelled
cdcl7
0.03
contiguously
and gel electrophoresis. appropriate
cdcl7
of the product
the amount
is located
by autoradiography
of label. In this experiment
17-mer and 1.O )_tgcrude cell extract
is separated
was assayed
primers),
from unreacted
and the assay
each assay contained
one 5’ end-labelled
substrate
is quantified
by denaturation
by cutting
out the
400 ng M 13 ss DNA, 2 ng unlabelled
for 4 min and results are expressed
as fmol of substrate
ligated.
324
compared
with 60”/
non-selective
loss after ten generations
a
of
growth),
In summary,
b
c
we have cloned a gene which comple-
ments cdcl7, integrates back into the genome at the CDCI 7 locus and which directs the synthesis of a DNA ligase. It is therefore and S 10 do contain (d) Identification
clear that plasmids
H2
the CDC17 gene.
and mapping of the CDCl7
Total RNA extracted
from exponentially
to Northern
hybridisation
1.23
tran-
O-84
growing
O-57
script
cells was subjected
1.65
anal-
ysis (Fig. 2). The ~~~zdIII-~g~II fragment, common to both SlO and H2, hybridised to two RNA species of 1.6 kb and 2.8 kb (Fig. 2, lane a), Subcloning experiments (see above) had shown that CDCI 7 spans the DNA between the leftmost EcoRI and &$I1 sites (Fig. 1) and since the PstI-CIaI fragment from within this region only hybridised to the 2.8-kb transcript (Fig. 2, lane b) then this must correspond to the CDCl7 mRNA. A probe prepared from part of the 880 bp of DNA to the left of the Hind111 site in SlO (Fig. 1) only hybridised to the 1.6-kb transcript (Fig. 1, lane c) which must therefore be derived from an adjacent gene. S 1 nuclease mapping of the CDCf 7 transcript was carried out by cloning into the polylinker site of
Oe36 Fig. 3. S I
nucloasemappingofthe
5’ end and 3’ polyadenylation
site of the CDCI7 gene. Appropriate ning the 5’ and 3’ ends ofCDCI7 cloned
into the bacteriophage
restriction
fragments
vector
hll3mpl
1 (Norrander
ct al.. 1983). Total S. porn/x RNA WDSthen hybridised with an excess of ss preparations M”,,
forrnanidc.
nt&xc:ml
for
The hybrid
was digested
1 h at 30-C under standard
a neutral
blotting.
l.anc c shwvs
agarox the
at 42‘C
of this RNA in the presence with 200 units conditions
et al., 19X2), and the protected DNA fragments through
span-
(see section d and Fig. 1) wcrc
gel and single
identified 5’-protected
of SI
(Mamatis
electrophoresed by
Southern
fragment
of
550 _t 50 nt and lane b shows the sin& 3’-protecrcd fragment of 600 + 50 nt. DNA fragments of known M, arc shown in lane a, the values given being in kb.
abed M 13mpl1, the 1.6-kb EcoRI fragment and the 2.6kb CIUI fragment, which should span the termini of thegene (see section b above, and Fig. 1). Total yeast
l-65
c
le23 Fig. 2. Identification extracted
of the CDCl7
from S. porn/w. subjected
transcript.
and then trnnsferrcd
to a nitroccllulose
198).
this membrane
After cutting
hybridised
with different
Total
‘*P-labeiled
membrane into strips,
(Aves et al., each lane was
DNA probes from the S 10
clone (Fig. 1) as follows: (a) the 4.2-kb NindIII-Bg/II (b) the l.Mb
Psrl-Cl01
(c) an internal
fragment
Hi~dlll
fragment
RNA was
to agarose gel electrophoresis
fragment;
from within the CDC17 gene;
from the 880-bp DNA to the left of the
site: (d) DNA f’ragmenrs of known /M,, the values given
hcing in kb,
RNA was hybridised to ss DNA fragments of appropriate orientations, and after nuclease digestion the protected fragment of the EcoRI subclone was found to be 550 + 50 bp and that of the ClaI subclone was 600 2 50 bp (Fig. 3, .lane c and b). The orientation of the inserts in these two phage DNAs, taken together with preliminary DNA sequence analysis of part of the CDCI 7 coding region indicated that transcription initiates within the EcoRI fragment and terminates within the C/u1 fragment (Fig. 1). This would give a total transcript size [without poly(A)] of 2700 nt, which is in good agreement with the value of2800 nt obtained by Northern hybridisation analysis and consistent with a M, of 90000, which has been determined for the S. ~(~~7be ligasc subunit (G. Banks, manuscript in preparation).
325
(e) CDCl7
does not complement
We have previously
S. cerevisiae
shown that the cloned gene for
DNA ligase CDC9, from the budding siae, is expressed cdcl7 mutations
cdc9
in S. pombe
and
yeast S. cerevicomplements
(Barker and Johnston,
1983). How-
ever, neither the H2 nor S 10 clones of CDCZ 7 were able to complement
cdc9. The most
ation for this is lack of transcription transcripts Northern
could not be detected analysis.
likely explansince CDCI 7
in S. cerevisiae by
A similar situation
exists between
the S. pombe CDC2 and S. cerevisiae CDC28 genes (Beach et al., 1982b) and these failures
of comple-
mentations may simply reflect differences between the promoters of the two organisms. The identification of the CDC17 gene and its transcript should now form the basis for further studies on the regulation of CDCI 7 both in the mitotic cell cycle and in response to DNA damage.
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We would like to thank Don Williamson cal reading of the manuscript.
for criti-
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