Embed Size (px)
Gene, 64 (1988) 165-172
Elsevier
GEN 02329
165
Short Communications
Cloning and analysis of a yeast genomic DNA sequence capable of directing gene transcription in Escherichia cofi as well as in yeast
(Recombinant DNA; Succharomyces cerevisiue; promoters; plasmid vectors; CAT assay; primer extension;
Southern blot)
Ju Won Kwak”, Jiyoung Kim”, Ook Joon Yoo b and Moon Hi Hans
” Genetic Engineering Center, and b Department of Biological Science and Engineering, KAIST, Seoul (Korea) Tel. (02)967-8901
Received 8 June 1987
Revised 15 September 1987
Accepted 11 December 1987
Received by publisher 5 January 1988
SUMMARY
A DNA fragment was isolated from yeast genomic sequences by its ability to direct the transcription of
promoterless CmR (cat) gene in Escherichiu coli and in yeast. Nucleotide sequencing and primer extension
analysis showed that yeast DNA contains sets of consensus sequences pertaining to prokaryotic and yeast-type
promoter elements. It was designated as yeast- and E. coli-type promoter (YEPZ). Typical E. coli-type
promoter elements are found at appropriate positions: TATTTT from -12 to -7 and TTGTCC from -35 to
-30 with their spacing of 17 bp from the single mRNA start point determined by the primer extension. Analysis
of cat transcripts from yeast cells showed that the YEPI caused multiple transcription initiations at more than
20 different points that are spaced over a lOO-bp region. The DNA is composed of A + T-rich sequences and
putative TATA-like sequences are found at several places upstream from the transcription start points. Deletion
analysis showed that a 276-bp sequence between -872 and -596 from the initiating ATG codon was required
for the maximal promoter activity in yeast but not in E. coli.
Correspondence to: Dr. M.H. Han, Genetic Engineering Center,
the Korea Advanced Institute of Science and Technology,
Cheongryang P.O. Box 131, Seoul (Korea) Tel. (02)967-890 1,
ext. 3341.
ExoIII, exonuclease III; kb, kilobase or 1000 bp; nt, nucleo-
tide(s); PolIk, large (Klenow) fragment of E. coli DNA polymer-
ase I; poly(A)+ , polyadenylated; R, resistance; Trp + , trypto-
phan prototroph (phenotype); UAS, upstream activation site;
YEPI, yeast- and E. coli-type promoter; YEPGE medium, see
Abbreviations: Ap, ampicillin; bp, base pair(s); CAT, Cm acetyl
transferase; cat, gene coding for CAT; Cm, chloramphenicol;
EXPERIMENTAL AND DISCUSSION, section a.
0378-l 119/SS/$O3.50 0 1988 Elsevier Science Publishers B.V. (Biomedical Division)
INTRODUCTION EXPERIMENTAL AND DISCUSSION
Functional expression of some yeast genes in
E. coli has been reported (review, Hollenberg, 1980).
In order for the expression to occur, the tran-
scriptional machinery of the prokaryotic cell must
recognize and interact with some DNA elements
which are contained in the 5’-flanking sequences of
yeast genes or in the adjacent plasmid nucleotide
sequences. In the case of yeast HIS3 gene, a region
close to or within the yeast promoter was essential
for expression in E. coli (Struhl and Davis, 1980).
The 5’-flanking sequences of the yeast URA3 genes
were revealed to contain E. coli-type promoter se-
quences (Rose et al., 1984).
The random genomic DNA fragments of Saccha-
romyces cerevisiae were tested for their ability to
express the plasmid gene of tetracycline resistance in
E. coli (Neve et al., 1979). The frequency with which
promoter-active recombinants were found among
total recombinants was as high as 28 %. The yeast
DNA segments which are transcriptionally active in
E. coli as well as in yeast would be expected to exist
in yeast genome with significant frequencies. Except
a few cases of well-characterized yeast genes, iso-
lation and characterization of the yeast DNA
segments has been limited. As a means of searching
for such a DNA fragment in yeast genome, we have
developed promoter-probe, shuttle plasmid vectors
between S. cerevisiue and E. coli (pK15 and pKW4,
Kwak et al., 1987) utilizing the promoterless CmR
gene. The bacterial CmR (cat) gene has been reported
to be functionally expressed in yeast (Cohen et al.,
1980) and proved to be an efficient marker for both
S. cerevisiue and E. coli (Hadfield et al., 1986).
In this paper, we describe cloning and analysis of
a yeast genomic nucleotide sequence capable of
directing gene transcription in E. coli and in yeast.
Sequencing and transcriptional analysis of the yeast
genomic nucleotide sequence revealed novel features
of E. coli and yeast-type promoter regions which are
conserved in natural S. cerevisiae genome.
(a) Isolation of a yeast genomic DNA sequence
capable of directing gene transcription in Escheri-
chia coli and in yeast
A promoter-probe shuttle plasmid vector, pK15,
was derived from a yeast 2 pm-based shuttle plasmid
between yeast and E. coli, into which the bacterial
promoterless cat gene of pBR325 was inserted. In
pK15, a unique BamHI site was introduced just
upstream from the ribosome-binding, Shine-Dal-
garno sequences of the promoterless cat gene, and
utilized for cloning of random yeast genomic DNA
fragments to isolate the transcriptionally active
DNA fragments in both organisms.
Genomic DNA with high M, was prepared from
yeast cells as described (Rodriguez and Tait, 1983),
and partially digested with AluI + HueIII. The DNA
fragments in the range of 0.5-2.5 kb in size were
inserted into Bum HI-cleaved and end-filled pK 15,
and introduced into E. co/i LE392 by transfor-
mation. BamHI sites were generated at both ends of
insert DNA in recombinant plasmids. The E. coli
cells carrying promoter-inserted plasmids were se-
lected and amplified, directly, by growing the trans-
formed cells in a medium containing Ap and Cm (50
pg/ml each). Plasmid DNA was prepared from the
amplified culture and reintroduced into yeast
D13-1A (MATa, his3-532, trpl, ga12) by lithium
acetate transformation (Ito et al., 1983). Of 50 Trp +
transformants selected on SD(-trp) agar medium
(0.67% yeast nitrogen base w/o amino acids and 2%
dextrose supplemented with necessary minimal
ingredients except tryptophan), ten colonies showed
resistance to 1 mg Cm/ml in YEPGE medium (1%
yeast extract, 2% peptone, 3% glycerol and 2%
ethanol). After analysis for the inserts in the recom-
binant plasmids by BamHI digestion, it was found
that all the CmR clones turned out to contain the
identical insert of 2.2 kb in length. This is probably
due to selective amplification of a specific clone in
the initial amplification step in E. cofi and/or failure
of weaker promoter-active clones to grow in the
following selection step in yeast, under selective
pressure given by the high concentrations of Cm
used. The insert was designated as YEPI.
167
A B B
I 1
2p or i. lRPI
SE B CK II I
B
C
i i I I I 1
i t
* I
I I ‘L-------l I
AP
YEP 1 (560)
YEP 1 (840)
YEP 1 (2,200)
‘ Primer ’
‘Southern’
s C TE T A BR R RAfH H RRK B
I I I I I I
Fig. 1. Restriction map of YEpl and sequencing strategy. (A) The upper box represents the entire sequence of plasmid YEPI-pK15. The
restriction map of the 2200-bp insert was determined. AluI in parentheses was deduced from the sequence data of cur gene and used
to prepare the primer (see panel B). (B) DNA fragments used for primer extension (‘Primer’) and as probe for Southern-blot hybridization
(‘Southern’). (C) Restriction map of YEPZ (840) and sequencing strategy. The arrows indicate the direction of sequencing by the method
of Sanger et al. (1977). The abbreviations used for restriction sites are: A, Alul; B, BarnHI; C, &I; E, EcoRI; H, HueIII; K, KpnI;
P, PvuII; R, RsaI; S, SalI; T, TuqI.
16X
(b) Nucleotide sequence analysis of YEPI
A restriction map of YEPl in pK15 is shown in
Fig. 1A. To narrow down the DNA region required
for promoter activity, YEPl sequence was subcloned
using available restriction sites. Three different sizes
of DNA fragments (in bp), YEPl(560), YEPI (840)
and YEPI (2200) were tested for in vivo promoter
function by measuring CAT activities of crude
extracts prepared from cells containing each plas-
mid, where the numbers in parentheses refer to the
size of the insert starting from BumHI site upstream
from the Shine-Dalgarno sequences of cut gene. As
shown in Table I, YEPI (560) was able to promote
gene expression to the same levels as YEPl(840) and
YEPl(2200) in E. cob, while gene expression by
YEPl(560) was reduced by about five-fold in yeast
cells. The results indicate that the DNA fragment
YEPl(840) contains DNA elements that are required
for efficient initiation of transcription in E. coli and
yeast cells.
Fig. 1C shows the segments of YEPl(840) region
that were sequenced and the sequencing strategy.
The sequence determined is shown in Fig. 2. Com-
puter search for homology in the yeast gene bank
using BIONETTM system (Smith et al., 1986) identi-
TABLE 1
Expression analysis of the YEPl promoter in yeast and
Escherichia coli
Plasmids” Levels of CAT b
S. cerevisiae E. coli
tied the YEPl sequence as a new one. The tran-
scription start points in E. coli and in yeast have been
determined (see below) and are indicated as solid
circles and solid squares, respectively.
The sequence data show that TATTTT, a Pribnow
box, is contained in a position from -12 to -7, and
TTGTCC from -35 to -30 from the mRNA start
point determined in E. coli. The two hexanucleotide
elements are separated by 17 bp like typical E. coli
promoters (Hawley and McClure, 1983). Shine-
DaIgarno sequences upstream from the ATG codon
(underlined) were derived from the bacterial cat gene.
It is likely that the DNA region containing the
canonical sequences of E. coli promoters is responsi-
ble for promoting transcription initiation in E. coli.
In S. cerevisiae, transcription of YEPl-cat fusion
gene was initiated at multiple sites. TATA-like se-
quences are found at multiple positions upstream
from the transcription initiation sites. It is known
that yeast promoters often contain multiple TATA
elements within 120 nt upstream from the tran-
scription start point (Nagawa and Fink, 1985; Hahn
et al., 1985). In YEPl DNA, TATA-like sequences
are spread out over a region of up to 200 nt at far
upstream sequences in multiple copies for tran-
scription initiation in yeast. The region is composed
of extremely A + T-rich sequences and stretches of
T‘s are also found at several places. The region from
-498 to -362 is composed of up to 80% (A + T).
Nucleotide sequence analysis of YEPl reveals struc-
tural features of DNA sequence which are very
similar to those of well-characterized promoters of
E. coli genes as well as of yeast genes. Coexistence
of both types of promoter elements in YEPl sequence
makes it functional as a yeast-E. coli dual promoter.
YEP1(2200)-pK15 5.5 25
YEPI (840)-pK15 4.3 28
YEPI (560)-pK15 1.3 27
YEPl (O)-pK15 0 0
(c) Determination of transcription start points in
Escherichia cofi and in yeast
d The regions of YEPI denoted by YEPl(2200), YEPZ (840) and
YEPI(560) are represented in Fig. 1A. YEPI(pK15 is the
parental plasmid without any promoter insert.
’ For CAT assay, crude extracts were prepared from E. coli or
yeast cells using acid-washed glass beads and the CAT activities
were determined spectrophotometrically as described by
Rodriguez and Tait (1983). Total protein concentration was
determined by the method of Bradford (1976), using protein-
assay dye reagent concentrate (Bio-Rad). The specific activity of
CAT was expressed as nmol/min/mg.
Primer extension was carried out by hybridizing
RNA synthesized in vivo in E. coli harboring the
plasmid YEPl -pK15 to a labelled primer and subse-
quently treating it with reverse transcriptase. 119 bp
of AluI-PvuII fragment of CmR DNA (Fig. 1B) was
used as primer following 32P-labelling by ExoIII
digestion and PolIk filling-in as described previously
(Guo and Wu, 1983). The location of the tran-
scriptional start point was identified by analysis of
169
Sal1 -850EcoRI GT~GACACACTG~ACACCTTGAATTCTTCCAC~TATTTAAGC~TTGGCAATG~AAAGTGTGC~GGCACGG
-800 -750
GAtCGTTACTAAiCCAGTAGTTtCTGAATCCAiTCTTTCAAG~CAAACGGGA~ATGTGGGGA~TTCGACT
-700
TT~ACCAGTTCCiTTTTTTTcTiAACAGTGAAiGGATCAGTA~GCAGATAGG~GAAGTCCTC~TTAGCGG
-650 -600 B~~HI
CT~GTCTTTGGA~GAGCTTTTTiTGAAAAACTATTTCTTTTA~AGAGATCAC~TGGCATGTT~CGGGATC
-550 ------I
CC~ATATTCTATSTTGGGGGTA~GCTGTCTTAAGTTTGCCTG~AAGTATTATTGTTGTCTCA~GTGCAAT ______ -500
----T TT~CGTTTTACA~TGGGCTAAC~CAACTTAATACAACTTTTC~TTCCTTTGT~TAGAGTCTT~ATGAATG _____ -450 -400
AA~GTCTTATTC~TTTTTTTTT~TTTTTAGCAiAGTTT;A~~~TCCTTTTTT~TTCCAAGAC~~~~~~TC -- ___ _____ -350 _____
TC~TTATATTCT~TTTAGTTTC~CATGGAATT~CAAGTACAC~~~~~~CTAC~GCCTTACTT~AAAATTG _____ ______ -300 -250
CCiGTCTGGGTC~TATACTTTG~ACCCTTGTA~AGCTTTGTA~TTTTGCCAA~TGTTAATCC~GATACAA
ClaI -200
TAiCGATGGCTT~TACATAGAT~CCACTGGCC~ATTGTCCTA~GTAAGAATA~TCTAAGGAG~CTGTTTG
-150
TA~ATCAACTTTiTTTGTAAAAiTTGGCCCAGiATTTTCATA~TCAATACAG~CACGTAGTA~~GGTACC
T1 mm n = +1
ATCCGAGATTTTtAGGAGCTiiiiG:iGCTAAAiiTG
? Fig. 2. Nucleotide sequence of YEPl. The first nucleotide of the translational start codon, ATG, for the CmR (cat) gene was numbered
+ 1. The sequence between the BumHI site (-34) and the ATG (+ 1) is derived from the bacterial cal gene. Sequences bearing
resemblance to canonical promoter sequences of E. coii are boxed; they are found at expected locations in relation to the determined
transcription start point (solid circle over G). The multiple start points for mRNA transcription in yeast are denoted by three different
sizes of squares above each nucleotide, according to their transcriptional efficiencies, i.e., high, moderate, and low. Putative TATA-like
sequences for YEPI as a yeast promoter are marked with dashed lines. An upward arrow indicates the position of 3’-end of the primer
used for the primer extension experiment.
the extension product on a sequencing gel. As seen known DNAin parallel. All mRNA transcripts from
in Fig. 3A, a single, discrete, labelled DNA species YEPI in E. coli started at a G nucleotide position
149 nt in length was obtained. The start point could (-35) as denoted in Fig. 2. In E. coli, 93% of
be identified precisely by running a sequence ladder messages start with a purine nucleotide (Hawley and
obtained by enzymatic dideoxy sequencing of a McClure, 1983).
A E3
220
154
154
119
119
Fig. 3. Primer extension analysis of start points for WI transcripts from YEPI in E. co/i (A) and yeast (B). Total RNA (E. co/i) or
poly(A)’ RNA (yeast) extracted from clones harboring YEPI-introduced pK15 plasmid was used. The primer used is represented in
Fig. 1B and the 3’.end of the primer is indicated by an arrow in Fig. 2. Total RNA from E. coli cells was isolated by extraction with
hot phenol (Scherrer and Darnell, 1962). and treatment with RNasc-free DNaseI (100 units/mg) for 30 min at room temperaturepas
described by Gabain et al. (1983). RNA from yeast cells was prepared as described by Russell and Hall (1982) from cells grown in YEPGE
medium (see EXPERIMENTAL AND DISCUSSION, section a) supplemented with Cm (1 mg/ml) for the sample in lane 4.
Poly(A) + RNA was fractionated by an oligo(dT) cellulose column. The RNAs were combined with “P-labelled primer DNA and primer
extension was done as described by Henikoff et al. (1986). Lanes I and 3, primer extension done on RNA extracted from E. c,oli (lane
1) or yeast (lane 3) cells harboring the parental plasmid pKl5, as controls. Lanes 2 and 4, primer extension done on RNA extracted
from E. co/i (lane 2) or yeast (lane 4) harboring the plasmid, YEPI-pKI5. Lane M, pBR322 Hinfl fragment, “P-labelled by PolIk fill-in.
S, nucleotide sequence ladders obtained by enzymatic dideoxy sequencing of known DNAs. Numbers on either side denote the sizes
in nt.
The result of the primer extension experiment of promoter (Faye et al., 1981). The start points deter-
mRNA synthesized in vivo in yeast is shown in mined are denoted with different sizes of squares
Fig. 3B. In contrast to the mRNA initiation in E. coli, according to transcriptional efficiencies in Fig. 2.
YEPl caused multiple mRNA initiations at more Analysis of 18 yeast promoters previously done by
than 20 different points that are spaced over a lOO-bp Hahn et al. (1985) revealed two preferred sequences
region in S. cerevisiue; this appears to be quite similar for mRNA initiation in yeast, TC(G/A)A and
to the start of transcription from the yeast CYCI PuPuPyPuPu. Of the transcription start points of
171
YEPl, several correspond to the suggested se-
quences; AGTGG, T’CAA and AATE, where the
arrows indicate the position and direction of tran-
scription initiation with moderate efficiencies. But
the most frequent initiation occurred at a separate
sequence, 17 bp upstream from the ATG codon of
the CAT-coding sequence.
(d) Existence of the YEPl sequence in yeast genome
Existence of the YEPl sequence in yeast genome
is expected from the procedure used in its isolation.
It was directly demonstrated by Southern-blot
hybridization of yeast genomic DNA with the 560-bp
SclnzHI fragment of the YEPJ sequence (Fig. 1B).
The “P-labelled YEPJ DNA was hybridized to
chromosomal DNA of S. cerevisiae that had been
digested with either of the restriction endonucleases
EcoRI, C&I, or EcoRI + CfaI, whose cutting sites
are contained in YEPJ sequence. As shown in Fig. 4,
the YEPJ sequence hybridizes to at least three
different restriction fragments of yeast genomic
DNA. The double digestion of yeast genomic DNA
with EcoRI + CJaI produced the band of 612 bp
which had been expected from the sequence of YEPJ in Fig. 2. No positive bands were obtained for paren-
tal plasmid pK15 containing no insert, which was
used as a negative hybridization control. The results
suggest that YEPJ sequence was actually derived
from yeast genomic DNA and more than one copy
of YEPJ-related nucleotide sequence exist in the
S. cerevisiae genome. However, it is not known
whether the YEPJ sequence originated from a
regulatory region of a yeast gene or from another
sequence which happens to contain promoter ele-
ments such that it could be functional when it is
placed in the right position and orientation.
It was demonstrated that deletion of sequence
between nt -872 and -596 of YEPJ region caused
significant reduction of transcription initiation in
vivo as deduced from the measurement of CAT ac-
tivities (Table I). It seems likely that the upstream
sequence of YEPJ may act as an UAS, which is
found in 5’-flanking sequences of many yeast genes,
such as CYCJ, HIS4, GALl, GALJO and PHOS. A
TATA element and a UAS region are the two types
of regulatory sequences required for efficient tran-
scription of yeast genes (Guarente, 1984). The YEPJ sequence seems to contain a TATA element and a
kb 3.0
20 I.6
Fig. 4. Southern-blot analysis of yeast genomic DNA with the
YEPI sequence. Standard Southern-blot analysis was carried
out using yeast genomic DNA cleaved with the following restric-
tion endonucleases: lanes: 1, EcoRI; 2, EcoRI + Club; 3, CluI.
The DNA probe represented in Fig. 1B (B-B) was 32P-labelled
by nick-translation. Parental plasmid pK15 (with no insert) was
run (lane 4) as a negative hybridization control. Lane M is a I-kb
DNA ladder (BRL) 32P-labelled by PolIk.
UAS region which are characteristic of the regu-
latory region of yeast genes coding for mRNA. It is
unlikely that nucleotide sequences other than regula-
tory regions would contain both a TATA element
and an upstream sequence which increases the level
of transcription. Thus, on the basis of sequence
analysis and deletion mutant analysis, we suggest
that the YEPl sequence may be derived from a regu-
latory region of a yeast gene.
Detailed analysis of the YEPI sequence by a com-
bination of in vitro mutagenesis and in viva func-
tional test of mutants will be required to identify the
elements in YEPJ which are important for regulation
of transcription initiation of protein-coding genes in
yeast. It will also be interesting to know the origin
and function of the YEPJ sequence in the native state
172
in yeast genome, which remains to be further investi-
gated.
ACKNOWLEDGEMENTS
This work was supported by a grant from the
Ministry of Science and Technology of Korea. We
are grateful to Prof. Chi-Born Chae, Department of
Biochemistry, University of North Carolina, for
computer analysis of the sequence data and invalu-
able advices. Thanks are also given to Drs. Doe Sun
Kang, Dae Sil Lee, and colleagues at the Molecular
Biology Laboratory, Genetic Engineering Center,
KAIST, for helpful discussions and suggestions.
REFERENCES
Bradford, M.M.: A rapid and sensitive method for the quanti-
tation of microgram quantities of protein utilizing the prin-
ciple of protein dye binding. Anal. Biochem. 72 (1976)
248-254.
Cohen, J.D., Eccleshall, T.R., Needleman, R.B., Federoff, H.,
Buchferer, B.A. and Marmur, J.: Functional expression in
yeast of the Escherichiu coli plasmid gene coding for chlor-
amphenicol acetyhransferase. Proc. Natl. Acad. Sci. USA 77
(1980) 1078-1082.
Faye, G., Leung, D.N., Tatchell, K., Hall, B.D. and Smith, M.:
Deletion mapping of sequences essential for in vivo tran-
scription of the iso-1-cytochrome c gene. Proc. Natl. Acad.
Sci. USA 78 (1981) 2258-2262.
Gabain, A., Belasco, J.G., Schottel, J.L., Chang, A.C.Y. and
Cohen, S.N.: Decay of mRNA in Escherichia coli: investi-
gation of the fate of specific segments of transcripts. Proc.
Natl. Acad. Sci. USA 80 (1983) 653-657.
Guarente, L.: Yeast promoters: positive and negative elements.
Cell 36 (1984) 799-800.
Guo, L.H. and Wu, R.: Exonuclease III: use for DNA sequence
analysis and in specific deletions of nucleotides. Methods
Enzymol. 100 (1983) 60-96.
Hadheld, C., Cashmore, A.M. and Meacock, P.A.: An efficient
chloramphenicol-resistance marker for Saccharomyces cerevi-
siae and Escherichia coli. Gene 45 (1986) 149-158.
Hahn, S., Hoar, E.T. and Guarente, L.: Each of three ‘TATA
elements’ specifies a subset ofthe transcription initiation sites
at the CYC-I promoter of Saccharomyces cerevisiae. Proc.
Natl. Acad. Sci. USA 82 (1985) 8562-8566.
Hawley, D.K. and McClure, W.R.: Compilation and analysis of
Escherichia coli promoter DNA sequences. Nucl. Acids Res.
11 (1983) 2237-2255.
Henikoff, S., Keene, M.A., Fechtel, K. and Fristrom, J.W.: Gene
within a gene: nested Drosophila genes encode unrelated pro-
teins on opposite DNA strands. Cell 44 (1986) 33-42.
Hollenberg, C.P.: Recombinant DNA research. An update of
techniques and results. Prog. Bot. 42 (1980) 171-185.
Ito, H., Fukuda, Y., Murata, K. and Kimura, A.: Transformation
of intact yeast cells treated with alkali cations. J. Bacterial.
153 (1983) 163-168.
Kwak, J.W., Kim, J., Yoo. O.J. and Han, M.H.: A method to
isolate DNA sequences that are promoter-active in Escheri-
chia coli and in yeast. Biochem. Biophys. Res. Commun. 149
(1987) 846-851.
Nagawa, F. and Fink, G.R.: The relationship between the
‘TATA’ sequence and the transcription initiation sites at the
HIS4 gene of Saccharomyces cerevisiae. Proc. Natl. Acad. Sci.
USA 82 (1985) 8557-8561.
Neve, R.L., West, R.W. and Rodriguez, R.L.: Eukaryotic DNA
fragments which act as promoters for a plasmid gene. Nature
277 (1979) 324-325.
Rodriguez, R.L. and Tait, R.C.: Recombinant DNA Techniques:
An Introduction. Addison-Wesley, Reading, MA, 1983.
Rose, M., Grisafi, P. and Botstein, D.: Structure and function of
the yeast U&43 gene: expression in Escherichia coli. Gene 29
(1984) 113-124.
Russell, P.R. and Hall, B.D.: Structure of the Schizosaccharo-
myces pombe cytochrome c gene. Mol. Cell. Biol. 2 (1982)
106-I 16.
Sanger, F., Nicklen, S. and Coulson, A.R.: DNA sequencing with
chain terminating inhibitors. Proc. Natl. Acad. Sci. USA 74
(1977) 5463-5467.
Scherrer, K. and Darnell, J.E.: Sedimentation characteristics of
rapidly labelled RNA from HeLa cells. Biochem. Biophys.
Res. Commun. 7 (1962) 486-490.
Smith, D.H., Brutlag, D., Friedland, P. and Kedes, L.H.:
BIONETTM: national computer resource for molecular
biology. Nucl. Acids Res. 14 (1986) 17-20.
Struhl, K. and Davis, R.D.: A physical, genetic and tran-
scriptional map of the cloned his3 gene region of Saccharo-
myces cerevisiae. J. Mol. Biol. 136 (1980) 309-332.
Communicated by G. Wilcox
