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An integrative vector exploiting the transposition properties of Tn1545 for insertional mutagenesis and cloning of genes from Gram-positive bacteria
Gene, 106 (1991) 21-27 0 1991 Elsevier Science
GENE
Publishers
B.V. All rights reserved.
21
0378-l 119/91/$03.50
06061
An integrative vector exploiting the transposition properties of Tn1.545 for insertional mutagenesis and cloning of genes from Gram-positive bacteria (Recombinant
DNA;
Patrick Trieu-Cuot,
multiple
cloning
site; erythromycin
resistance;
CCcile Carlier, Claire Poyart-Salmeron
kanamycin
resistance;
electroporation;
mobilization)
* and Patrice Courvalin
Unit& des Agents Antibacttkiens, Institut Pasteur, 75724 Paris Cedex 15 (France) Received by J.-P. Lecocq: 3 June 1991 Accepted: 2 July 1991 Received at publishers: 23 July 1991
SUMMARY
We have constructed and used an integrative vector, pAT112, that takes advantage of the transposition properties (integration and excision) of transposon Tn154.5. This 4.9-kb plasmid is composed of: (i) the replication origin of pACYC 184; (ii) the attachment site (art) of Tn1545; (iii) erythromycinand kanamycin-resistance-encoding genes for selection in Gram _ of the vector from and Gram+ bacteria; and (iv) the transfer origin of IncP plasmid RK2, which allows mobilization recipients. Integration of pAT112 requires the presence of the transposon-encoded Escherichia coli to various Gram+ integrase, Int-Tn, in the new host. This vector retains the insertion specificity of the parental element Tn1545 and utilises it to carry out insertional mutagenesis, as evaluated in Enterococcusfaecafis. Since pATl12 contains the pACYC184 replicon and lacks most of the restriction sites that are commonly used for molecular cloning, a gene from a Gram+ bacterium disrupted with this vector can be recovered in E. coli by cleavage of genomic DNA, intramolecular ligation and transformation. Regeneration of the gene, by excision of pAT112, can be obtained in an E. coli strain expressing the excisionase and integrase of Tn1545. The functionality of this system was illustrated by characterization of an IS3O-like structure in the chromosome of En. fuecalis. Derivatives pATl13 and pATl14 contain ten unique cloning sites that allow screening of recombinants having DNA inserts by !x-complementation in E. coli carrying the dM 15 deletion of 1acZcr. These vectors are useful to clone and introduce foreign genes into the genomes of Gram+ bacteria.
INTRODUCTION
Conjugative transposons Tn1545 (Courvalin and Carlier, 1986) and Tn916 (Franke and Clewell, 1981) have been proven to be powerful genetic tools in a large variety of Correspondence Institut
Pasteur,
to: Dr. P. Trieu-Cuot,
Tel. (33-1)456883 * Present
Unite des Agents
Antibacteriens,
25 rue du Dr. Roux, 75724 Paris Cedex
15 (France)
Laboratoire
mycin;
ernr, gene encoding
group; int-Tn, gene encoding kb, kilobase
18; Fax (33-1)45688319.
address:
Gram + bacteria (Caparon and Scott, 1987; Gaillard et al., 1986; Ivins et al., 1988; Wooley et al., 1989). Transposition of these elements proceeds by way of excision of a free, nonreplicative, covalently closed circular intermediate that is a substrate for integration (Scott et al., 1988). The inte-
de Microbiologic,
HBpital
Enfants Malades, 149 rue de Stvres, 75730 Paris Cedex Tel. (33-1)42738842; Fax (33-1)42738844.
Necker-
15 (France)
Abbreviations: 3’-aminoglycoside Tn1545;
aa, amino acid(s); Ap, ampicillin; phosphotransferase;
replication;
bp, base pair(s);
uphA-3, gene encoding
attTnZ545,
BHI, brain heart infusion;
unit(s); Cm, chloramphenicol;
attachment
site of
cfu, colony-forming
d, deletion; En., Enterococcus; Er, erythro-
Tra,
integrase
ofTn1545;
or 1000 bp; Km, kanamycin;
Mob, mobilizable; deoxyribonucleotide; rifampicin;
ErR methyltransferase;
oriT, origin
self-transferable;
plasmid-carrier
sequence;
MCS, multiple cloning site;
Nal, nalidixic acid; nt, nucleotide(s); oligo, oligoORF, open reading frame; oriR, origin of DNA of DNA
Sm, streptomycin;
pyranoside;
Inc, incompatibility IS, insertion
XGal,
R, resistance/resistant;
Rif,
SmR; Tc, tetracycline;
5-bromo-4-chloro-3-indolyl-/?-D-galacto-
xis-Tn, gene encoding state.
transfer,
Str, chromosomal excisionase
of T&545;
[ 1, denotes
22 ration-excision system of these transposons is structurally and functionally related to that of lambdoid phages (Poyart-Salmeron et al., 1989; 1990). Excision and integration occur by reciprocal site-specific recombination
and is devoid of most of the restriction sites that are commonly used for molecular cloning. This vector is intended for insertional
mutagenesis
and
cloning
of genes
from
between nonhomologous nt sequences of 6 or 7 bp, designated overlap sequences (Caparon and Scott, 1989; Poyart-Salmeron et al., 1989; 1990). Excisive recombination requires two transposon-encoded proteins, an excisionase (Xis-Tn) and an integrase (Int-Tn), whereas Int-Tn alone is sufficient for integration (Poy~-Salmeron et al., 1990). Excision can, but does not always restore the original target sequence (Clewell et al., 1988; Poyart-Salmeron et al., 1989). In Escherichia coii, these elements excise at high frequencies when cloned on multi-copy plasmids (Courvalin and Carlier, 1987; Gawron-Burke and Clewell, 1984). Based on this property, a cloning strategy which allows regeneration of an insertionally inactivated gene from a Gram + bacterium after excision of Tn916 in E. cofi has been proposed (Gawron-Burke and Clewell, 1984). This strategy was successfully used to clone in E. coli a mutacin-associated gene from Streptococcus mutans (Cautield et al., 1990). Conjugative transposons are large DNA segments (2 16.4 kb) moderately convenient for fine-scale genetic analysis. The aim of the present study was to construct and use a small 4.9-kb integrative vector which utilizes the transposition properties (integration and excision) of Tn1545. This vector, designated pAT112, was designed to allow easy recovery in E. coli of an insertionally inactivated gene and its utility was investigated in a strain of En. faecalis. Two derivatives of pATl12 were also constructed for integration of recombinant DNA into the chromosome of Gram+ hosts.
(HP)
/ ,
/
/
/
MCS
E
SC
K
SIX
3
pATl13
1
I
1
1
1
II
sp
P
Sl
Xb
R
pATll4
I
I
I
I
I
I
Fig. 1. Structure pATll4.
of the
integrative
The components
PstI-SmaI
fragment
(a) Structure of integrative vectors pAT112, pAT113 and pATl14 The structure of integrative vectors pAT112, pATl13 and pAT114 is shown in Fig. 1. The plasmids were designed to possess the replication properties of the Gram- replicon pACYC184 and the integrative properties of the pneumococcal transposon Tn154.5 (Figs. 1 and 2). Since the three hybrids contain the origin of transfer plasmid RK2 of incompatibility group IncP, they are transferable by conjugation to various Gram+ bacteria provided that the E. coli donor contains a co-resident self-transferable IncP plasmid (Trieu-Cuot et al., 1991). They all confer resistance to Er and Km in E. cofi (selective concentrations, 150 pg Er/ml and 50 pg Km/ml), in Gram+ aerobes (8 pg Er/ml and 50 pg Km/ml) and in Gram + anaerobes (8 pg Er/ml and 500 pg Km/ml). Plasmid pATl12 has a length of 4.9 kb
conjugative
transposon
(Trieu-Cuot
et al.,
containing
1
s/x
K
SE
E
I
I
I
I
pAT1 I3 and
fragment
and Yakobson,
containing
the KmR gene
pJH I (Trieu-Cuot
fragment
frag-
1988); (ii) a 0.7-kb
(Rose,
containing
and
and Courvalin,
the erm gene of the
to as anTnI54S.
0.32-kb KpnI-EcoRl
(v)a
of Tni.545
in the attachment
Plasmid
a unique AvaI restriction
KpnI, PstI, SacI, SalI, SmaI, SphI,XbaI.
site but no sites for BarnHI,
a 0.45-kb HpaI fragment
gene of pUC19
fragment
coll~guration
and
pAT112 has a size of 4.9 kb and
contains
and pATl14,
It
’
pATl12,
HindHI, reporter
sp
Tn154.5 from Srrepfococcirs pneumoniae BM4200 1990);
the termini
hence referred
P
1
are: (i) a 1.4-kb EcoRI-XbaI
plasmid
1983); (iv) 1.3-kb BamHI-KpnI
\ \
’
ariT of RK2 (Guiney
containing
uphA- from the enterococcal
.
St
’
pACYCl84
1983); (iii) a 1.3-kb Clai-Hind111 AND DISCUSSION
Xb
vectors
of pATll2
ariR of plasmid
ment containing
RESULTS
‘\,
containing
(pATI 13) or pUCl8
To construct
EcoRI, pAT1 I3
the MCS and the 1ucZr (pATll4)
(Stewart
et ai.,
1986) was inserted at the junction of the DNA fragments carrying a&4-S and ori?? Symbols: uphA-3, gene encoding 3’-aminoglycoside phosphotransferase;
attTnl545,
attachment
site of Tn1545;
erm, gene encoding
ErR methyltransferase; lucZr, gene encoding P-galactosidase (a-peptide); MCS. multiple cloning site; oriR, origin of replication; oriT, origin of transfer. transfer
Arrows
indicate
at oriT (Grinter,
the direction
of transcripti
1981). Heavy
black triangles
and left(L) termini ofTn154.5
(attTn1545).
A,AvaI;
and of DNA depict
B, BarnHI;
right (R) C, Clc21;
E, EcoRI; H, NindIII; Hp, HpaI; K, KpnI; P, PsrI; SC. SacI; Sl, SalI; S, SmaI; Sp, SphI; X&, XbaI; X, XmaI. The restriction sites in parentheses were destroyed by DNA polymerase and fused to form the vectors.
23 Rightextremity SO GGTACCA~~TCPTGTTUTTAGTAGTAGTAC~T~TTTACTACTTATTTAC~~CTGA~~T~GACATG DR2 Du2 *
160 240
~TA~AT~TCTAG~ATCC~AT f_----
~M~TAT~~T~TTAG~~TATAC~~GT~atttt --
320
~CT~CTPATCA~CTTTAT~~TC~CCACTC~TTTACTACTMTTTACTACTTAT~TGA~TTTGA * DR2 DR2 TACGACGATTTATCCGAATTC
341
EcoRl Left Fig. 2. Nucleotide
sequence
1988) of the corresponding
extremity
of the 341-bp KpnI-EcoRI region in circular
fragment
intermediates
AGG) and the right (5’-GGTACCAGGAGCGTCTTGTTGCTTAG) Presence
of the
not shown).
1I-bp directly repeated nt sequences
Imperfect
inverted
repeats
containing
extremities
DR2 in both arms of anTnl545
and DR2 ofarrTnl.745
The DNA fragment
arrTnl545.
was obtained
by amplification
(Saiki et al.,
of Tn154.5 using oligos specific for the left (5’-GAATTCGGATTAAATCGTCGTATCAA-
are depicted
of the element.
Right and IeR extremities
was found to be essential
by horizontal
refer to integrated
for efficient integration
arrows. The 6-bp variable
of pATI
elements. (data
overlap region is shown in lower-case
letters.
+ bacteria in E. coli. Plasmids pATI and pATI are 5.4 kb in length and contain ten unique cloning sites (Fig. 1) which allow screening of derivatives containing DNA inserts by cc-complementation in E. coli carrying the dM15 deletion of 1acZa. They are therefore adapted to stable inte~ation of foreign DNA into the genome of Gram + bacteria. In each vector, a DNA fragment having two different restriction sites compatible with the MCS can be inserted in either orientation relative to that of the luc promoter. Therefore, pATll3 and pATI are transcriptional fusion vectors permitting expression in E. co/i of genes from Gram + bacteria with promoter sequences not recognized by E. coli I%o’~ RNA polymerase. Gram
(b) Mutagenesis of Entemewcus fueculis with pAT112 The genome of various En. faecalis strains was mutagenesed with pATl12 using two transfer methods (conjugation and electroporation) and two compiementation systems (Tn916 or pAT145) to provide the transposonencoded integrase Int-Tn in trans (Tables I and II). The efficiency of PAT 112 integration depended upon the combination used to deliver and rescue the vector (Table II). With both transfer methods, the inte~ation frequency of pATl12 in En. fuecalis BM4111 (Tn916) was two orders of magnitude lower than that obtained with En. faecalis BM4112 (pAT145). Overproduction of Int-Tn in cells harbouring pATI relative to those containing Tn916 is the most likely cause for this difference in integration frequency. This implies that the level of synthesis of integrase in the recipient is a rate-limiting factor for integration of pAT112. The frequencies of integration obtained following delivery of pATl12 by mating or electroporation are not comparable because they simply reflect the fact that the number of ErR electrotransformants recovered per plate was approx. 102fold greater than that of ErR transconjugants for a given recipient, BM4111 or BM4112. Finally, the presence of the
tr~sposon-encoded integrase in the new host was found to be essential for integration of PAT112 since ErR clones were not obtained when En. faecafis BM4110 (no complementation system) was used as a recipient. Taken together, these resuits indicate that obtention of numerous and nonredundant mutants in a given species will be greatly facilitated by (i) the construction of a strain harbouring pAT145, or any functionally similar replicon, and (ii) the availability of an efficient electroporation procedure for introduction of pATl12. For inte~ation of foreign DNA, transfer by conjugation of PAT 113 and PAT 114 derivatives carrying inserts from an E. coli donor to a Gram+ recipient Tn916 represents a convenient alternative. (c) Physical analysis of pATll2
harbouring
insertions in Enterococcus
faecalis In each of the four integration systems described in Table II, ten ErR clones of En. faecalis originating from the same experiment were selected for further studies. Total DNA from these clones was digested with E;coRI or Hind111 and analysed by Southern hybridization using a DNA probe specific for the erm gene to detect the restriction fragment(s) carrying pAT112. The hybridization patterns obtained in the four groups of transcipients studied indicated that, in every experiment, a single copy of pATl12 had inserted at ten different loci (Fig. 2 shows part of this analysis). (d) Stability of pAT112 insertions in Enterococcus fuecdis BM4111 In En. faecalis BM4111, resident Tn916 can catalyze integration and excision of a related element defective for these functions. We therefore studied segregation and structural stability of pAT112 insertions in this strain. Unrestricted total DNA (5 pg) from six mutants of En.~ecal~s B&I4111 with pATl12 at different loci in the
24 TABLE
I
Bacterial Strain”
strains
and plasmids
or plasmid
Relevant
properties”
Reference
Bacteria E. coli JM83
ara, A(iac-proAB), strA, @So IacZAM 15
Messing
K802N
hsdR ~,
Trieu-Cuot
DHl
F ~, recA I, endA 1) gyrA96, thi, hsdR 1I, supE44, relA I,
hsdM+, gal-, tnet ~, supE, NalR, Rip A:
(1983) et al. (1991)
Low (1968)
En. faecalis BM4110
StrR
Courvalin
BM4111
StrR, TcR; (BM41 lO::Tn916)
This paper
BM4112
KmR, StrR; (BM4110
[pATl45])
Storrs
pRK24
ApK, TcR; Tra + , Mob
’ , IncP, trpE
Thomas
and Smith (1987)
pHG327 pHG329
ApR, IacZr
but rap + )
Stewart
et al. (1986)
pAT145
KmR; pATl87-102.2-kb
pAT295
CmR; pHSG57602-kb
and Carlier
(1986)
et al. (1991)
Plasmids + (as pUCl8,
ApR, 1ucZz + (as pUCl9. but rap + )
Stewart
EcoRI fragment Sau3A
fragment
int-Tn transcribed
containing containing
from spat promoter
xis-Tn and int-Tn transcribed
Storrs
et al. (1986) et al. (1991)
from lac
promoter
Poyart-Salmeron This paper
pATl14
; oriR pACYC184, attTn1545 ErR, KmR, Mob + ; oriR pACYCl84, attTn1545, lacZa’, MCS of pUCl9 ErK, KmR, Mob + ; oriR pACYCl84, attTnl.54.5, lacZa’, MCS of pUCl8
pAT307
pATll2::2.6-kb
pAT308
pAT307QpHG327
This paper This paper
pAT309
pHG327Q2.6-kb
pATl12
ErR, KmR, Mob+
pATl13
.I Bacteria
were grown
b rap, repressor
in BHI broth
EcoRI
enterococcal
EcoRI enterococcical or agar. All incubations
of primer; spat, hybrid promoter
DNA fragment DNA fragment were carried
of the phage SPOl-26
et al. (1989)
This paper This paper
This paper out at 37°C.
early gene promoter
and the fat operator;
a, in vitro insertion;
:: in vivo insertion
(novel joint).
TABLE
II
Integration Transfer
of plasmid
pATll2
in Enterococcusfaecalis
Recipient
system
Conjugatiot+
Integration
En. fuecalis BM4110
< 10 - ‘(’
En. faecalis BM4111
4x lo-’ 1.5 X 10-7
En. faecalis BM4112 Electroporation”
En. faecalis BM41 IO
En. faecalis BM4111
4x lomh
En. faecalis BM4112
2x lo-”
.’ Values are means of three independent within one order h Filter
matings
matings
frequency”
and were reproducible
of magnitude. E. co/i JM83[pRK24+pATll2]
between
faecalis were as described
(Trieu-Cuot
and
et al., 1991) and integration
En. fre-
quency was expressed as the number of transconjugants per donor cfu after mating. Transconjugants were selected on BHI agar containing Nal (50 pg/ml)
and Er (8 pg/ml).
i_ En. faecalis cells were transformed with 2.5 pg of plasmid DNA by electroporation (Cruz-Rodz and Gilmore, 1990) using a BioRad Gene Pulser apparatus and integration frequency was expressed as the number of electrotransformants per pg of DNA per viable cell. Electrotransformants
were selected
on BHI agar containing
Er (8 pgiml).
genome was introduced by transformation into restrictiondeficient E. coli K802N and clones containing the excised vector were selected on Km. Transformants were obtained at a very low frequency with a single DNA preparation and all contained intact pATl12. Stability of pATl12 in the same enterococcal mutants was also assessed by replica plating of a minimum of 100 colonies after growth for approx. 100 generations in antibiotic-free broth. No clone susceptible to Er was found which corresponds to a frequency of pAT112 loss lower than lo- 3. Total DNA extracted from the mutants every 20 generations during this growth period was analyzed by Southern hybridization as described in section c. Migration of pATl12 from one locus to another was only observed with the En. faecalis mutant that produced excised vectors (data not shown). These results demonstrate that integrative recombination of pATl12 and related vectors in En. faecalis BM4111 can be reversible, and that the rare excision events are followed by reinsertion of the vector at a new site of the host genome. Plasmid pAT145, which does not encode Xis-Tn, is therefore more appropriate than Tn916 to obtain stable p AT 112generated mutants. In addition, this replicon can be lost
25 spontaneously
in the absence of selective pressure (data not
shown). (e) Recovery of DNA fragments after integration of pATll2 and insertion specificity of the vector Recovery in E. coli of a DNA fragment after integration of pATl12 by using its replication properties is facilitated by the fact that the vector is devoid of most of the restriction sites commonly used for cloning. To study the specificity of insertion of the vector, we cloned into E. coli various enterococcal DNA fragments following pATl12 insertion. Total DNA of twelve mutants of En. faecalis BM4111 and BM4112, six of each isolated in the same experiment, was digested with EcoRI or Hind111 to obtain the smaller pAT112 hybrid, as determined by Southern analysis (Fig. 3). Following self-ligation, DNA was introduced by transformation into E. coli K802N and clones were selected on Km and Er. The plasmid content of twelve E. coli transformants representative of the En. faecalis mutants studied was purified and the vector-target junctions were sequenced (data not shown). Integration of Tn1545 and related elements occurs by reciprocal site-specific recombination between nonhomologous regions of attTn and of the target 12345678910
kb
4lIlmb (
(
12
3
Fig. 3. Integration DNA
4
5
purified (Courvalin
and Carlier,
ferred onto a Nytran fragment intragenic 1989). The two bands digestion
8
of BM4112
1986), digested
by agarose
9
IO
kb
(
5.00
+
4.50
a
2.x5
Total
resistant
2.85
genomic
to Er were
with EcoRI (panel A) or
gel (0.8%) electrophoresis,
trans-
membrane, and hybridized with a 560-bp SspI DNA to erm labeled in vitro with 32P (Sambrook et al., in panel A, lane 6, result from incomplete
since a single band
Hind111 digestion.
7
in En. faecalis BM4112.
of pATl12
from ten electrotransformants
Hind111 (Panel B), resolved
6
14.40
Molecular
is present
in panel
sizes (kb) are indicated
EcoRI
B, lane 6, following on the right margin.
site (Poyart-Salmeron et al., 1989; 1990). Therefore, knowledge of the nt sequences of attTn1.545 in pATl12 and of the vector-target junctions enables deduction of those of the target sites prior to integration (Fig. 4). Analysis of the data revealed that the specificity of integration of pAT112 is similar in En. faecafis BM4111 and BM4112. The twelve targets contained, on each side of the recombining site, a ‘I-bp-long segment which exhibits extensive similarity with the corresponding region in attTn1545 (Fig. 4). Similar motives are present in all the Tn1545/Tn916 integration sites characterized
so far (Caillaud
and Courvalin,
1987;
Clewell et al., 1988; Caparon and Scott, 1989; PoyartSalmeron et al., 1990) indicating that pATl12 has retained the specificity of insertion of the parental element. (f) Regeneration of a DNA fragment by excision of pATl12 One of the BM4112::pAT112 mutants was resistant to low levels of Er suggesting that, in this strain, the erm gene of pAT112 is transcribed counterclockwise relative to a chromosomal promoter. This mutant was selected to illustrate the strategy proposed to regenerate a DNA fragment by excision of pATl12. Recovery in E. co/i of the enterococcal fragment containing pAT112 was obtained following EcoRI digestion. The vector-target junctions of the EcoRIgenerated pATl12 derivative, designated pAT307, were sequenced and the nt sequence of the target site before integration was deduced (Fig. 4, insertion 1). Plasmid pAT308 was then constructed by inserting the EcoRIlinearized and dephosphorylated plasmid pHG327 into the unique EcoRI site of pAT307. To recover the insertionally inactivated enterococcal gene, excision of pATll2 from pAT308 was catalyzed by providing in tram Xis-Tn and Int-Tn. To do so, pAT308 was introduced by transformation into E. coli DHI harbouring pAT295 (pHSG576Qxis-Tn + int-Tn) and clones were selected on Ap and Cm. The plasmids from eight transformants obtained independently have been purified and used to transform E. coli JM83 cells that were plated on BHI agar containing Ap and XGal. In every experiment, the plasmid content of a lac - transformant resistant to Ap and susceptible to Cm and Km was analysed by agarose gel electrophoresis following digestion with EcoRI. All clones were found to contain a single plasmid, designated pAT309, consisting of pHG327 plus the 2.6-kb fragment of En. faecalis BM4112 chromosome. Partial sequencing of the enterococcal insert in these plasmids revealed the presence of either of the two expected hexanucleotides at the excision site of pATl12 (Fig. 5) and at approximately similar ratios (5/8 vs. 3/8). Precise regeneration of the enterococcal DNA fragment occurred in all plasmids that contained the TAACAT motif. This analysis also revealed the presence of the 3’-OH terminus of an ORF having the expected location and orientation relative to erm in
26 Right extremity
Left extremity
-----
-y---f atttta
GATAATTAGAAATTTATACTTTGTTT
-Ty_-AAAAA
** ** *** I atgtta IAAAACA>$TTTGT;A~TT~~G~G l
T~CTEG~=TCGZ~TGTTAA~T~~A l
l **
l **
l
~TcG&TTTTT~A&ATTTTTTT * l* GTTACAATTGCTA%CCT~A~T~~~
*
l
**
aatata
TTATTCACTGTG;&T&T;A;T:;; ~ATTA~CCT~GGZ~~T~CT=~~T~~~ l ** AT$iTAG;~TCT%G;CTTTTTTTT
B
t**
GTAiATtiTidGZ'iiTGATGG *et* AAAATAhA&&CCSCTAGAG~T *et** l * l l AAAAACAGAXOiATTTTCCGiACAG~T
****
* ** * *
AAZATAGTATCCTTTTTATATMCG
IX
IGiAAAGAGTCTT~GGAATCMGT l **** l l ** * *t CGTTTACGGkA ~CAAACAAAA t***** t* * l
**
l
l
*t*
l
l
****
l
l
l
l
.
l
*
*
AAFAAZACCTGACGATTAACGTCAGT
*tt
t***
***
CATTATAGAGTCTTTTGTCTTTTTTT
112
AMAACAGAAAATTT&GAAC!iGT I&aat I***** * I
.
ofintegration
****
AMATTAAGAAAGAGGT;TT;&T
** **
.
. .
.
-
l
I
. . .
.
. . . . .
.
l
.
12 in En. faecalis strains BM4111 (A) and BM4112 (B) (see Table I). Sequence
ofpAT
on purified double-stranded
DNA (Sambrook
AAG) and the right (5’-CGTGAAGTATCTTCCTACAGT) relative to Int-Tn cleavage
and boxed. Horizontal
denote terminal
are indicated
of TnZ.545 as primers.
sites (Poyart-Salmeron
imperfect
by asterisks.
inverted
Blackened
determination
ofthe vector-target
et al., 1989) using oligo specific for the left (5’-GGATAAATCGTCGTATCA-
extremities
aligned with that of attTnl545 arrows
*
17
Ill
the termini of attTnl545
*
l
tagaai l **** ctttta * l * gtaata
It0
was performed
l
t;a;;g
IY
Fig. 4. Specificity
****et**
l *****
AAAAATTTCATAAAAARATCTTAAAA l **** * ** l l * l * * AAAAACAACM4AUdGCAAAGCTTAC
l
junctions
AAAAATCTAGTTATC
repeats
squares
The nt sequences
et al., 1989; 1990). Overlap
in attTn1545. denote
Identical
positions
nt, in pairwise
with a minimum
of the target
regions
sites were deduced
are presented
comparisons,
score of identity
in lower-case
between
and
letters
every target and
of eight out of twelve target
DNAs.
Tn1.545 and can be introduced into Gram+ hosts by electroporation or by mobilization from E. cofi. Integration of these plasmids requires the presence of the transposonencoded integrase in the recipient. Plasmid pATl12 lacks most of the restriction sites that are commonly used for cloning and was constructed for insertional-mutagenesis in Gram + hosts and subsequent cloning and regeneration of the mutated gene in E. coli. The functionality of this system
pAT307. This ORF was truncated by cloning and could code for the C-terminal segment of a protein that shares significant aa similarity with the corresponding moiety of the transposase of IS30 from E. coli (Dalrymple et al., 1984) (Fig. 5). This ORF is currently being further characterized. (g) Conclusions We have constructed and used integrative vectors that should facilitate genetic analysis and manipulation of a large variety of Gram+ bacteria. These vectors capitalize on the transposition properties (integration and excision) of
E. coli (IS30)
Q Y TQHELD L V A R Q Y F P K K T C LA NTNGLI * * t * t:*t: *: SSVSNQRNH KSMDFREVNQTFI 'N S N G I RRNGLP GRATTCTAACGGGATTCGGCGTMTGGACT~C~T~T~ATTTTA~~GT~TCA~~TTTATTTCCAGTGT~~TCMCGTMTCAT
En.faecalis E.
Cob
was illustrated by the characterization of an IS30-like structure in the chromosome of an En. faecalis strain. Plasmids pATl13 and pAT114, which contain ten unique restriction sites, are adapted to the introduction of foreign genes into
(IS30)
R
P
R
K
T
L
K
*t*:t
F
K
T
P
::t*
K
E
I
l
.
I
E
R
G
V
A
L
T
A
Q t
L
N t
N
100
D End
t
En.foecnlis
FLSYVQEA I P R K S L N Y RTPIEI ATTCCAAG~TCATTGAATTACAGAACACCMTT~~TATTTTT~~TATGTA~~~TTTTA~M~M~
F
En.faecalis
CAAAAAAAAAATTTATTTTTTMTTTTCTTTTTGTTMCT~CGMTTTTTT~TGTTTTTCTM~T~~~~T~M
Y
S
N
L
I End GACAAATCATMTTT
200 300
taacat
En. faecalis
400
TAAMTTMCAMCGAGTTCGTAGTATAGCACGGATTTTTTCTCATGTAAACATCATTAMTAAACA~AATTTA
AAACGTTGTTTT taaaat
En.faecalis Fig. 5. Sequence site of pATll2 1). Numbering and compared
418
TACATATTTCTCAGCTM
of an enterococcal are indicated
DNA fragment
by superscript
after integration
and subscript
lower-case
and excision ofpAT
12. The two alternative
letters, The DNA strand
is complementary
hexanucleotides
detected
to that presented
at the excision
in Fig. 4 (insertion
begins at the first nt of the EcoRI site. The deduced aa sequence of the C-terminal moiety of the putative protein encoded is presented with that of the transposase oflS30 from E. coli (Dalrymple et al., 1984). Asterisks and colons indicate identical and homologous (I-L-V-M,
D-E, R-K, Q-N, S-T and F-Y) residues,
respectively.
The aa are aligned
with the second
nt of each codon.
27 Grinter,
the genome of Gram + bacteria. These vectors are routinely used in our laboratory for complementation and expression
N.J.:
Analysis
of chromosome
mobilization
between plasmid RP4 and a fragment Plasmid
of genes in En. faecalis.
using
ofbacteriophage
hybrids
i, carrying
ISI.
5 (1981) 267-276.
lvins, B.E., Welkos, Tn916
S.L., Knudson,
G.B. and Leblanc,
in Bacillus anthracis. Infect.
mutagenesis
D.J.: Transposon Immun.
56 (1988)
176-181. Low, B.: Formation recipient strains
ACKNOWLEDGEMENTS
This work was supported Institut
by a grant (CCAR)
from the
Pasteur.
of merodiploids in matings with a class of Recof Escherichia coli K12. Proc. Nat]. Acad. Sci. USA
60 (1968) 160-167. Messing, J.: New Ml3 vectors
for cloning. Methods
Enzymol.
Poyart-Salmeron, C., Trieu-Cuot, P., Carlier, C. and Molecular characterization of two proteins involved of the conjugative
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F. and Courvalin, shuttle
P.: Nucleotide
transposon
sequence
Tnl545.
of the ends of the
Mol.
Genet.
209 (1987)
of a gene that regulates
M.G. and Scott, J.R.: Identification
expression
of M protein,
streptococci. Caparon,
the major virulence
Proc. Natl. Acad.
transposon
Tn916 involves
determinant
of group A
and insertion
mechanism.
Cell
P.W., Shah, G.R. and Hdllingshead, to inactivate
and
isolate
analysis
Bacterial.
170 (1988) 3046-3052.
Courvalin,
of termini of the conjugative
P. and Carlier, C.: Transposable P. and Carlier,
Mol. Gen. Genet. Cruz-Rodz, plasmid
multiple antibiotic
M.S.:
prokaryotic
shuttle transposon.
mobile
efficiency
introduction
of
genetic
W.: Nucleotide
element
IS30.
sequence
EMBO
of the
J. 3 (1984)
A.E. and Clewell,
resistance
transposon
of ‘conjugal’ teriol. Gaillard,
transfer
D.B.: Evidence
for a chromosome
borne
(Tn916) in Streptococcusfuecalis that is capable in the absence
of conjugative
plasmid.
J. Bac-
J.L., Berche, P. and Sansonetti,
a tool to study
the role of hemolysin
monocytogenes. Infect. Immun. inactivated
P.: Transposon
C. and
in the virulence
as
of Listeriu
D.B.:
DNA
Regeneration
fragments
of insertionally
after excision
of trans-
poson Tn916 in Escherichiu co/i: strategy for targeting and cloning genes from Gram-positive bacteria. J. Bacterial. 159 (1984) 214-221. Guiney, D.G. and Yakobson, transfer Acad.
origin
E.: Location
of the broad
and nucleotide
host range
Sci. USA 80 (1983) 3595-3598.
plasmid
sequence RK2. Proc.
Erlich,
H.A.:
phages.
Nucleic Acids Res.
S.J., Higuchi,
R., Horn,
Primer-directed
enzymatic
DNA polymerase.
E.F. and Maniatis,
Manual,
Cold Spring
T.: Molecular
2nd ed. Cold Spring Harbor
Harbor,
Scott, J.R., Kirchman,
Science
Cloning.
Laboratory
A
Press,
NY, 1989. P. and Caparon,
of the conjugative
Stewart,
G.S.A.B.,
Storrs,
M.G.: An intermediate
transposon
Lubinsky-Minsk,
in trans-
Tn916. Proc. Natl. Acad. Sci.
Plasmid
Conjugative teriol. Thomas,
ofthe Nat].
S., Jackson,
a pBR322 copy number
C.G., Cassel,
A. and
of pUC8 for cloning and
15 (1986) 172-181.
M.J., Poyart-Salmeron, transposition
C., Trieu-Cuot, ofTn916
P. and Courvalin,
requires
of the transposon-encoded
P.:
the excisive and integraintegrase
Int-Tn.
J. Bac-
173 (1991) 4347-4352. C.M., and Smith, CA.: Incompatibility
group P plasmids:
and use in genetic manipulation.
gen-
Annu. Rev. Micro-
biol. 41 (1987) 77-101. Trieu-Cuot,
P.
and
Courvalin,
P.:
Nucleotide
Sfreptococcus faecalis gene encoding Trieu-Cuot,
otide sequence Trieu-Cuot, Shuttle
Tn1545.
vectors
bacteria. Wooley,
of
the
phos-
resistance
P.: Nucle-
gene of the conjugative
Acids Res. 18 (1990) 3660.
C., Poyart-Salmeron, a multiple
C. and
cloning
Courvalin,
site and a lucZr
P.: gene
of DNA from Escherichia coli to Gram-positive
102 (1991) 99-104.
R.C., Pennock,
Transfer
Nucleic
containing
transfer
Gene
C., Carlier, C. and Courvalin,
of the erythromycin
P., Carlier,
for conjugal
sequence
the 3’5”-aminoglycoside
type III. Gene 23 (1983) 331-341.
P., Poyart-Salmeron,
transposon
52 (1986) 50-55.
Clewell,
streptococcal
mutagenesis
Stoffel, S., Scharf,
and
J., Fritsch,
photransferase
145 (1981) 494-502.
Gawron-Burke,
Sambrook,
etics, evolution,
2145-2149. Franke,
of lambddid
of pACYC184.
of DNA with a thermostable
tive activities
224 (1990) 152-154.
P. and Arber,
sequence
D.H.,
K.B.
Kuhn, J.: pHG165:
Enterococcus fuecalis by electropo-
DNA into glycine treated B., Caspers,
Mullis,
expression.
High
to those
P.: The Tn1545 is
USA 85 (1988) 4809-4813.
resistance
205 (1986) 291-297.
C.: Tn154.5: a conjugative
Mol. Gen. Genet.
Dalrymple,
C.:
Tn916. J.
206 (1987) 259-264.
A.L. and Gilmore,
ration.
G.T.,
Laboratory
transposon
related
transposon
4 (1990) 1513-1521.
Rose, R.E.: The nucleotide
position
in Streptococcus pneumoniae. Mol. Gen. Genet. Courvalin,
gene from
58 (1990) 4126-4135.
S.E., Ike, Y., Jones, J.M. and Gawron-Burke,
Sequence
C. and Courvalin,
239 (1988) 487-494.
S.K.: Use of transposon
a mutacin-associated
Streptococcus murans. J. Bacterial. Clewell, D.B., Flanagan,
and functionally
amplification
59 (1989) 1027-1034. Tn916
P., Carlier,
system of the conjugative
Mol. Microbial.
with other site-
EMBO J. 8 (1989) 2425-2433.
C., Trieu-Cuot,
integration-excision
Saiki, R.K., Gelfand,
of the conjugative
a novel recombination
Tn1.545: homologies
Courvalin, P.: in the excision
16 (1988) 355.
Sci. USA 84 (1987) 8677-8681.
M.G. and Scott, J.R.: Excision
Cautield,
Poyart-Salmeron, structurally
110-115. Caparon,
transposon
specific recombinases.
conjugative
lOl(l983)
20-78.
ofTnlS45
22 (1989) 169-174.
A., Ashton,
R.J., Davies,
A. and Young,
M.:
and Tn916 to Clostridiumacetobutylicum. Plasmid
GENE
Publishers
B.V. All rights reserved.
21
0378-l 119/91/$03.50
06061
An integrative vector exploiting the transposition properties of Tn1.545 for insertional mutagenesis and cloning of genes from Gram-positive bacteria (Recombinant
DNA;
Patrick Trieu-Cuot,
multiple
cloning
site; erythromycin
resistance;
CCcile Carlier, Claire Poyart-Salmeron
kanamycin
resistance;
electroporation;
mobilization)
* and Patrice Courvalin
Unit& des Agents Antibacttkiens, Institut Pasteur, 75724 Paris Cedex 15 (France) Received by J.-P. Lecocq: 3 June 1991 Accepted: 2 July 1991 Received at publishers: 23 July 1991
SUMMARY
We have constructed and used an integrative vector, pAT112, that takes advantage of the transposition properties (integration and excision) of transposon Tn154.5. This 4.9-kb plasmid is composed of: (i) the replication origin of pACYC 184; (ii) the attachment site (art) of Tn1545; (iii) erythromycinand kanamycin-resistance-encoding genes for selection in Gram _ of the vector from and Gram+ bacteria; and (iv) the transfer origin of IncP plasmid RK2, which allows mobilization recipients. Integration of pAT112 requires the presence of the transposon-encoded Escherichia coli to various Gram+ integrase, Int-Tn, in the new host. This vector retains the insertion specificity of the parental element Tn1545 and utilises it to carry out insertional mutagenesis, as evaluated in Enterococcusfaecafis. Since pATl12 contains the pACYC184 replicon and lacks most of the restriction sites that are commonly used for molecular cloning, a gene from a Gram+ bacterium disrupted with this vector can be recovered in E. coli by cleavage of genomic DNA, intramolecular ligation and transformation. Regeneration of the gene, by excision of pAT112, can be obtained in an E. coli strain expressing the excisionase and integrase of Tn1545. The functionality of this system was illustrated by characterization of an IS3O-like structure in the chromosome of En. fuecalis. Derivatives pATl13 and pATl14 contain ten unique cloning sites that allow screening of recombinants having DNA inserts by !x-complementation in E. coli carrying the dM 15 deletion of 1acZcr. These vectors are useful to clone and introduce foreign genes into the genomes of Gram+ bacteria.
INTRODUCTION
Conjugative transposons Tn1545 (Courvalin and Carlier, 1986) and Tn916 (Franke and Clewell, 1981) have been proven to be powerful genetic tools in a large variety of Correspondence Institut
Pasteur,
to: Dr. P. Trieu-Cuot,
Tel. (33-1)456883 * Present
Unite des Agents
Antibacteriens,
25 rue du Dr. Roux, 75724 Paris Cedex
15 (France)
Laboratoire
mycin;
ernr, gene encoding
group; int-Tn, gene encoding kb, kilobase
18; Fax (33-1)45688319.
address:
Gram + bacteria (Caparon and Scott, 1987; Gaillard et al., 1986; Ivins et al., 1988; Wooley et al., 1989). Transposition of these elements proceeds by way of excision of a free, nonreplicative, covalently closed circular intermediate that is a substrate for integration (Scott et al., 1988). The inte-
de Microbiologic,
HBpital
Enfants Malades, 149 rue de Stvres, 75730 Paris Cedex Tel. (33-1)42738842; Fax (33-1)42738844.
Necker-
15 (France)
Abbreviations: 3’-aminoglycoside Tn1545;
aa, amino acid(s); Ap, ampicillin; phosphotransferase;
replication;
bp, base pair(s);
uphA-3, gene encoding
attTnZ545,
BHI, brain heart infusion;
unit(s); Cm, chloramphenicol;
attachment
site of
cfu, colony-forming
d, deletion; En., Enterococcus; Er, erythro-
Tra,
integrase
ofTn1545;
or 1000 bp; Km, kanamycin;
Mob, mobilizable; deoxyribonucleotide; rifampicin;
ErR methyltransferase;
oriT, origin
self-transferable;
plasmid-carrier
sequence;
MCS, multiple cloning site;
Nal, nalidixic acid; nt, nucleotide(s); oligo, oligoORF, open reading frame; oriR, origin of DNA of DNA
Sm, streptomycin;
pyranoside;
Inc, incompatibility IS, insertion
XGal,
R, resistance/resistant;
Rif,
SmR; Tc, tetracycline;
5-bromo-4-chloro-3-indolyl-/?-D-galacto-
xis-Tn, gene encoding state.
transfer,
Str, chromosomal excisionase
of T&545;
[ 1, denotes
22 ration-excision system of these transposons is structurally and functionally related to that of lambdoid phages (Poyart-Salmeron et al., 1989; 1990). Excision and integration occur by reciprocal site-specific recombination
and is devoid of most of the restriction sites that are commonly used for molecular cloning. This vector is intended for insertional
mutagenesis
and
cloning
of genes
from
between nonhomologous nt sequences of 6 or 7 bp, designated overlap sequences (Caparon and Scott, 1989; Poyart-Salmeron et al., 1989; 1990). Excisive recombination requires two transposon-encoded proteins, an excisionase (Xis-Tn) and an integrase (Int-Tn), whereas Int-Tn alone is sufficient for integration (Poy~-Salmeron et al., 1990). Excision can, but does not always restore the original target sequence (Clewell et al., 1988; Poyart-Salmeron et al., 1989). In Escherichia coii, these elements excise at high frequencies when cloned on multi-copy plasmids (Courvalin and Carlier, 1987; Gawron-Burke and Clewell, 1984). Based on this property, a cloning strategy which allows regeneration of an insertionally inactivated gene from a Gram + bacterium after excision of Tn916 in E. cofi has been proposed (Gawron-Burke and Clewell, 1984). This strategy was successfully used to clone in E. coli a mutacin-associated gene from Streptococcus mutans (Cautield et al., 1990). Conjugative transposons are large DNA segments (2 16.4 kb) moderately convenient for fine-scale genetic analysis. The aim of the present study was to construct and use a small 4.9-kb integrative vector which utilizes the transposition properties (integration and excision) of Tn1545. This vector, designated pAT112, was designed to allow easy recovery in E. coli of an insertionally inactivated gene and its utility was investigated in a strain of En. faecalis. Two derivatives of pATl12 were also constructed for integration of recombinant DNA into the chromosome of Gram+ hosts.
(HP)
/ ,
/
/
/
MCS
E
SC
K
SIX
3
pATl13
1
I
1
1
1
II
sp
P
Sl
Xb
R
pATll4
I
I
I
I
I
I
Fig. 1. Structure pATll4.
of the
integrative
The components
PstI-SmaI
fragment
(a) Structure of integrative vectors pAT112, pAT113 and pATl14 The structure of integrative vectors pAT112, pATl13 and pAT114 is shown in Fig. 1. The plasmids were designed to possess the replication properties of the Gram- replicon pACYC184 and the integrative properties of the pneumococcal transposon Tn154.5 (Figs. 1 and 2). Since the three hybrids contain the origin of transfer plasmid RK2 of incompatibility group IncP, they are transferable by conjugation to various Gram+ bacteria provided that the E. coli donor contains a co-resident self-transferable IncP plasmid (Trieu-Cuot et al., 1991). They all confer resistance to Er and Km in E. cofi (selective concentrations, 150 pg Er/ml and 50 pg Km/ml), in Gram+ aerobes (8 pg Er/ml and 50 pg Km/ml) and in Gram + anaerobes (8 pg Er/ml and 500 pg Km/ml). Plasmid pATl12 has a length of 4.9 kb
conjugative
transposon
(Trieu-Cuot
et al.,
containing
1
s/x
K
SE
E
I
I
I
I
pAT1 I3 and
fragment
and Yakobson,
containing
the KmR gene
pJH I (Trieu-Cuot
fragment
frag-
1988); (ii) a 0.7-kb
(Rose,
containing
and
and Courvalin,
the erm gene of the
to as anTnI54S.
0.32-kb KpnI-EcoRl
(v)a
of Tni.545
in the attachment
Plasmid
a unique AvaI restriction
KpnI, PstI, SacI, SalI, SmaI, SphI,XbaI.
site but no sites for BarnHI,
a 0.45-kb HpaI fragment
gene of pUC19
fragment
coll~guration
and
pAT112 has a size of 4.9 kb and
contains
and pATl14,
It
’
pATl12,
HindHI, reporter
sp
Tn154.5 from Srrepfococcirs pneumoniae BM4200 1990);
the termini
hence referred
P
1
are: (i) a 1.4-kb EcoRI-XbaI
plasmid
1983); (iv) 1.3-kb BamHI-KpnI
\ \
’
ariT of RK2 (Guiney
containing
uphA- from the enterococcal
.
St
’
pACYCl84
1983); (iii) a 1.3-kb Clai-Hind111 AND DISCUSSION
Xb
vectors
of pATll2
ariR of plasmid
ment containing
RESULTS
‘\,
containing
(pATI 13) or pUCl8
To construct
EcoRI, pAT1 I3
the MCS and the 1ucZr (pATll4)
(Stewart
et ai.,
1986) was inserted at the junction of the DNA fragments carrying a&4-S and ori?? Symbols: uphA-3, gene encoding 3’-aminoglycoside phosphotransferase;
attTnl545,
attachment
site of Tn1545;
erm, gene encoding
ErR methyltransferase; lucZr, gene encoding P-galactosidase (a-peptide); MCS. multiple cloning site; oriR, origin of replication; oriT, origin of transfer. transfer
Arrows
indicate
at oriT (Grinter,
the direction
of transcripti
1981). Heavy
black triangles
and left(L) termini ofTn154.5
(attTn1545).
A,AvaI;
and of DNA depict
B, BarnHI;
right (R) C, Clc21;
E, EcoRI; H, NindIII; Hp, HpaI; K, KpnI; P, PsrI; SC. SacI; Sl, SalI; S, SmaI; Sp, SphI; X&, XbaI; X, XmaI. The restriction sites in parentheses were destroyed by DNA polymerase and fused to form the vectors.
23 Rightextremity SO GGTACCA~~TCPTGTTUTTAGTAGTAGTAC~T~TTTACTACTTATTTAC~~CTGA~~T~GACATG DR2 Du2 *
160 240
~TA~AT~TCTAG~ATCC~AT f_----
~M~TAT~~T~TTAG~~TATAC~~GT~atttt --
320
~CT~CTPATCA~CTTTAT~~TC~CCACTC~TTTACTACTMTTTACTACTTAT~TGA~TTTGA * DR2 DR2 TACGACGATTTATCCGAATTC
341
EcoRl Left Fig. 2. Nucleotide
sequence
1988) of the corresponding
extremity
of the 341-bp KpnI-EcoRI region in circular
fragment
intermediates
AGG) and the right (5’-GGTACCAGGAGCGTCTTGTTGCTTAG) Presence
of the
not shown).
1I-bp directly repeated nt sequences
Imperfect
inverted
repeats
containing
extremities
DR2 in both arms of anTnl545
and DR2 ofarrTnl.745
The DNA fragment
arrTnl545.
was obtained
by amplification
(Saiki et al.,
of Tn154.5 using oligos specific for the left (5’-GAATTCGGATTAAATCGTCGTATCAA-
are depicted
of the element.
Right and IeR extremities
was found to be essential
by horizontal
refer to integrated
for efficient integration
arrows. The 6-bp variable
of pATI
elements. (data
overlap region is shown in lower-case
letters.
+ bacteria in E. coli. Plasmids pATI and pATI are 5.4 kb in length and contain ten unique cloning sites (Fig. 1) which allow screening of derivatives containing DNA inserts by cc-complementation in E. coli carrying the dM15 deletion of 1acZa. They are therefore adapted to stable inte~ation of foreign DNA into the genome of Gram + bacteria. In each vector, a DNA fragment having two different restriction sites compatible with the MCS can be inserted in either orientation relative to that of the luc promoter. Therefore, pATll3 and pATI are transcriptional fusion vectors permitting expression in E. co/i of genes from Gram + bacteria with promoter sequences not recognized by E. coli I%o’~ RNA polymerase. Gram
(b) Mutagenesis of Entemewcus fueculis with pAT112 The genome of various En. faecalis strains was mutagenesed with pATl12 using two transfer methods (conjugation and electroporation) and two compiementation systems (Tn916 or pAT145) to provide the transposonencoded integrase Int-Tn in trans (Tables I and II). The efficiency of PAT 112 integration depended upon the combination used to deliver and rescue the vector (Table II). With both transfer methods, the inte~ation frequency of pATl12 in En. fuecalis BM4111 (Tn916) was two orders of magnitude lower than that obtained with En. faecalis BM4112 (pAT145). Overproduction of Int-Tn in cells harbouring pATI relative to those containing Tn916 is the most likely cause for this difference in integration frequency. This implies that the level of synthesis of integrase in the recipient is a rate-limiting factor for integration of pAT112. The frequencies of integration obtained following delivery of pATl12 by mating or electroporation are not comparable because they simply reflect the fact that the number of ErR electrotransformants recovered per plate was approx. 102fold greater than that of ErR transconjugants for a given recipient, BM4111 or BM4112. Finally, the presence of the
tr~sposon-encoded integrase in the new host was found to be essential for integration of PAT112 since ErR clones were not obtained when En. faecafis BM4110 (no complementation system) was used as a recipient. Taken together, these resuits indicate that obtention of numerous and nonredundant mutants in a given species will be greatly facilitated by (i) the construction of a strain harbouring pAT145, or any functionally similar replicon, and (ii) the availability of an efficient electroporation procedure for introduction of pATl12. For inte~ation of foreign DNA, transfer by conjugation of PAT 113 and PAT 114 derivatives carrying inserts from an E. coli donor to a Gram+ recipient Tn916 represents a convenient alternative. (c) Physical analysis of pATll2
harbouring
insertions in Enterococcus
faecalis In each of the four integration systems described in Table II, ten ErR clones of En. faecalis originating from the same experiment were selected for further studies. Total DNA from these clones was digested with E;coRI or Hind111 and analysed by Southern hybridization using a DNA probe specific for the erm gene to detect the restriction fragment(s) carrying pAT112. The hybridization patterns obtained in the four groups of transcipients studied indicated that, in every experiment, a single copy of pATl12 had inserted at ten different loci (Fig. 2 shows part of this analysis). (d) Stability of pAT112 insertions in Enterococcus fuecdis BM4111 In En. faecalis BM4111, resident Tn916 can catalyze integration and excision of a related element defective for these functions. We therefore studied segregation and structural stability of pAT112 insertions in this strain. Unrestricted total DNA (5 pg) from six mutants of En.~ecal~s B&I4111 with pATl12 at different loci in the
24 TABLE
I
Bacterial Strain”
strains
and plasmids
or plasmid
Relevant
properties”
Reference
Bacteria E. coli JM83
ara, A(iac-proAB), strA, @So IacZAM 15
Messing
K802N
hsdR ~,
Trieu-Cuot
DHl
F ~, recA I, endA 1) gyrA96, thi, hsdR 1I, supE44, relA I,
hsdM+, gal-, tnet ~, supE, NalR, Rip A:
(1983) et al. (1991)
Low (1968)
En. faecalis BM4110
StrR
Courvalin
BM4111
StrR, TcR; (BM41 lO::Tn916)
This paper
BM4112
KmR, StrR; (BM4110
[pATl45])
Storrs
pRK24
ApK, TcR; Tra + , Mob
’ , IncP, trpE
Thomas
and Smith (1987)
pHG327 pHG329
ApR, IacZr
but rap + )
Stewart
et al. (1986)
pAT145
KmR; pATl87-102.2-kb
pAT295
CmR; pHSG57602-kb
and Carlier
(1986)
et al. (1991)
Plasmids + (as pUCl8,
ApR, 1ucZz + (as pUCl9. but rap + )
Stewart
EcoRI fragment Sau3A
fragment
int-Tn transcribed
containing containing
from spat promoter
xis-Tn and int-Tn transcribed
Storrs
et al. (1986) et al. (1991)
from lac
promoter
Poyart-Salmeron This paper
pATl14
; oriR pACYC184, attTn1545 ErR, KmR, Mob + ; oriR pACYCl84, attTn1545, lacZa’, MCS of pUCl9 ErK, KmR, Mob + ; oriR pACYCl84, attTnl.54.5, lacZa’, MCS of pUCl8
pAT307
pATll2::2.6-kb
pAT308
pAT307QpHG327
This paper This paper
pAT309
pHG327Q2.6-kb
pATl12
ErR, KmR, Mob+
pATl13
.I Bacteria
were grown
b rap, repressor
in BHI broth
EcoRI
enterococcal
EcoRI enterococcical or agar. All incubations
of primer; spat, hybrid promoter
DNA fragment DNA fragment were carried
of the phage SPOl-26
et al. (1989)
This paper This paper
This paper out at 37°C.
early gene promoter
and the fat operator;
a, in vitro insertion;
:: in vivo insertion
(novel joint).
TABLE
II
Integration Transfer
of plasmid
pATll2
in Enterococcusfaecalis
Recipient
system
Conjugatiot+
Integration
En. fuecalis BM4110
< 10 - ‘(’
En. faecalis BM4111
4x lo-’ 1.5 X 10-7
En. faecalis BM4112 Electroporation”
En. faecalis BM41 IO
En. faecalis BM4111
4x lomh
En. faecalis BM4112
2x lo-”
.’ Values are means of three independent within one order h Filter
matings
matings
frequency”
and were reproducible
of magnitude. E. co/i JM83[pRK24+pATll2]
between
faecalis were as described
(Trieu-Cuot
and
et al., 1991) and integration
En. fre-
quency was expressed as the number of transconjugants per donor cfu after mating. Transconjugants were selected on BHI agar containing Nal (50 pg/ml)
and Er (8 pg/ml).
i_ En. faecalis cells were transformed with 2.5 pg of plasmid DNA by electroporation (Cruz-Rodz and Gilmore, 1990) using a BioRad Gene Pulser apparatus and integration frequency was expressed as the number of electrotransformants per pg of DNA per viable cell. Electrotransformants
were selected
on BHI agar containing
Er (8 pgiml).
genome was introduced by transformation into restrictiondeficient E. coli K802N and clones containing the excised vector were selected on Km. Transformants were obtained at a very low frequency with a single DNA preparation and all contained intact pATl12. Stability of pATl12 in the same enterococcal mutants was also assessed by replica plating of a minimum of 100 colonies after growth for approx. 100 generations in antibiotic-free broth. No clone susceptible to Er was found which corresponds to a frequency of pAT112 loss lower than lo- 3. Total DNA extracted from the mutants every 20 generations during this growth period was analyzed by Southern hybridization as described in section c. Migration of pATl12 from one locus to another was only observed with the En. faecalis mutant that produced excised vectors (data not shown). These results demonstrate that integrative recombination of pATl12 and related vectors in En. faecalis BM4111 can be reversible, and that the rare excision events are followed by reinsertion of the vector at a new site of the host genome. Plasmid pAT145, which does not encode Xis-Tn, is therefore more appropriate than Tn916 to obtain stable p AT 112generated mutants. In addition, this replicon can be lost
25 spontaneously
in the absence of selective pressure (data not
shown). (e) Recovery of DNA fragments after integration of pATll2 and insertion specificity of the vector Recovery in E. coli of a DNA fragment after integration of pATl12 by using its replication properties is facilitated by the fact that the vector is devoid of most of the restriction sites commonly used for cloning. To study the specificity of insertion of the vector, we cloned into E. coli various enterococcal DNA fragments following pATl12 insertion. Total DNA of twelve mutants of En. faecalis BM4111 and BM4112, six of each isolated in the same experiment, was digested with EcoRI or Hind111 to obtain the smaller pAT112 hybrid, as determined by Southern analysis (Fig. 3). Following self-ligation, DNA was introduced by transformation into E. coli K802N and clones were selected on Km and Er. The plasmid content of twelve E. coli transformants representative of the En. faecalis mutants studied was purified and the vector-target junctions were sequenced (data not shown). Integration of Tn1545 and related elements occurs by reciprocal site-specific recombination between nonhomologous regions of attTn and of the target 12345678910
kb
4lIlmb (
(
12
3
Fig. 3. Integration DNA
4
5
purified (Courvalin
and Carlier,
ferred onto a Nytran fragment intragenic 1989). The two bands digestion
8
of BM4112
1986), digested
by agarose
9
IO
kb
(
5.00
+
4.50
a
2.x5
Total
resistant
2.85
genomic
to Er were
with EcoRI (panel A) or
gel (0.8%) electrophoresis,
trans-
membrane, and hybridized with a 560-bp SspI DNA to erm labeled in vitro with 32P (Sambrook et al., in panel A, lane 6, result from incomplete
since a single band
Hind111 digestion.
7
in En. faecalis BM4112.
of pATl12
from ten electrotransformants
Hind111 (Panel B), resolved
6
14.40
Molecular
is present
in panel
sizes (kb) are indicated
EcoRI
B, lane 6, following on the right margin.
site (Poyart-Salmeron et al., 1989; 1990). Therefore, knowledge of the nt sequences of attTn1.545 in pATl12 and of the vector-target junctions enables deduction of those of the target sites prior to integration (Fig. 4). Analysis of the data revealed that the specificity of integration of pAT112 is similar in En. faecafis BM4111 and BM4112. The twelve targets contained, on each side of the recombining site, a ‘I-bp-long segment which exhibits extensive similarity with the corresponding region in attTn1545 (Fig. 4). Similar motives are present in all the Tn1545/Tn916 integration sites characterized
so far (Caillaud
and Courvalin,
1987;
Clewell et al., 1988; Caparon and Scott, 1989; PoyartSalmeron et al., 1990) indicating that pATl12 has retained the specificity of insertion of the parental element. (f) Regeneration of a DNA fragment by excision of pATl12 One of the BM4112::pAT112 mutants was resistant to low levels of Er suggesting that, in this strain, the erm gene of pAT112 is transcribed counterclockwise relative to a chromosomal promoter. This mutant was selected to illustrate the strategy proposed to regenerate a DNA fragment by excision of pATl12. Recovery in E. co/i of the enterococcal fragment containing pAT112 was obtained following EcoRI digestion. The vector-target junctions of the EcoRIgenerated pATl12 derivative, designated pAT307, were sequenced and the nt sequence of the target site before integration was deduced (Fig. 4, insertion 1). Plasmid pAT308 was then constructed by inserting the EcoRIlinearized and dephosphorylated plasmid pHG327 into the unique EcoRI site of pAT307. To recover the insertionally inactivated enterococcal gene, excision of pATll2 from pAT308 was catalyzed by providing in tram Xis-Tn and Int-Tn. To do so, pAT308 was introduced by transformation into E. coli DHI harbouring pAT295 (pHSG576Qxis-Tn + int-Tn) and clones were selected on Ap and Cm. The plasmids from eight transformants obtained independently have been purified and used to transform E. coli JM83 cells that were plated on BHI agar containing Ap and XGal. In every experiment, the plasmid content of a lac - transformant resistant to Ap and susceptible to Cm and Km was analysed by agarose gel electrophoresis following digestion with EcoRI. All clones were found to contain a single plasmid, designated pAT309, consisting of pHG327 plus the 2.6-kb fragment of En. faecalis BM4112 chromosome. Partial sequencing of the enterococcal insert in these plasmids revealed the presence of either of the two expected hexanucleotides at the excision site of pATl12 (Fig. 5) and at approximately similar ratios (5/8 vs. 3/8). Precise regeneration of the enterococcal DNA fragment occurred in all plasmids that contained the TAACAT motif. This analysis also revealed the presence of the 3’-OH terminus of an ORF having the expected location and orientation relative to erm in
26 Right extremity
Left extremity
-----
-y---f atttta
GATAATTAGAAATTTATACTTTGTTT
-Ty_-AAAAA
** ** *** I atgtta IAAAACA>$TTTGT;A~TT~~G~G l
T~CTEG~=TCGZ~TGTTAA~T~~A l
l **
l **
l
~TcG&TTTTT~A&ATTTTTTT * l* GTTACAATTGCTA%CCT~A~T~~~
*
l
**
aatata
TTATTCACTGTG;&T&T;A;T:;; ~ATTA~CCT~GGZ~~T~CT=~~T~~~ l ** AT$iTAG;~TCT%G;CTTTTTTTT
B
t**
GTAiATtiTidGZ'iiTGATGG *et* AAAATAhA&&CCSCTAGAG~T *et** l * l l AAAAACAGAXOiATTTTCCGiACAG~T
****
* ** * *
AAZATAGTATCCTTTTTATATMCG
IX
IGiAAAGAGTCTT~GGAATCMGT l **** l l ** * *t CGTTTACGGkA ~CAAACAAAA t***** t* * l
**
l
l
*t*
l
l
****
l
l
l
l
.
l
*
*
AAFAAZACCTGACGATTAACGTCAGT
*tt
t***
***
CATTATAGAGTCTTTTGTCTTTTTTT
112
AMAACAGAAAATTT&GAAC!iGT I&aat I***** * I
.
ofintegration
****
AMATTAAGAAAGAGGT;TT;&T
** **
.
. .
.
-
l
I
. . .
.
. . . . .
.
l
.
12 in En. faecalis strains BM4111 (A) and BM4112 (B) (see Table I). Sequence
ofpAT
on purified double-stranded
DNA (Sambrook
AAG) and the right (5’-CGTGAAGTATCTTCCTACAGT) relative to Int-Tn cleavage
and boxed. Horizontal
denote terminal
are indicated
of TnZ.545 as primers.
sites (Poyart-Salmeron
imperfect
by asterisks.
inverted
Blackened
determination
ofthe vector-target
et al., 1989) using oligo specific for the left (5’-GGATAAATCGTCGTATCA-
extremities
aligned with that of attTnl545 arrows
*
17
Ill
the termini of attTnl545
*
l
tagaai l **** ctttta * l * gtaata
It0
was performed
l
t;a;;g
IY
Fig. 4. Specificity
****et**
l *****
AAAAATTTCATAAAAARATCTTAAAA l **** * ** l l * l * * AAAAACAACM4AUdGCAAAGCTTAC
l
junctions
AAAAATCTAGTTATC
repeats
squares
The nt sequences
et al., 1989; 1990). Overlap
in attTn1545. denote
Identical
positions
nt, in pairwise
with a minimum
of the target
regions
sites were deduced
are presented
comparisons,
score of identity
in lower-case
between
and
letters
every target and
of eight out of twelve target
DNAs.
Tn1.545 and can be introduced into Gram+ hosts by electroporation or by mobilization from E. cofi. Integration of these plasmids requires the presence of the transposonencoded integrase in the recipient. Plasmid pATl12 lacks most of the restriction sites that are commonly used for cloning and was constructed for insertional-mutagenesis in Gram + hosts and subsequent cloning and regeneration of the mutated gene in E. coli. The functionality of this system
pAT307. This ORF was truncated by cloning and could code for the C-terminal segment of a protein that shares significant aa similarity with the corresponding moiety of the transposase of IS30 from E. coli (Dalrymple et al., 1984) (Fig. 5). This ORF is currently being further characterized. (g) Conclusions We have constructed and used integrative vectors that should facilitate genetic analysis and manipulation of a large variety of Gram+ bacteria. These vectors capitalize on the transposition properties (integration and excision) of
E. coli (IS30)
Q Y TQHELD L V A R Q Y F P K K T C LA NTNGLI * * t * t:*t: *: SSVSNQRNH KSMDFREVNQTFI 'N S N G I RRNGLP GRATTCTAACGGGATTCGGCGTMTGGACT~C~T~T~ATTTTA~~GT~TCA~~TTTATTTCCAGTGT~~TCMCGTMTCAT
En.faecalis E.
Cob
was illustrated by the characterization of an IS30-like structure in the chromosome of an En. faecalis strain. Plasmids pATl13 and pAT114, which contain ten unique restriction sites, are adapted to the introduction of foreign genes into
(IS30)
R
P
R
K
T
L
K
*t*:t
F
K
T
P
::t*
K
E
I
l
.
I
E
R
G
V
A
L
T
A
Q t
L
N t
N
100
D End
t
En.foecnlis
FLSYVQEA I P R K S L N Y RTPIEI ATTCCAAG~TCATTGAATTACAGAACACCMTT~~TATTTTT~~TATGTA~~~TTTTA~M~M~
F
En.faecalis
CAAAAAAAAAATTTATTTTTTMTTTTCTTTTTGTTMCT~CGMTTTTTT~TGTTTTTCTM~T~~~~T~M
Y
S
N
L
I End GACAAATCATMTTT
200 300
taacat
En. faecalis
400
TAAMTTMCAMCGAGTTCGTAGTATAGCACGGATTTTTTCTCATGTAAACATCATTAMTAAACA~AATTTA
AAACGTTGTTTT taaaat
En.faecalis Fig. 5. Sequence site of pATll2 1). Numbering and compared
418
TACATATTTCTCAGCTM
of an enterococcal are indicated
DNA fragment
by superscript
after integration
and subscript
lower-case
and excision ofpAT
12. The two alternative
letters, The DNA strand
is complementary
hexanucleotides
detected
to that presented
at the excision
in Fig. 4 (insertion
begins at the first nt of the EcoRI site. The deduced aa sequence of the C-terminal moiety of the putative protein encoded is presented with that of the transposase oflS30 from E. coli (Dalrymple et al., 1984). Asterisks and colons indicate identical and homologous (I-L-V-M,
D-E, R-K, Q-N, S-T and F-Y) residues,
respectively.
The aa are aligned
with the second
nt of each codon.
27 Grinter,
the genome of Gram + bacteria. These vectors are routinely used in our laboratory for complementation and expression
N.J.:
Analysis
of chromosome
mobilization
between plasmid RP4 and a fragment Plasmid
of genes in En. faecalis.
using
ofbacteriophage
hybrids
i, carrying
ISI.
5 (1981) 267-276.
lvins, B.E., Welkos, Tn916
S.L., Knudson,
G.B. and Leblanc,
in Bacillus anthracis. Infect.
mutagenesis
D.J.: Transposon Immun.
56 (1988)
176-181. Low, B.: Formation recipient strains
ACKNOWLEDGEMENTS
This work was supported Institut
by a grant (CCAR)
from the
Pasteur.
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60 (1968) 160-167. Messing, J.: New Ml3 vectors
for cloning. Methods
Enzymol.
Poyart-Salmeron, C., Trieu-Cuot, P., Carlier, C. and Molecular characterization of two proteins involved of the conjugative
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