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Characterization of Tn3926, a new mercury-resistance transposon from Yersinia enterocolitica
Gene. 40 (1985) 79-91 Elsevier GENE
1458
Characterization (Recombinant plasmid;
of Tn3926, a new mercury-resistance
DNA; restriction
complementation;
map; transposition
function;
transposon from Yersinia enterocolitica homologies
to Tn21, Tn501, Tnl721;
resolvase;
Hg2 +
Marie-Claire Lett”*, Peter M. Bennettb and Dominique J-M. Vidon” “Universite Louis Pasteur. Laboratoire de Bactt+iologie. FaculttG de Pharmacie, BP 10, 67048 Strasbourg Cede-x (France) Tel. 188)66.90.77, poste 707, and bDepartment of Bacteriology, Medical School. Universitll Walk, Bristol BS8 1 TD (U.K.J Tel. 272 24 161, ext. 919 (Received
April 25th, 1985)
(Revision
received
(Accepted
September
September
17th, 1985)
ISth, 1985)
SUMMARY
A new transposon coding for mercury resistance (HgR), Tn3926, has been found in a strain of Yersinia YE138A14. The element has a size of 7.8 kb and transposes to conjugative plasmids belonging to different incompatibility groups. A restriction map has been established. DNA-DNA hybridization indicates that Tn3926 displays homology with both Tn501 and Tn2I ; the greatest homology is shown with the regions of these transposons that encode Hg R. Weaker homology is observed between Tn3926 sequences and those regions of TnSOl and Tn2I that encode transposition functions. Complementation experiments indicate that the Tn3926 transposase mediates transposition of Tn21, albeit somewhat inefficiently, but not of Tn501, while the resolvase mediates resolution of transposition cointegrates formed via Tn21, Tn501, or TnZ721. enterocolitica,
INTRODUCTION
Mercury resistance in bacteria is both well-known and widespread. The earliest observations were reported 20 years ago and involved hospital isolates
* To whom correspondence
and
reprint
requests
should
be
addressed. Abbreviations:
Ap, ampicillin;
phenicol;
Hg, mercuric
nalidixic
acid;
resistant;
Rif, rifampicin;
tetracycline;
Nm, neomycin;
Cm, chloram-
nt, nucleotides;
Sm. streptomycin;
Tn, transposon;
soy agar; TSB, trypcase plasmid-carrier
bp, base pair(s);
ions; kb, 1000 bp; Km, kanamycin; Su, sulfamides;
Tp, trimethoprim;
soy broth;
0
1985 Elsevier
Science
Tc,
TSA, trypcase
::, novel joint;
[ 1,designates
state.
0378-I 119/85/$03.30
Nal,
R, resistance,
Publishers
of Staphylococcus aureus (Richmond and John, 1964). Subsequently, HgR bacteria were isolated from mercury-polluted soils (Tonomura and Kanzaki, 1969). In most cases, genetic studies of mercury resistance have shown that the determinants of this phenotype are plasmid-borne (Smith, 1967; Summers et al., 1975; Silver et al., 1976; Weiss et al., 1978; Ogawa et al., 1984). Plasmids conferring in a resistance to Hg2+ have been demonstrated wide range of species including S. aureus (Novick and Roth, 1968; Weiss et al., 1977) Pseudomonas sp. (Joly et al., 1976; Clark et al., 1977), Escherichia coli (Summers and Silver, 1972; Nakahara et al., 1977) and other enteric bacteria (Schottel et al., 1974). The prototype HgR determinant in Gram-negative bac-
teria is that carried (Tanakaet Silver,
on the IncFII
plasmid
RlOO
al., 1976; Miki et al., 1978; Summers
1978;
Silver
and
Kinscherf,
1982;
and
resistance
to mercuric
strains
of Pseudomonas
Friello
and Chakrabarty,
et
et al.,
1977;
1980), E. coli (Summers
al., 1980), Citrobacter, Klebsiella (Radford
constituents
of transposable
agar (Institut
agar or
Production).
(b) Genetic experiments
et al.,
et al., 1983) are
Transposition of HgK gene(s) was detected by mating strains containing both a plasmid encoding HgR (PLY 1 or pCL4) R388, pUB307) tive recipient
elements.
plasmid
selected either for acquisition
designated
[ R388]; TcR, [pUB307]).
by the target
(Sa,
mercury-sensi-
strain of E. coli. Transconjugants
encoded
which was the only resistant
and a target
with a plasmid-free,
We reported previously the isolation of a HgK strain of Yersiniu enterocolitica (Vidon et al., 1981), YE138A14,
Pasteur
ions in certain
(Stanisich
1981) and Proteus mirubilis (Tanaka
Mueller-Hinton
Misra
et al., 1985). It has also been shown that the genes determining
TSB on Luria broth (L broth) or on Hektoen
were
of HgR or a resistance (Cm”[ Sa] ; Tp”,
plasmid
The ratio of the number
of
one among more than 200 strains isolated from raw milk. Although YEl38A14 is resistant to mercuric chloride and merbromin, it is sensitive to the organomercurial derivatives sodium merthiolate and phenyl mercuric borate. This phenotype corresponds to the narrow spectrum of resistance found in a number of mercury-resistant enterobacteria. This paper reports that the HgR of Yersiniu enterocolitica 138A14 is carried on a transposon, Tn3926. This transposon forms part of a nonconjugative plasmid, named pLY1, present in YEl38A14. Some molecular properties of Tn3926 are presented and its relationship to Tn.501 (Bennett et al., 1978) and to Tn21 (Nisen et al., 1977; de la Cruz and Grinsted, 1982) is investigated.
the former to the number transposition frequency.
k1.KI’kRlALS
mutants of Tn21, Tn501 and Tnl721, experiments were executed as described by Grinsted et al. (1982). Derivatives of E. coli UB5201 containing the conjugal plasmid R388, a plasmid carrying the appropriate mutant transposon and a plasmid carrying
AND METHODS
(a) Media Bacteria TABLE Relevant
were grown on TSA (Biomtrieux)
or in
of the latter gave the Donor strains were
counterselected with Nal, Sm, or Rif, as appropriate. Crosses were carried out by growing both donor and recipient strains in mixed culture on Mueller-Hinton agar (18 h, 37’(Z), after which the cells were resuspended in 1 ml to a cell density of approx. 10”’ cells/ml. 0.1 ml of appropriate dilutions were spread on selective agar. The levels of antimicrobials used in selective agar were: mercuric chloride, 12 pg/ml; Km, 12 pg/ml; Nal, 40 pg/ml; Sm, 100 pg/ml; Rif, 100 pg/ml; Tc, 20 pg/ml; Cm, 25 Llgiml; Tp. 25 [[g/ml. Drugs were incorporated in TSA (except when Tp was used; then minimal agar with appropriate supplements or Mueller-Hinton agar was used). To test the ability of Tn3926 to complement tnpA
I properties
of the bacterial
Strain
Species
strains
used Relevant
genotype
Source
or reference
BJ 6183
E. co/i
recBC sbcB end& gul met SW thi bio hsdR
B. Jarry
HB 101
E. co/i
pro leu thi lcrc gal recA rpsL (SmR)
G. Gerbaud
C 600
E. coli
thr leu thi lrrc tmA supE
G. Gerbaud
YE 13XAl4
Y. enrrrocolitica
this study. Vidon et al. (1981)
Nal 4
E. coli
W? F recA .sv CrrgC metA NalR
LIB 281
E. coli
pro, met, NalK
Bennett
and Richmond
(1976)
JC 6310
E. coli
hi\, try, IJS, luc, recA, rpsL (SmR)
Bennett
and Richmond
(1976)
UB 5201
E. coli
pro, met, recA, NalR
Bennett
et al. (1977)
UB 1832
E. coli
his, rry, l.1.3,lm, rpsL, rpoB, RifK
Sanchez
this study.
et al. (1982)
Tn3926
were constructed
E. coli UB1637.
Selection
which had acquired
number ance
crossed
with
was for transconjugants
linked resistance
marker on the mutant total number
and then
transposon.
to Tp and the The ratio of the
of such transconjugants
of transconjugants
which
to only Tp was taken
to the total acquired
resist-
samples
were
mounted
technique
(1969) as described
on grids
of Westmoreland
by Davis
using et al.
et al. (197 1). Phage
$X174 single- or double-stranded was used as internal standard.
DNA (5375 nt)
RESUI.TS AND DlSClJSSION
To test the ability of Tn3926 of TnZI, pCLi7
was transformed
to complement
tnpR
Tn.501 and Trill 721, experiments
were carried out as described Plasmid
DNA
the formamide
as the transposition
frequency. mutants
(e) Electron microscopy
(otherwise
by Diver et al. (1983). pACYC184:
into derivatives
:Tn3926)
of E. coii UB5201
containing one of the test plasmids pJOE562, pUB2589 or pUB2591. Resolution was seen to have occurred when linkage between the ApR determinant and the other resistance determinant(s) on the test plasmid was broken.
(c) Isolation of plasmid DNA (i) Rapid preparation. Rapid plasmid preparation was performed essentially as described by McCormick et al. (198 1). Plasmid DNA isolated by this method was used to determine plasmid size after electrophoresis in 0.7% (w/v) agarosc gels by comparison with standard plasmids. (iij Large-scale isolation of plasmid DNA Plasmid DNA was isolated using a Triton X-100 cleared-lysate procedure (Davis et al., 1980). 500 ml overnight cultures in L-broth were used as starting material. DNA was recovered from agarose scribed by Hubert et al. (1980).
(d) DNA-DNA
gels as de-
hybridization
DNA from 17; (w/v) agarose gels was transferred to Schleicher & Schuell nitrocellulose sheets according to the procedure of Southern (1975). Plasmid DNA probes were prepared by nick translation (Maniatis et al., 1975). Hybridization was carried out in heat-sealable plastic bags at 42°C for 20 h with a 3”P-labelled probe (1-5 x lo6 cpm) as described by Maniatis et al. (1975). Filters were autoradiographed at -2O’C for 48-168 h.
(a) Plasmid content of YE138A14 YE138A14 merbromin
is resistant
to mercuric
but not to merthiolate
chloride
and
nor to phenyl
mercuric borate. The strain contains two plasmids: one of 30 kb (PLY 1) and one of 13 kb (pLY2), as determined by agarose gel electrophoresis. Electron microscope contour length measurements gave values of 31.6 kb and 12.5 kb for pLY1 and pLY2, respectively, in good agreement with the values obtained from gel electrophoresis. HgK was not transferred by conjugation. To determine if HgR was related to extrachromosomal DNA, we extracted plasmid DNA from the agarose gel and used it to transform E. coli BJ6183. Hgn transformants were selected. These were recovered when pLYI, but not pLY2, was the transforming DNA, and such transformants contained a plasmid that comigrated with PLY 1. Plasmid DNA isolated from these transformants was able, in turn, to transform E. co/i HBlOl to HgK. (b) Mobilization and transposition of mercury resistance and isolation of the recombinant plasmids All attempts to transfer HgR by conjugation from YE138A14 to E. coli Na14 were unsuccessful, both at 37 “C and at 28’C. Consequently, mobilization of the HgR determinant by the R plasmids Sa, R388 and pUB307 was investigated (see MAT‘ERIALS AND METHODS, section b). HgR transconjugants were isolated from all crosses at a frequency of about lo-‘. Five of the recombinant plasmids, designated pCL4, pCL5, pCL6, pCL7 and pCL9 (see Table II), were chosen for further study. All but pCL.5 were larger than the parent plasmid and the phenotypes conferred by the recombinant plasmids were those of the recipient plasmid plus HgR (see Table II). Comparing the restriction digest of plasmids obtained during such crosses with those ofthe parent plasmids (not shown) we could determine that PLY 1 was not
TABLE
II
Plasmids.
host cells and bacterial
Plasmids
Relevant
pLYl
HgK
strains
used Construction
characteristics“
source this paper
PLY?
this paper gift of N. Dattab
Sa
IncW. Tra, SmR, Kmn, CmR, SuK
Ward
and Grinsted
(19X2)
R388
IncW, Tra, SuR. TpR
Ward
and Grinsted
(1982)
pUB307
IncP, Tra, NmiKm,
Bennett
pBR322
TcR. ApR
pACYCl84
TcR, CmR
pVSl
Sun. HgK
pCL4
IncW,
Ten
et al. (1977)
Gift of G. Loison Gift of V. Stanisich‘
Tra,
SmR. KmR, CmR, Sun,
Sa::Tn3Y26’
this paper
HgR pCL5
IncW, Tra, Smn. KmR, SuR, Hgn
Sad::Tn3Y26”
this paper
pCL6
IncW. Tra, Sun, Tpn, HgR
R388::TnSY26’
this paper
pCL7
IncP, Tra, NmK:KmK.
Ten, HgR
pUB307::Tn3926”
this paper
pCL9
IncP, Tra, NmR:KmR.
TcR, HgR
pUB307::T1r3926~
this paper
pCLl7
CmK, HgK, TcK
pACYC184::Tn3926
this paper
pUB78 1
ColEI ::TnSOl
p U B8 I0
Hgn CmK
pUBXlX
TcR, ApK
pUB2401
Cmn,
pUB2402
TcK, SmK:SpH,
pUB2406
Cmn
SmR/SpR,
HgR, SuR SuK, HgR
of pDS6501
Gift of J. Grinstcd
deletion
derivative’
of pJOE105
Gift of J. Grinsted
pACYC184
(rer::TnZly
pACYC184
(ccrt::Tn21)’
EcoRI deletion
Gift of J. Grinsted Gift of J. Grinsted
derivativek
of
Gift of J. Grinsted
I Gift of J. Grinsted
pBR322::TnZlA
ApK TcR
et al. (1978)
derivativeh
pUB240 pIJB3321
Bennett
deletion
carrying
the same Tn21 EcoRI
dele-
tion as pUB2406 ptiB2575
Tpn, TcR
R388::Tn1721
pJOE562
Apn. KmR
pBR322
derivative
tro and carrying flanked
by direct repeats
Cointegrate
ApR. TpR, SuR
pUB2589
constructed
generated
tion of Tn8/3
in vi-
a KmR determinant
R. Schmitt
via J. Grinsted
(Altenbuchner
and Schmitt,
19X3)
of Tnl721 by transposi-
J. Grinsted
from pBR322::Tn813
to R38X Apn. Tpn. SuR, KmR
pUB2591
Cointegrate tion
generated
of Tn1727
from
J. Grinsted
by transposipJOE529’
to
R388 I’ Symbols
for resistance
’ Dept. of Bacteriology, ‘ Dr. V.A. Stanisich,
phenotypes
Department
cl Plasmid
Sa was introduced
containing
mercuric
were selected probably
chloride
a deletion
into YEl38A14
’ Plasmid pCL6 was constructed
” pIJBXI0 (Grinsted repeats
Hammersmtth University, (Lesage
by Novick
Hospital,
Bundoora
Ducane
et al. (1976). Road,
WI2 OHS (U.K.)
(Australia).
et al., 1975). Transconjugants
YEl38Al4(Sa)
London
3083, Melbourne
were selected
on Hektoen
agar
were in turn crossed with E. co/i Nal4 and transconjugants
resistance. Sa. The Cmn gene is lost. The deletion
recombination
across
the short homologous
to occur with Sa itself in both UB28l by transforming
(Cohen
is not adjacent
sequences
and UB5201
flanking
(P.M. Bennett
et al., 1972) pLY1 into the rerA
to the Tn3Y26 insertion, the CmR gene (Ireland,
and V.G. Krishna,
strain
UB5201
(R388).
but 1983).
unpublished). Transformants
both plasmids were. in turn, crossed with E. coli JC6310. Transconjugants were selected for Sm and mercury resistance. pCL7 and pCL9 were constructed by mtroducing pCL3 in the ret strain UB5201 [pUB307] by conjugation. TranscoirJuganta
vvcre in turn. crossed of Glasgow).
La Trobe
by conjugation
of 5.2 kb of plasmid
We have also shovvn this deletion
follow those proposed
School,
and Km. These transconjugants
arose due to host-dependent
harbouring ” Plasmids
by plasmids Medical
of Microbiology,
for Nal and mercury
’ pCL5 contains
conferred
Royal Postgraduate
pDS6501
are intact,
with E. w/i UB1832.
Progeny
et al., 1982) is a deletion is a pACYCl84::TnSOl
but all other functions
of these crossed
derivative
of pDS6501
recombinant
plasmid.
have been lost or damaged.
were selected (obtained
for Rif, mercury
and Tc resistances.
from Prof. D. Sherratt,
The 6-kb deletion
is fully contained
Dept. of Genetics,
University
within Tn501. The inverted
a
b
a 12
1234
2
3
4
2 .6kb
Fig. 2. Comparison
of plasmids
(1 “b) slab gel electrophoresis Fig. I. Comparison
of plasmids
Sa, pCL3,
restriction
fragments
ofplasmids:
(1) Sa; (2) pCL4; (3) pCL5. (b)
autoradiographs
Southern
blot autoradiographs
of EcoRI
ffindII1,
plasmids
(1) Sa; (2) pCL4; (3) pCL5, 3”P-labeled PLY i DNA.
translated.
pCL5. digested
hybridized
(a) EcoRi DNAs
EeoRI,
of
to nick-
’ pUB818
(Grinsted
DNA
(4) SalI,
et al., 198 I) is a insertion
derivative
digested
by (1) EcoRI,
hybridized
k pUB2406
(de la Cruz fragment
’ pJOE529, generated
blot (2)
to nick-translated,
pCL4 DNA.
(c) Verification of Tn3926 on recombinant plasmids The relationship between pLY1 and pCL4 and pCL5 was investigated by DNA-DNA hybridization. “2P-labelled pLY1 was used as a DNA probe against Southern blot transfers of pCL4 and pCL5 digested with EcoRI (Fig. 1). Plasmid pLY1 did not hybridize to Sa DNA but did hybridize with two fragments each of pCL4 (one of 2.6 kb and one larger fragment) and two fragments of pCL.5 (one of 2.6 kb and one larger fragment). In the reciprocal hybridization using 12P-labelled pCL4 DNA against a Southern blot transfer of PLY 1 digested with EcoRI, pCL4 hybridized with two fragments of PLY 1 (one of 2.4 kb and one of 9.3 kb, Fig. 2). Comparison of restriction digests of Sa, pCL4 and pCL5 showed that the 2.6skb fragment
of pJOElO5.
of Tn I72i into a derivative
B pUR2401and pUB2402 (de la Cruz and Grinsted,
EroRl-EcoRI
by (I)
(b) Southern
----
et al., 1982) is a deletion
the IL’?gene, and in pUB2402
pJOE529
of pL.Yl
1 DNA digested
(4) S&I.
_
-~.I_--
encodes
(3) BarnHI,
(3) BarnHI,
‘*P-labeled
mobilized and that each HgR transconjugant contained a recombinant plasmid comprising the conjugative plasmid (Sa, R388 or pUB307) and part of pLYI. On the other hand the recombin~t plasmids showed the same DNA sequence inserted into two different sites in Sa (generating pCL4 and pCL5) and into two different sites in pUB307 (generating pCL7 and pCL9). Insertion into R388 generated pCL6. These data are consistent with the interpretation that the HgR determinant originating in YE138A14 and carried on pLY1 is part of a transposable element. The element is designated Tn3926. Tn3926 was, in turn, transposed from pCL6 to pACYC184 to generate pCL17 and its integrity was confirmed by showing that it could retranspose to R388 at a frequency of 10e5.
(Sch6ffl
(2) HindIII,
PLY1 and pCL4. (a) Agarose of PLY
insertion
and Grinsted,
Deletion
overlaps
part of the mpA gene of Tn1721.
pJOE105
of pBR322.
1982) are recombinants
of pACYC184
and TnZI.
In pUB2401
insertion
is into
is into the cat gene. 1982) was generated
after EcoRI
digestion
of pUB2401.
This plasmid
has lost the inner
of Tn21. from the pBR322 derivative
KmK by virtue of the insertion was kindly supplied
plasmid
pJOElO0
(Schbf?l et al., 1981), carries Tni727.
of the KmR gene of Tn5 into the H&d111 site of TnJOl.
by R. Schmitt.
Tn1727
a derivative carries
ofTnSOI
which
the res site of TnSOI.
84 EBt3H
h
p
BhB
h I
E
B
h I
P
hhBB Illi
t
I
/
,
hBB
H
h I
II
I
I
/
EP iI
E
i
&_
..---
.__
Fig, 3. Restriction E, EcoRI; PwII, acetate,
fragments
_-__p-*
Tn 3926
map of pCLl7.
H, HirzdIII;
were obtained
generated
___
h, HitidIl;
Length
of restriction
from Miles or BRL. Digestions were analysed
10 mM disodium
EDTA,
fragments
B, Rgll; P, PvuII. EcoRI, Hindll, on horizontal
were performed
agarose
pH S.3) or Tris borate
HindIll,
were purchased
as described
of pCL17
Comparison of restriction digests of pACYC 184 and pCL17 indicated that the latter was generated from the former by the insertion of a single 7.8-kb DNA sequence with the restriction map presented in Fig. 3. The insertion, Tn3926, has two EcoRI sites, one site each for HindIII and PvuII, six Hind11 sites and seven BglI sites. of Tn3926 to TnSUZ and Tn2I
Transposons Tn21 and Tn501 also confer resistance to mercuric ions and merbromin (Nisen et al., 1977; de la Cruz and Grinsted, 1982; Stanisich et al., 1977; Bennett et al., 1978). The relationship of Tn3926 to these elements was examined, therefore, using DNA-DNA hybridization. (1) Hybridization to Tn501 “‘P-labelled pLY1 DNA was hybridized to Southern blots of pUB78 1, a ColEl : : Tn501 derivative, digested with BglI and PvuIl, and BglI and E’coRI. Plasmid pLY1 hybridized with four BgZI-generated fragments of pUB781 (A,B,C,D), four PvuII
pACYC
location
184
----.--__*
of the boundorics
from Boehringer-Mannheim;
by Grinsted
slab gels using either Tris acetate
to Sa.
(e) Hybridization
is given in kb. The precise
buffer (Petrocheiiou
was derived entirely from Tn3926. Furthermore, the fact that, in addition to the 2.6-kb EcoRI fragment, both pCL4 and pCL5 display only one other EcoRI fragment with sequence homology to PLY 1 led us to conclude that one of the two EcoRI sites of Tn3926 must be located at or very close to one end of the clement. These results con~rmed the conclusion that DNA sequences, i.e., Tn3926, had transposed from PLY 1
(d) Characterization
~------_
et al. (1978). Restriction
buffer
is uncertain. Bg/I, and endonucleasc-
( 150 mM Tris OH. 50 mM sodium
et al., lir’lh}.
fragments (A,B,D,E), live fragments generated with BglI plus PvuII (A,B,C,E,F) and three generated with BglI plus EcoRI (B,D,E) (Fig. 4A). The degree of hybridization to the various fragments was not uniform and appeared to be most efficient with Bg0 fragment C, PvuII fragment A, BglI-PvuII fragment E and Bg!I-EcoRI fragment E, all of which include either part of, or the entire gene for mercu~ reductase. Less intense hybridization was observed between PLY 1 sequences and fragments of pUB78 1 derived from the transposition region of Tn5OI. A reciprocal hybridization indicated that “Plabelled pUB781 DNA hybridized to seven fragments of pCL17 generated with Hind11 plus EcoRI (fragments A,B,C,D,G,H,I, Fig. 4B). With the exception of fragment A, all of these fragments are derived from Tn3926. Fragments A,C,D and H show more intense hybridization than do fragments B,G and I. Fragment A contains the replication region of pACYC184 which is related to that of ColEl (Stuber and Bujard, 198 l), and so hybridization between pUB781 (otherwise ColEl : : Tn501) and pCLl7 (otherwise pACYC184 : : Tn3926) was to be expected. Hybridization to other fragments of pCL17 confirms that there is homology between Tn3926 and Tn501. The transposition functions of Trill 721 have been shown to be very closely related to those of Tn501 (Altenbuchner et al., 1981; Grinsted et al., 1982). In agreement with this result and results reported above we found that Tn3926 displayed homology with Tn1721 (not shown). (2) Hybridization to Tn 2 1 Tn3926 was also compared with Tn21 which is known to show homology with Tn.501 (Grinsted et al., 1982). ASP-labelled pLY1 was hybridized
to
85
1 b
a
4
3
2 a
a
b
b
a
Tn 501 res
pvu
ttlpR
A*
fl
a
b
tnpA
Fig. 4. Hybridization
of Tn3926
to TnSOI. (A) Hybridization
is shown on the bottom. hybridization).
Agarose
Length
has been described
to pCL17
of restriction
fragments
(1“()) slab gel electrophoresis
I b, Zh, 3b, 4b. (B) Hybridization pCLl7
bctwecn
in Fig. 3. Agarose
is shov,,tn in lanes (b).
between
pUB781
pCLl7
is given in kb.
+
(a ColEl ::TnSOI
and pLY1 labelled with “I’. The map ofTn501
(Bennett
digested
by a mixture
+
derivative)
digested
of HilldIl
by
et al.. 1978; Altenbuchner
(A, EcoRI, +. PvuII. V, Bgll. Asterisks:
is shown in la, _?a, 3a, 4a, and hybridization
( I ‘I,,) slab gel electrophoresis
B*
E*
D*
l
Rx/I-Portll; (3) PvuII; (4) Bg/I-EcoRI,
b
of “P-1abelled
+ EcoRI and pUB781
bands
(1) Bgil; (2) ct al., 19x1) that shop
a
pLYl to plJB7XI
in
labelled with “P, The map of
is shown in lanes (a) and hybridization
of “P-labellcd
pUB7XI
X6
1 a
2 a
b
b
UB2402
A
C
F
t-
Tn21A
E
pUB2406
0
Fig. 5. Hybridization
ofTn3926
to Tn21. Hybridization
PLY I DNA. The map of pUB2402
EcoRI). pUB2406
Agarose
and pUB2406
(I “,,) slab gel electrophoresis
is shown
in lanes
8.7
5
ofpUB
(shown is shown
t
(1) and pUB2406
at the bottom) in lanes
(2), both digested
have been described
la, 2a and hybridization
by EcoRI, with nick-translated (1982); (7, I with pUB2402 and
by de la Cruz and Grinsted of 72P-labelled
PLY
lb, 2b.
Southern blots of EcoRI-digested pUB2402 and pUB2406 (pACYC184 : : Tn21 derivatives). Plasmid pLY1 displayed homology with fragments A,C,D and G of pUB2402 and with fragments A and B of pUB2406 (Fig. 5). Since pLY1 did not hybridize to
pACYC184 itself (not shown), then the hybridization noted in these experiments indicated hybridization of Tn21 sequences. Hybridization was most efficient with fragments D and G from pUB2402 and fragment B from pUB2406, fragments known to carry
87
sequences
encoding
the mercuric
Tn21 (de la Cruz and Grinsted, hybridization
to fragments
reductase
gene of
1982). In contrast,
A and C from pUB2402
and fragment A from pUB2406, which quences derived from the transposition
carry segenes of
end-products
position functions
of mutations
in the trans-
of Tu22, TnSOZ and Tn1721
by
of pUB810
pVSS82, ment
which carries
such as Tn21,
Tn5UI
and Tnf 721
transpose in a two-stage process which uses transposase function ft3zpA) for the first stage to generate cointegrate molecules (Arthur and Sherratt, 1979; Shapiro, 1979; Grinsted et al., 1982; Diver et al., 1983), which are resolved in the second stage to yield the transposition end product, together with a DNA molecule indistinguishable from the original transposon donor (Arthur and Sherratt, 1979; Shapiro, 1979). This second stage involves a site-specific recombination system comprising a tnpR gene which encodes the resolution enzyme, resolvase, and a res site, the site at which the resolvase acts. The hybridization experiments clearly indicated homology between Tn3926 and those sequences of Tn501, Tn1721 and Tn2I encoding transposition functions. Hence experiments were undertaken to determine if Tn3926 encodes functions which can complement one or more of the functions encoded by Tn21, Tn501
and Tn1721.
(1) Transpusase (tnpA) function Plasmid pUB8 18 carries a copy of Tn 1721 with a deletion that has removed part of the tnpl4 gene. The remainder of the element still encodes TcR and can transpose if complemented (Grinsted et al., 1982). We were unable to detect any complementation mediated by PLY 1 or pCL6 (frequency < 6 x lo-‘), although in control experiments pUB2575, which carries Tn1721, did complement to give a transposition frequency for the TcR of pUB818 of 2 x 10-h. Plasmid pUB810 carries a deleted Tn501. Both end-points of the deletion are within the element but it has inactivated both the HgR determinant and the transposition functions. When appropriately complemented, however, the deleted element generates cointegrates, rather than normal transposition
(containing
1.5 x lo-‘). Tn501
of the
and cointegrates
a frequency Transposons
1979; Shapiro, is a self-trans-
into R388 or pUB307,
of detection
transposition
pUB810
Tn 3924
DNA
missible plasmid, then, such cointegrates
tively (limit (f) Complementation
and Sherratt,
the recipient
pUB8 10) encode CmR and can be conjugally transferred. Neither pLY1 nor pCL6 mediated cointegration
Tn21 was less efficient.
(Arthur
1979). When
of about
intact,
respec-
In contrast, did comple-
residual
element
on
with R388 were formed at 10m4, as expected
(Grinsted
et al., 1982). Hence, neither pLY 1 nor pCL6, both of. which carry Tn3926, mutant
TnSOf
complement
or Tnl721
transposition
elements.
of
in contrast,
complementation of a mutant Tn21 was detected. Plasmid pUB2406 is a deletion derivative of the pACYC184: : Tn21 recombinant pUB2401 (Grinsted et al., 1982) and plasmid pUB3321 contains the same EcoRI deletions of Tn21 as pUB2406 but is a pBR322 : : Tn21 derivative. The deletion removed only Tn21 sequences, but left the ends of the element intact. Both the transposon encoded drug-resistance genes and the transposition functions were inactivated. Nonetheless, the residual element can be complemented to transpose by wild-type Tn2f transposition functions (Grinsted et al., 1982), to generate cointegrates comprising pUB2406 or pUB3321 and the recipient DNA molecule. In the presence of PLY 1, pUB2406 formed cointegrates with R388 (frequency, 1.9 x 10-7), while pCL6 mediated cointegration of pUB2406 and pUB307 (frequency, 1.3 x 10dh). Further pCL17, a pACYCl84: : Tn3926 recombinant also mediated cointegration of pUB3321 and R388 (frequency 4 x IO-“). That the transconjugants generated in these crosses did harbour cointegrates was confirmed by demonstrating that the CmK determinant of pUB2406 was linked to the TpR determinant of R388 because the former marker always cotransferred with the TpK determinant in conjugal crosses, irrespective ofwhich marker was selected. The transconjugants examined each contained a single plasmid, all of which were indistinguishable in size but which were larger than either pUB2406 or pUB3321 or R388. Restriction enzyme digests of some of these (data not shown) displayed fragment proliles which could be distinguished but which were all consistent with the recombinant plasmids being cointegrates of ~1182406 or pUB332 1 and R388 generated by trans-
xx position
of the deleted Tn21 present
on the former
plasmid.
tation of tnpR gene function. to indicate
that Tn3926
These results are taken
does possess
and therefore, by implication, (2) Resolvase (tnpR) function Plasmid
pUB2589
is
cointegrate
of R388
and
Tn813, a tnpR derivative and which encodes resolvase cons
is
pBR322
ofTn2l
mediated
by
(g) Conclusions
(Diver et al., 1983) When the missing
supplied
to yield
to be tested.
a transposon-generated
TpRApRTcR.
activity
resolve
that remains
a tnpR gene,
a res site, a conclusion
the
R388: :Tn813
two (TpK)
repliand
(1) Two plasmids, PLY 1 and pLY2, with sizes of 30 kb and 13 kb, respectively, have been identified within
YE138A14,
a
HgK
wild-type
strain
of
pBR322 : : Tn813 (ApRTcR), and the former plasmid can be conjugally transferred independently of the
Y. enterocolitica. The 30-kb plasmid, PLY 1, encodes resistance to mercuric ions and merbromin. The Hg”
latter. Plasmid pUB2591 is a cointegrate of R388 and pJOE529, generated by transposition of the Tn1727 element (a derivative of Tn501 constructed in vitro
gene(s)
and encoding KmR) carried on pJOE529, and encodes TpKKmRApR. Resolution generates two plasTpKKmK and the other mids, one encoding ApRKmR. Again the former plasmid can be conjugally transferred independently of the latter. Plasmid pJOE562 is a derivative of pBR322 constructed in vitro. It encodes ApRKmK and the KmR determinant is flanked by direct repeats of the Tn1721 res site (Altenbuchner and Schmitt, 1983). Recombination across the duplicate res sites deletes the Kmn gene, which, because it is not longer linked to an origin of replication, is not recovered. Plasmid pCLl7 was transformed into UB5201 containing pUB2589, pUB2591 or pJOE562, and retention of linkage of “cointegrate” markers was determined. In all cases linkage of “cointegratc” markers was stable in the absence of pCLl7 (Table III), while in the presence of pCLl7 the link was severed (Table III), indicative of complemen-
TABLt Integrity Plnsmid
was
belonging
mobilized
by conjugative
to different incompatibility
cally Sa and R388 (both IncW) and pUB307 (IncP). The transconjugants from these experiments contained recombinant plasmids which all bore the same insert located at different sites on the different target plasmids. This recombination occurred in a recA strain, as well as in a Ret + strain. All these results together supported the conclusion that mercury resistance encoded by PLY 1 constitutes part of a transposon now called Tn3926. (2) Tn3926 is a 7.8-kb transposon which contains two EcoRI sites, one located very close to one end of the element and 2.6 kb from the other site. A Hind111 site is located between these EcoRI sites, 0.5 kb from the EcoRI site located at the end of the element (Fig. 3). These data indicate that Tn3926 is. in these respects, similar to Tn2613, another transposon encoding HgK (Tanaka et al., 1983). Other parts of the sequence are not obviously related to Tn2613. The restriction pattern differs from that of the prototype HgR transposon, Tn501, a transposon of almost the same size as Tn3926.
III of plasmids
carrying
two directly
repeated
ret sites in the presence
Linked resistance
Source
determinants
repented
of pCLl7
of directly
Linkage
YESyitc
second -pc1.17
of .ApK to marker’ tpC‘LI7
pJOE562
ApK. KmK
Tnl72l
50:50
I) 100
PUB2589
ApK, 1‘P K Ap’. TpK
‘I 1121
5050
0 100
Tn501
48.5lJ
13 50
pUB2591
I’ Loss of linkage of ApK and KmK (pJOE562) (pl!B2589
plasmids
groups, specifi-
and plJB2591)
was dctcrmined
WBS determined
by conjugal
transfer
by loss of Km” but retention of TpK unlinked
to Ap’
of ApK. Loss of linkage of ApK and Tp”
89
(3)
Tn3926
displayed
Tn501 and Tnl721
homology
with
as shown in hybridization
ments (Figs. 4 and 5). It hybridized
Tn21,
ACKNOWLEDGEMENTS
experi-
most strongly to
We
are
indebted
Schneider, F. Lacroute
zation
mation.
We thank
electron
microscopy
showed
a strong homology
and the left-hand the two EcoRI
sequences
between
of Tn3926,
sites (Fig. 4B). Together
Tn501
defined
by
to
M.
Nguyen-Juilleret,
and A. Mercenier
for materials
J. Menissier study.
Gerbaud,
above data this suggests that the genes for HgR en-
bacterial
coded by Tn3926
advice and a gift of plasmids.
on the left of the ele-
ment (Fig. 3). Homology
between Tn3926
was strong and involved
sequences
the latter element,
and Tn21
at both ends of
one end of which accommodates
genes for Hg R, including a mercury reductase gene. Our data are consistent with the previously observed homology between the mercury resistance genes of Tn501 and Tn21 (Tanaka et al., 1983). (4) The hybridization data clearly indicate homology between sequences carried by Tn3926 and sequences encoding transposition functions on Tn21, and Tn501 (and Tnl721), the transposition systems of which are known to be related (Grinsted et al., 1982; Diver et al., 1983). However, while Tn3926 was able to complement a tnpA mutant of Tn21, complementation of analogous mutants of Tn.501 and Tn 1721 was not observed. However, in that the transposase of Tn21 complements tnpA mutants of Tn501 and Tn1721, but not vice versa, despite the fact that these systems are related (Grinsted et al., 1982) the genetic results are consistent with the interpretation that the tnpA gene of Tn3926 is related to the equivalent genes of these other transposons. Transposon Tn3926 also encodes a function that can substitute for the resolvase functions of Tn21, Tn.501 and Tnl721 (Table 3), which are interchangeable (Diver et al., 1983). The data indicate that the transposition systems of all four elements are related and that there is a common progenitor sequence for all four transposons. Hence Tn3926 is clearly related to the family of transposons, the prototypes of which are Tn21 and Tn501, but is distinct from both. Our data suggest that Tn3926 is more closely related to Tn21 than to Tn.501 in that the former element displays homology with the latter throughout its sequence, and the transposition functions of Tn3926 can substitute for the equivalent gene products of Tn21.
N. Datta strains,
is indebted
or infor-
for her help in the
We are grateful
with the
are located
C.
G. Loison, R. Jund, A. Labigne-Roussel,
the fragments of TnSOl which encode the genes for mercury resistance (Fig. 4A). The reciprocal hybridi-
and V. Stanisich
we thank
to G.
for a gift of
J. Grinsted
for fruitful
One of us (M.C.L.)
to FEBS and EMBO
for financial
sup-
port to stay at the Medical School of Bristol, and to AH. Linton for his hospitality. This research was supported in part by the A.T.P. ‘Microbiologie’ No. 1482 from the Centre National de la Recherche Scientilique.
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Characterization (Recombinant plasmid;
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DNA; restriction
complementation;
map; transposition
function;
transposon from Yersinia enterocolitica homologies
to Tn21, Tn501, Tnl721;
resolvase;
Hg2 +
Marie-Claire Lett”*, Peter M. Bennettb and Dominique J-M. Vidon” “Universite Louis Pasteur. Laboratoire de Bactt+iologie. FaculttG de Pharmacie, BP 10, 67048 Strasbourg Cede-x (France) Tel. 188)66.90.77, poste 707, and bDepartment of Bacteriology, Medical School. Universitll Walk, Bristol BS8 1 TD (U.K.J Tel. 272 24 161, ext. 919 (Received
April 25th, 1985)
(Revision
received
(Accepted
September
September
17th, 1985)
ISth, 1985)
SUMMARY
A new transposon coding for mercury resistance (HgR), Tn3926, has been found in a strain of Yersinia YE138A14. The element has a size of 7.8 kb and transposes to conjugative plasmids belonging to different incompatibility groups. A restriction map has been established. DNA-DNA hybridization indicates that Tn3926 displays homology with both Tn501 and Tn2I ; the greatest homology is shown with the regions of these transposons that encode Hg R. Weaker homology is observed between Tn3926 sequences and those regions of TnSOl and Tn2I that encode transposition functions. Complementation experiments indicate that the Tn3926 transposase mediates transposition of Tn21, albeit somewhat inefficiently, but not of Tn501, while the resolvase mediates resolution of transposition cointegrates formed via Tn21, Tn501, or TnZ721. enterocolitica,
INTRODUCTION
Mercury resistance in bacteria is both well-known and widespread. The earliest observations were reported 20 years ago and involved hospital isolates
* To whom correspondence
and
reprint
requests
should
be
addressed. Abbreviations:
Ap, ampicillin;
phenicol;
Hg, mercuric
nalidixic
acid;
resistant;
Rif, rifampicin;
tetracycline;
Nm, neomycin;
Cm, chloram-
nt, nucleotides;
Sm. streptomycin;
Tn, transposon;
soy agar; TSB, trypcase plasmid-carrier
bp, base pair(s);
ions; kb, 1000 bp; Km, kanamycin; Su, sulfamides;
Tp, trimethoprim;
soy broth;
0
1985 Elsevier
Science
Tc,
TSA, trypcase
::, novel joint;
[ 1,designates
state.
0378-I 119/85/$03.30
Nal,
R, resistance,
Publishers
of Staphylococcus aureus (Richmond and John, 1964). Subsequently, HgR bacteria were isolated from mercury-polluted soils (Tonomura and Kanzaki, 1969). In most cases, genetic studies of mercury resistance have shown that the determinants of this phenotype are plasmid-borne (Smith, 1967; Summers et al., 1975; Silver et al., 1976; Weiss et al., 1978; Ogawa et al., 1984). Plasmids conferring in a resistance to Hg2+ have been demonstrated wide range of species including S. aureus (Novick and Roth, 1968; Weiss et al., 1977) Pseudomonas sp. (Joly et al., 1976; Clark et al., 1977), Escherichia coli (Summers and Silver, 1972; Nakahara et al., 1977) and other enteric bacteria (Schottel et al., 1974). The prototype HgR determinant in Gram-negative bac-
teria is that carried (Tanakaet Silver,
on the IncFII
plasmid
RlOO
al., 1976; Miki et al., 1978; Summers
1978;
Silver
and
Kinscherf,
1982;
and
resistance
to mercuric
strains
of Pseudomonas
Friello
and Chakrabarty,
et
et al.,
1977;
1980), E. coli (Summers
al., 1980), Citrobacter, Klebsiella (Radford
constituents
of transposable
agar (Institut
agar or
Production).
(b) Genetic experiments
et al.,
et al., 1983) are
Transposition of HgK gene(s) was detected by mating strains containing both a plasmid encoding HgR (PLY 1 or pCL4) R388, pUB307) tive recipient
elements.
plasmid
selected either for acquisition
designated
[ R388]; TcR, [pUB307]).
by the target
(Sa,
mercury-sensi-
strain of E. coli. Transconjugants
encoded
which was the only resistant
and a target
with a plasmid-free,
We reported previously the isolation of a HgK strain of Yersiniu enterocolitica (Vidon et al., 1981), YE138A14,
Pasteur
ions in certain
(Stanisich
1981) and Proteus mirubilis (Tanaka
Mueller-Hinton
Misra
et al., 1985). It has also been shown that the genes determining
TSB on Luria broth (L broth) or on Hektoen
were
of HgR or a resistance (Cm”[ Sa] ; Tp”,
plasmid
The ratio of the number
of
one among more than 200 strains isolated from raw milk. Although YEl38A14 is resistant to mercuric chloride and merbromin, it is sensitive to the organomercurial derivatives sodium merthiolate and phenyl mercuric borate. This phenotype corresponds to the narrow spectrum of resistance found in a number of mercury-resistant enterobacteria. This paper reports that the HgR of Yersiniu enterocolitica 138A14 is carried on a transposon, Tn3926. This transposon forms part of a nonconjugative plasmid, named pLY1, present in YEl38A14. Some molecular properties of Tn3926 are presented and its relationship to Tn.501 (Bennett et al., 1978) and to Tn21 (Nisen et al., 1977; de la Cruz and Grinsted, 1982) is investigated.
the former to the number transposition frequency.
k1.KI’kRlALS
mutants of Tn21, Tn501 and Tnl721, experiments were executed as described by Grinsted et al. (1982). Derivatives of E. coli UB5201 containing the conjugal plasmid R388, a plasmid carrying the appropriate mutant transposon and a plasmid carrying
AND METHODS
(a) Media Bacteria TABLE Relevant
were grown on TSA (Biomtrieux)
or in
of the latter gave the Donor strains were
counterselected with Nal, Sm, or Rif, as appropriate. Crosses were carried out by growing both donor and recipient strains in mixed culture on Mueller-Hinton agar (18 h, 37’(Z), after which the cells were resuspended in 1 ml to a cell density of approx. 10”’ cells/ml. 0.1 ml of appropriate dilutions were spread on selective agar. The levels of antimicrobials used in selective agar were: mercuric chloride, 12 pg/ml; Km, 12 pg/ml; Nal, 40 pg/ml; Sm, 100 pg/ml; Rif, 100 pg/ml; Tc, 20 pg/ml; Cm, 25 Llgiml; Tp. 25 [[g/ml. Drugs were incorporated in TSA (except when Tp was used; then minimal agar with appropriate supplements or Mueller-Hinton agar was used). To test the ability of Tn3926 to complement tnpA
I properties
of the bacterial
Strain
Species
strains
used Relevant
genotype
Source
or reference
BJ 6183
E. co/i
recBC sbcB end& gul met SW thi bio hsdR
B. Jarry
HB 101
E. co/i
pro leu thi lcrc gal recA rpsL (SmR)
G. Gerbaud
C 600
E. coli
thr leu thi lrrc tmA supE
G. Gerbaud
YE 13XAl4
Y. enrrrocolitica
this study. Vidon et al. (1981)
Nal 4
E. coli
W? F recA .sv CrrgC metA NalR
LIB 281
E. coli
pro, met, NalK
Bennett
and Richmond
(1976)
JC 6310
E. coli
hi\, try, IJS, luc, recA, rpsL (SmR)
Bennett
and Richmond
(1976)
UB 5201
E. coli
pro, met, recA, NalR
Bennett
et al. (1977)
UB 1832
E. coli
his, rry, l.1.3,lm, rpsL, rpoB, RifK
Sanchez
this study.
et al. (1982)
Tn3926
were constructed
E. coli UB1637.
Selection
which had acquired
number ance
crossed
with
was for transconjugants
linked resistance
marker on the mutant total number
and then
transposon.
to Tp and the The ratio of the
of such transconjugants
of transconjugants
which
to only Tp was taken
to the total acquired
resist-
samples
were
mounted
technique
(1969) as described
on grids
of Westmoreland
by Davis
using et al.
et al. (197 1). Phage
$X174 single- or double-stranded was used as internal standard.
DNA (5375 nt)
RESUI.TS AND DlSClJSSION
To test the ability of Tn3926 of TnZI, pCLi7
was transformed
to complement
tnpR
Tn.501 and Trill 721, experiments
were carried out as described Plasmid
DNA
the formamide
as the transposition
frequency. mutants
(e) Electron microscopy
(otherwise
by Diver et al. (1983). pACYC184:
into derivatives
:Tn3926)
of E. coii UB5201
containing one of the test plasmids pJOE562, pUB2589 or pUB2591. Resolution was seen to have occurred when linkage between the ApR determinant and the other resistance determinant(s) on the test plasmid was broken.
(c) Isolation of plasmid DNA (i) Rapid preparation. Rapid plasmid preparation was performed essentially as described by McCormick et al. (198 1). Plasmid DNA isolated by this method was used to determine plasmid size after electrophoresis in 0.7% (w/v) agarosc gels by comparison with standard plasmids. (iij Large-scale isolation of plasmid DNA Plasmid DNA was isolated using a Triton X-100 cleared-lysate procedure (Davis et al., 1980). 500 ml overnight cultures in L-broth were used as starting material. DNA was recovered from agarose scribed by Hubert et al. (1980).
(d) DNA-DNA
gels as de-
hybridization
DNA from 17; (w/v) agarose gels was transferred to Schleicher & Schuell nitrocellulose sheets according to the procedure of Southern (1975). Plasmid DNA probes were prepared by nick translation (Maniatis et al., 1975). Hybridization was carried out in heat-sealable plastic bags at 42°C for 20 h with a 3”P-labelled probe (1-5 x lo6 cpm) as described by Maniatis et al. (1975). Filters were autoradiographed at -2O’C for 48-168 h.
(a) Plasmid content of YE138A14 YE138A14 merbromin
is resistant
to mercuric
but not to merthiolate
chloride
and
nor to phenyl
mercuric borate. The strain contains two plasmids: one of 30 kb (PLY 1) and one of 13 kb (pLY2), as determined by agarose gel electrophoresis. Electron microscope contour length measurements gave values of 31.6 kb and 12.5 kb for pLY1 and pLY2, respectively, in good agreement with the values obtained from gel electrophoresis. HgK was not transferred by conjugation. To determine if HgR was related to extrachromosomal DNA, we extracted plasmid DNA from the agarose gel and used it to transform E. coli BJ6183. Hgn transformants were selected. These were recovered when pLYI, but not pLY2, was the transforming DNA, and such transformants contained a plasmid that comigrated with PLY 1. Plasmid DNA isolated from these transformants was able, in turn, to transform E. co/i HBlOl to HgK. (b) Mobilization and transposition of mercury resistance and isolation of the recombinant plasmids All attempts to transfer HgR by conjugation from YE138A14 to E. coli Na14 were unsuccessful, both at 37 “C and at 28’C. Consequently, mobilization of the HgR determinant by the R plasmids Sa, R388 and pUB307 was investigated (see MAT‘ERIALS AND METHODS, section b). HgR transconjugants were isolated from all crosses at a frequency of about lo-‘. Five of the recombinant plasmids, designated pCL4, pCL5, pCL6, pCL7 and pCL9 (see Table II), were chosen for further study. All but pCL.5 were larger than the parent plasmid and the phenotypes conferred by the recombinant plasmids were those of the recipient plasmid plus HgR (see Table II). Comparing the restriction digest of plasmids obtained during such crosses with those ofthe parent plasmids (not shown) we could determine that PLY 1 was not
TABLE
II
Plasmids.
host cells and bacterial
Plasmids
Relevant
pLYl
HgK
strains
used Construction
characteristics“
source this paper
PLY?
this paper gift of N. Dattab
Sa
IncW. Tra, SmR, Kmn, CmR, SuK
Ward
and Grinsted
(19X2)
R388
IncW, Tra, SuR. TpR
Ward
and Grinsted
(1982)
pUB307
IncP, Tra, NmiKm,
Bennett
pBR322
TcR. ApR
pACYCl84
TcR, CmR
pVSl
Sun. HgK
pCL4
IncW,
Ten
et al. (1977)
Gift of G. Loison Gift of V. Stanisich‘
Tra,
SmR. KmR, CmR, Sun,
Sa::Tn3Y26’
this paper
HgR pCL5
IncW, Tra, Smn. KmR, SuR, Hgn
Sad::Tn3Y26”
this paper
pCL6
IncW. Tra, Sun, Tpn, HgR
R388::TnSY26’
this paper
pCL7
IncP, Tra, NmK:KmK.
Ten, HgR
pUB307::Tn3926”
this paper
pCL9
IncP, Tra, NmR:KmR.
TcR, HgR
pUB307::T1r3926~
this paper
pCLl7
CmK, HgK, TcK
pACYC184::Tn3926
this paper
pUB78 1
ColEI ::TnSOl
p U B8 I0
Hgn CmK
pUBXlX
TcR, ApK
pUB2401
Cmn,
pUB2402
TcK, SmK:SpH,
pUB2406
Cmn
SmR/SpR,
HgR, SuR SuK, HgR
of pDS6501
Gift of J. Grinstcd
deletion
derivative’
of pJOE105
Gift of J. Grinsted
pACYC184
(rer::TnZly
pACYC184
(ccrt::Tn21)’
EcoRI deletion
Gift of J. Grinsted Gift of J. Grinsted
derivativek
of
Gift of J. Grinsted
I Gift of J. Grinsted
pBR322::TnZlA
ApK TcR
et al. (1978)
derivativeh
pUB240 pIJB3321
Bennett
deletion
carrying
the same Tn21 EcoRI
dele-
tion as pUB2406 ptiB2575
Tpn, TcR
R388::Tn1721
pJOE562
Apn. KmR
pBR322
derivative
tro and carrying flanked
by direct repeats
Cointegrate
ApR. TpR, SuR
pUB2589
constructed
generated
tion of Tn8/3
in vi-
a KmR determinant
R. Schmitt
via J. Grinsted
(Altenbuchner
and Schmitt,
19X3)
of Tnl721 by transposi-
J. Grinsted
from pBR322::Tn813
to R38X Apn. Tpn. SuR, KmR
pUB2591
Cointegrate tion
generated
of Tn1727
from
J. Grinsted
by transposipJOE529’
to
R388 I’ Symbols
for resistance
’ Dept. of Bacteriology, ‘ Dr. V.A. Stanisich,
phenotypes
Department
cl Plasmid
Sa was introduced
containing
mercuric
were selected probably
chloride
a deletion
into YEl38A14
’ Plasmid pCL6 was constructed
” pIJBXI0 (Grinsted repeats
Hammersmtth University, (Lesage
by Novick
Hospital,
Bundoora
Ducane
et al. (1976). Road,
WI2 OHS (U.K.)
(Australia).
et al., 1975). Transconjugants
YEl38Al4(Sa)
London
3083, Melbourne
were selected
on Hektoen
agar
were in turn crossed with E. co/i Nal4 and transconjugants
resistance. Sa. The Cmn gene is lost. The deletion
recombination
across
the short homologous
to occur with Sa itself in both UB28l by transforming
(Cohen
is not adjacent
sequences
and UB5201
flanking
(P.M. Bennett
et al., 1972) pLY1 into the rerA
to the Tn3Y26 insertion, the CmR gene (Ireland,
and V.G. Krishna,
strain
UB5201
(R388).
but 1983).
unpublished). Transformants
both plasmids were. in turn, crossed with E. coli JC6310. Transconjugants were selected for Sm and mercury resistance. pCL7 and pCL9 were constructed by mtroducing pCL3 in the ret strain UB5201 [pUB307] by conjugation. TranscoirJuganta
vvcre in turn. crossed of Glasgow).
La Trobe
by conjugation
of 5.2 kb of plasmid
We have also shovvn this deletion
follow those proposed
School,
and Km. These transconjugants
arose due to host-dependent
harbouring ” Plasmids
by plasmids Medical
of Microbiology,
for Nal and mercury
’ pCL5 contains
conferred
Royal Postgraduate
pDS6501
are intact,
with E. w/i UB1832.
Progeny
et al., 1982) is a deletion is a pACYCl84::TnSOl
but all other functions
of these crossed
derivative
of pDS6501
recombinant
plasmid.
have been lost or damaged.
were selected (obtained
for Rif, mercury
and Tc resistances.
from Prof. D. Sherratt,
The 6-kb deletion
is fully contained
Dept. of Genetics,
University
within Tn501. The inverted
a
b
a 12
1234
2
3
4
2 .6kb
Fig. 2. Comparison
of plasmids
(1 “b) slab gel electrophoresis Fig. I. Comparison
of plasmids
Sa, pCL3,
restriction
fragments
ofplasmids:
(1) Sa; (2) pCL4; (3) pCL5. (b)
autoradiographs
Southern
blot autoradiographs
of EcoRI
ffindII1,
plasmids
(1) Sa; (2) pCL4; (3) pCL5, 3”P-labeled PLY i DNA.
translated.
pCL5. digested
hybridized
(a) EcoRi DNAs
EeoRI,
of
to nick-
’ pUB818
(Grinsted
DNA
(4) SalI,
et al., 198 I) is a insertion
derivative
digested
by (1) EcoRI,
hybridized
k pUB2406
(de la Cruz fragment
’ pJOE529, generated
blot (2)
to nick-translated,
pCL4 DNA.
(c) Verification of Tn3926 on recombinant plasmids The relationship between pLY1 and pCL4 and pCL5 was investigated by DNA-DNA hybridization. “2P-labelled pLY1 was used as a DNA probe against Southern blot transfers of pCL4 and pCL5 digested with EcoRI (Fig. 1). Plasmid pLY1 did not hybridize to Sa DNA but did hybridize with two fragments each of pCL4 (one of 2.6 kb and one larger fragment) and two fragments of pCL.5 (one of 2.6 kb and one larger fragment). In the reciprocal hybridization using 12P-labelled pCL4 DNA against a Southern blot transfer of PLY 1 digested with EcoRI, pCL4 hybridized with two fragments of PLY 1 (one of 2.4 kb and one of 9.3 kb, Fig. 2). Comparison of restriction digests of Sa, pCL4 and pCL5 showed that the 2.6skb fragment
of pJOElO5.
of Tn I72i into a derivative
B pUR2401and pUB2402 (de la Cruz and Grinsted,
EroRl-EcoRI
by (I)
(b) Southern
----
et al., 1982) is a deletion
the IL’?gene, and in pUB2402
pJOE529
of pL.Yl
1 DNA digested
(4) S&I.
_
-~.I_--
encodes
(3) BarnHI,
(3) BarnHI,
‘*P-labeled
mobilized and that each HgR transconjugant contained a recombinant plasmid comprising the conjugative plasmid (Sa, R388 or pUB307) and part of pLYI. On the other hand the recombin~t plasmids showed the same DNA sequence inserted into two different sites in Sa (generating pCL4 and pCL5) and into two different sites in pUB307 (generating pCL7 and pCL9). Insertion into R388 generated pCL6. These data are consistent with the interpretation that the HgR determinant originating in YE138A14 and carried on pLY1 is part of a transposable element. The element is designated Tn3926. Tn3926 was, in turn, transposed from pCL6 to pACYC184 to generate pCL17 and its integrity was confirmed by showing that it could retranspose to R388 at a frequency of 10e5.
(Sch6ffl
(2) HindIII,
PLY1 and pCL4. (a) Agarose of PLY
insertion
and Grinsted,
Deletion
overlaps
part of the mpA gene of Tn1721.
pJOE105
of pBR322.
1982) are recombinants
of pACYC184
and TnZI.
In pUB2401
insertion
is into
is into the cat gene. 1982) was generated
after EcoRI
digestion
of pUB2401.
This plasmid
has lost the inner
of Tn21. from the pBR322 derivative
KmK by virtue of the insertion was kindly supplied
plasmid
pJOElO0
(Schbf?l et al., 1981), carries Tni727.
of the KmR gene of Tn5 into the H&d111 site of TnJOl.
by R. Schmitt.
Tn1727
a derivative carries
ofTnSOI
which
the res site of TnSOI.
84 EBt3H
h
p
BhB
h I
E
B
h I
P
hhBB Illi
t
I
/
,
hBB
H
h I
II
I
I
/
EP iI
E
i
&_
..---
.__
Fig, 3. Restriction E, EcoRI; PwII, acetate,
fragments
_-__p-*
Tn 3926
map of pCLl7.
H, HirzdIII;
were obtained
generated
___
h, HitidIl;
Length
of restriction
from Miles or BRL. Digestions were analysed
10 mM disodium
EDTA,
fragments
B, Rgll; P, PvuII. EcoRI, Hindll, on horizontal
were performed
agarose
pH S.3) or Tris borate
HindIll,
were purchased
as described
of pCL17
Comparison of restriction digests of pACYC 184 and pCL17 indicated that the latter was generated from the former by the insertion of a single 7.8-kb DNA sequence with the restriction map presented in Fig. 3. The insertion, Tn3926, has two EcoRI sites, one site each for HindIII and PvuII, six Hind11 sites and seven BglI sites. of Tn3926 to TnSUZ and Tn2I
Transposons Tn21 and Tn501 also confer resistance to mercuric ions and merbromin (Nisen et al., 1977; de la Cruz and Grinsted, 1982; Stanisich et al., 1977; Bennett et al., 1978). The relationship of Tn3926 to these elements was examined, therefore, using DNA-DNA hybridization. (1) Hybridization to Tn501 “‘P-labelled pLY1 DNA was hybridized to Southern blots of pUB78 1, a ColEl : : Tn501 derivative, digested with BglI and PvuIl, and BglI and E’coRI. Plasmid pLY1 hybridized with four BgZI-generated fragments of pUB781 (A,B,C,D), four PvuII
pACYC
location
184
----.--__*
of the boundorics
from Boehringer-Mannheim;
by Grinsted
slab gels using either Tris acetate
to Sa.
(e) Hybridization
is given in kb. The precise
buffer (Petrocheiiou
was derived entirely from Tn3926. Furthermore, the fact that, in addition to the 2.6-kb EcoRI fragment, both pCL4 and pCL5 display only one other EcoRI fragment with sequence homology to PLY 1 led us to conclude that one of the two EcoRI sites of Tn3926 must be located at or very close to one end of the clement. These results con~rmed the conclusion that DNA sequences, i.e., Tn3926, had transposed from PLY 1
(d) Characterization
~------_
et al. (1978). Restriction
buffer
is uncertain. Bg/I, and endonucleasc-
( 150 mM Tris OH. 50 mM sodium
et al., lir’lh}.
fragments (A,B,D,E), live fragments generated with BglI plus PvuII (A,B,C,E,F) and three generated with BglI plus EcoRI (B,D,E) (Fig. 4A). The degree of hybridization to the various fragments was not uniform and appeared to be most efficient with Bg0 fragment C, PvuII fragment A, BglI-PvuII fragment E and Bg!I-EcoRI fragment E, all of which include either part of, or the entire gene for mercu~ reductase. Less intense hybridization was observed between PLY 1 sequences and fragments of pUB78 1 derived from the transposition region of Tn5OI. A reciprocal hybridization indicated that “Plabelled pUB781 DNA hybridized to seven fragments of pCL17 generated with Hind11 plus EcoRI (fragments A,B,C,D,G,H,I, Fig. 4B). With the exception of fragment A, all of these fragments are derived from Tn3926. Fragments A,C,D and H show more intense hybridization than do fragments B,G and I. Fragment A contains the replication region of pACYC184 which is related to that of ColEl (Stuber and Bujard, 198 l), and so hybridization between pUB781 (otherwise ColEl : : Tn501) and pCLl7 (otherwise pACYC184 : : Tn3926) was to be expected. Hybridization to other fragments of pCL17 confirms that there is homology between Tn3926 and Tn501. The transposition functions of Trill 721 have been shown to be very closely related to those of Tn501 (Altenbuchner et al., 1981; Grinsted et al., 1982). In agreement with this result and results reported above we found that Tn3926 displayed homology with Tn1721 (not shown). (2) Hybridization to Tn 2 1 Tn3926 was also compared with Tn21 which is known to show homology with Tn.501 (Grinsted et al., 1982). ASP-labelled pLY1 was hybridized
to
85
1 b
a
4
3
2 a
a
b
b
a
Tn 501 res
pvu
ttlpR
A*
fl
a
b
tnpA
Fig. 4. Hybridization
of Tn3926
to TnSOI. (A) Hybridization
is shown on the bottom. hybridization).
Agarose
Length
has been described
to pCL17
of restriction
fragments
(1“()) slab gel electrophoresis
I b, Zh, 3b, 4b. (B) Hybridization pCLl7
bctwecn
in Fig. 3. Agarose
is shov,,tn in lanes (b).
between
pUB781
pCLl7
is given in kb.
+
(a ColEl ::TnSOI
and pLY1 labelled with “I’. The map ofTn501
(Bennett
digested
by a mixture
+
derivative)
digested
of HilldIl
by
et al.. 1978; Altenbuchner
(A, EcoRI, +. PvuII. V, Bgll. Asterisks:
is shown in la, _?a, 3a, 4a, and hybridization
( I ‘I,,) slab gel electrophoresis
B*
E*
D*
l
Rx/I-Portll; (3) PvuII; (4) Bg/I-EcoRI,
b
of “P-1abelled
+ EcoRI and pUB781
bands
(1) Bgil; (2) ct al., 19x1) that shop
a
pLYl to plJB7XI
in
labelled with “P, The map of
is shown in lanes (a) and hybridization
of “P-labellcd
pUB7XI
X6
1 a
2 a
b
b
UB2402
A
C
F
t-
Tn21A
E
pUB2406
0
Fig. 5. Hybridization
ofTn3926
to Tn21. Hybridization
PLY I DNA. The map of pUB2402
EcoRI). pUB2406
Agarose
and pUB2406
(I “,,) slab gel electrophoresis
is shown
in lanes
8.7
5
ofpUB
(shown is shown
t
(1) and pUB2406
at the bottom) in lanes
(2), both digested
have been described
la, 2a and hybridization
by EcoRI, with nick-translated (1982); (7, I with pUB2402 and
by de la Cruz and Grinsted of 72P-labelled
PLY
lb, 2b.
Southern blots of EcoRI-digested pUB2402 and pUB2406 (pACYC184 : : Tn21 derivatives). Plasmid pLY1 displayed homology with fragments A,C,D and G of pUB2402 and with fragments A and B of pUB2406 (Fig. 5). Since pLY1 did not hybridize to
pACYC184 itself (not shown), then the hybridization noted in these experiments indicated hybridization of Tn21 sequences. Hybridization was most efficient with fragments D and G from pUB2402 and fragment B from pUB2406, fragments known to carry
87
sequences
encoding
the mercuric
Tn21 (de la Cruz and Grinsted, hybridization
to fragments
reductase
gene of
1982). In contrast,
A and C from pUB2402
and fragment A from pUB2406, which quences derived from the transposition
carry segenes of
end-products
position functions
of mutations
in the trans-
of Tu22, TnSOZ and Tn1721
by
of pUB810
pVSS82, ment
which carries
such as Tn21,
Tn5UI
and Tnf 721
transpose in a two-stage process which uses transposase function ft3zpA) for the first stage to generate cointegrate molecules (Arthur and Sherratt, 1979; Shapiro, 1979; Grinsted et al., 1982; Diver et al., 1983), which are resolved in the second stage to yield the transposition end product, together with a DNA molecule indistinguishable from the original transposon donor (Arthur and Sherratt, 1979; Shapiro, 1979). This second stage involves a site-specific recombination system comprising a tnpR gene which encodes the resolution enzyme, resolvase, and a res site, the site at which the resolvase acts. The hybridization experiments clearly indicated homology between Tn3926 and those sequences of Tn501, Tn1721 and Tn2I encoding transposition functions. Hence experiments were undertaken to determine if Tn3926 encodes functions which can complement one or more of the functions encoded by Tn21, Tn501
and Tn1721.
(1) Transpusase (tnpA) function Plasmid pUB8 18 carries a copy of Tn 1721 with a deletion that has removed part of the tnpl4 gene. The remainder of the element still encodes TcR and can transpose if complemented (Grinsted et al., 1982). We were unable to detect any complementation mediated by PLY 1 or pCL6 (frequency < 6 x lo-‘), although in control experiments pUB2575, which carries Tn1721, did complement to give a transposition frequency for the TcR of pUB818 of 2 x 10-h. Plasmid pUB810 carries a deleted Tn501. Both end-points of the deletion are within the element but it has inactivated both the HgR determinant and the transposition functions. When appropriately complemented, however, the deleted element generates cointegrates, rather than normal transposition
(containing
1.5 x lo-‘). Tn501
of the
and cointegrates
a frequency Transposons
1979; Shapiro, is a self-trans-
into R388 or pUB307,
of detection
transposition
pUB810
Tn 3924
DNA
missible plasmid, then, such cointegrates
tively (limit (f) Complementation
and Sherratt,
the recipient
pUB8 10) encode CmR and can be conjugally transferred. Neither pLY1 nor pCL6 mediated cointegration
Tn21 was less efficient.
(Arthur
1979). When
of about
intact,
respec-
In contrast, did comple-
residual
element
on
with R388 were formed at 10m4, as expected
(Grinsted
et al., 1982). Hence, neither pLY 1 nor pCL6, both of. which carry Tn3926, mutant
TnSOf
complement
or Tnl721
transposition
elements.
of
in contrast,
complementation of a mutant Tn21 was detected. Plasmid pUB2406 is a deletion derivative of the pACYC184: : Tn21 recombinant pUB2401 (Grinsted et al., 1982) and plasmid pUB3321 contains the same EcoRI deletions of Tn21 as pUB2406 but is a pBR322 : : Tn21 derivative. The deletion removed only Tn21 sequences, but left the ends of the element intact. Both the transposon encoded drug-resistance genes and the transposition functions were inactivated. Nonetheless, the residual element can be complemented to transpose by wild-type Tn2f transposition functions (Grinsted et al., 1982), to generate cointegrates comprising pUB2406 or pUB3321 and the recipient DNA molecule. In the presence of PLY 1, pUB2406 formed cointegrates with R388 (frequency, 1.9 x 10-7), while pCL6 mediated cointegration of pUB2406 and pUB307 (frequency, 1.3 x 10dh). Further pCL17, a pACYCl84: : Tn3926 recombinant also mediated cointegration of pUB3321 and R388 (frequency 4 x IO-“). That the transconjugants generated in these crosses did harbour cointegrates was confirmed by demonstrating that the CmK determinant of pUB2406 was linked to the TpR determinant of R388 because the former marker always cotransferred with the TpK determinant in conjugal crosses, irrespective ofwhich marker was selected. The transconjugants examined each contained a single plasmid, all of which were indistinguishable in size but which were larger than either pUB2406 or pUB3321 or R388. Restriction enzyme digests of some of these (data not shown) displayed fragment proliles which could be distinguished but which were all consistent with the recombinant plasmids being cointegrates of ~1182406 or pUB332 1 and R388 generated by trans-
xx position
of the deleted Tn21 present
on the former
plasmid.
tation of tnpR gene function. to indicate
that Tn3926
These results are taken
does possess
and therefore, by implication, (2) Resolvase (tnpR) function Plasmid
pUB2589
is
cointegrate
of R388
and
Tn813, a tnpR derivative and which encodes resolvase cons
is
pBR322
ofTn2l
mediated
by
(g) Conclusions
(Diver et al., 1983) When the missing
supplied
to yield
to be tested.
a transposon-generated
TpRApRTcR.
activity
resolve
that remains
a tnpR gene,
a res site, a conclusion
the
R388: :Tn813
two (TpK)
repliand
(1) Two plasmids, PLY 1 and pLY2, with sizes of 30 kb and 13 kb, respectively, have been identified within
YE138A14,
a
HgK
wild-type
strain
of
pBR322 : : Tn813 (ApRTcR), and the former plasmid can be conjugally transferred independently of the
Y. enterocolitica. The 30-kb plasmid, PLY 1, encodes resistance to mercuric ions and merbromin. The Hg”
latter. Plasmid pUB2591 is a cointegrate of R388 and pJOE529, generated by transposition of the Tn1727 element (a derivative of Tn501 constructed in vitro
gene(s)
and encoding KmR) carried on pJOE529, and encodes TpKKmRApR. Resolution generates two plasTpKKmK and the other mids, one encoding ApRKmR. Again the former plasmid can be conjugally transferred independently of the latter. Plasmid pJOE562 is a derivative of pBR322 constructed in vitro. It encodes ApRKmK and the KmR determinant is flanked by direct repeats of the Tn1721 res site (Altenbuchner and Schmitt, 1983). Recombination across the duplicate res sites deletes the Kmn gene, which, because it is not longer linked to an origin of replication, is not recovered. Plasmid pCLl7 was transformed into UB5201 containing pUB2589, pUB2591 or pJOE562, and retention of linkage of “cointegrate” markers was determined. In all cases linkage of “cointegratc” markers was stable in the absence of pCLl7 (Table III), while in the presence of pCLl7 the link was severed (Table III), indicative of complemen-
TABLt Integrity Plnsmid
was
belonging
mobilized
by conjugative
to different incompatibility
cally Sa and R388 (both IncW) and pUB307 (IncP). The transconjugants from these experiments contained recombinant plasmids which all bore the same insert located at different sites on the different target plasmids. This recombination occurred in a recA strain, as well as in a Ret + strain. All these results together supported the conclusion that mercury resistance encoded by PLY 1 constitutes part of a transposon now called Tn3926. (2) Tn3926 is a 7.8-kb transposon which contains two EcoRI sites, one located very close to one end of the element and 2.6 kb from the other site. A Hind111 site is located between these EcoRI sites, 0.5 kb from the EcoRI site located at the end of the element (Fig. 3). These data indicate that Tn3926 is. in these respects, similar to Tn2613, another transposon encoding HgK (Tanaka et al., 1983). Other parts of the sequence are not obviously related to Tn2613. The restriction pattern differs from that of the prototype HgR transposon, Tn501, a transposon of almost the same size as Tn3926.
III of plasmids
carrying
two directly
repeated
ret sites in the presence
Linked resistance
Source
determinants
repented
of pCLl7
of directly
Linkage
YESyitc
second -pc1.17
of .ApK to marker’ tpC‘LI7
pJOE562
ApK. KmK
Tnl72l
50:50
I) 100
PUB2589
ApK, 1‘P K Ap’. TpK
‘I 1121
5050
0 100
Tn501
48.5lJ
13 50
pUB2591
I’ Loss of linkage of ApK and KmK (pJOE562) (pl!B2589
plasmids
groups, specifi-
and plJB2591)
was dctcrmined
WBS determined
by conjugal
transfer
by loss of Km” but retention of TpK unlinked
to Ap’
of ApK. Loss of linkage of ApK and Tp”
89
(3)
Tn3926
displayed
Tn501 and Tnl721
homology
with
as shown in hybridization
ments (Figs. 4 and 5). It hybridized
Tn21,
ACKNOWLEDGEMENTS
experi-
most strongly to
We
are
indebted
Schneider, F. Lacroute
zation
mation.
We thank
electron
microscopy
showed
a strong homology
and the left-hand the two EcoRI
sequences
between
of Tn3926,
sites (Fig. 4B). Together
Tn501
defined
by
to
M.
Nguyen-Juilleret,
and A. Mercenier
for materials
J. Menissier study.
Gerbaud,
above data this suggests that the genes for HgR en-
bacterial
coded by Tn3926
advice and a gift of plasmids.
on the left of the ele-
ment (Fig. 3). Homology
between Tn3926
was strong and involved
sequences
the latter element,
and Tn21
at both ends of
one end of which accommodates
genes for Hg R, including a mercury reductase gene. Our data are consistent with the previously observed homology between the mercury resistance genes of Tn501 and Tn21 (Tanaka et al., 1983). (4) The hybridization data clearly indicate homology between sequences carried by Tn3926 and sequences encoding transposition functions on Tn21, and Tn501 (and Tnl721), the transposition systems of which are known to be related (Grinsted et al., 1982; Diver et al., 1983). However, while Tn3926 was able to complement a tnpA mutant of Tn21, complementation of analogous mutants of Tn.501 and Tn 1721 was not observed. However, in that the transposase of Tn21 complements tnpA mutants of Tn501 and Tn1721, but not vice versa, despite the fact that these systems are related (Grinsted et al., 1982) the genetic results are consistent with the interpretation that the tnpA gene of Tn3926 is related to the equivalent genes of these other transposons. Transposon Tn3926 also encodes a function that can substitute for the resolvase functions of Tn21, Tn.501 and Tnl721 (Table 3), which are interchangeable (Diver et al., 1983). The data indicate that the transposition systems of all four elements are related and that there is a common progenitor sequence for all four transposons. Hence Tn3926 is clearly related to the family of transposons, the prototypes of which are Tn21 and Tn501, but is distinct from both. Our data suggest that Tn3926 is more closely related to Tn21 than to Tn.501 in that the former element displays homology with the latter throughout its sequence, and the transposition functions of Tn3926 can substitute for the equivalent gene products of Tn21.
N. Datta strains,
is indebted
or infor-
for her help in the
We are grateful
with the
are located
C.
G. Loison, R. Jund, A. Labigne-Roussel,
the fragments of TnSOl which encode the genes for mercury resistance (Fig. 4A). The reciprocal hybridi-
and V. Stanisich
we thank
to G.
for a gift of
J. Grinsted
for fruitful
One of us (M.C.L.)
to FEBS and EMBO
for financial
sup-
port to stay at the Medical School of Bristol, and to AH. Linton for his hospitality. This research was supported in part by the A.T.P. ‘Microbiologie’ No. 1482 from the Centre National de la Recherche Scientilique.
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