Family of Class 1 Integrons Related to In4 from Tn1696

doi:10.1128/AAC.45.11.3014-3020.2001

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Antimicrobial Agents and Chemotherapy, November 2001, p. 3014-3020, Vol. 45, No. 11
0066-4804/01/$04.00+0 DOI: 10.1128/AAC.45.11.3014-3020.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Family of Class 1 Integrons Related to In4 from Tn1696

Sally R. Partridge,¹^,² Gavin D. Recchia,¹^,²^, H. W. Stokes,² and Ruth M. Hall¹^,^*

CSIRO Molecular Science, North Ryde, New South Wales 2113,¹ and Department of Biological Sciences, Macquarie University, Sydney, New South Wales 2109,² Australia

Received 26 March 2001/Returned for modification 11 June 2001/Accepted 5 August 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The class 1 integron In28, found in the multidrug resistance transposon Tn1403, was found to be located in the res site ofthe backbone transposon and is flanked by a 5-bp direct duplication,indicating that it reached this position by transposition. In28has a backbone structure related to that of In4, but has lostinternal sequences, including the sul1 gene, due to an IS6100-mediateddeletion. In28 also lacks the partial copy of IS6100 found inIn4 and contains different gene cassettes, blaP1, cmlA1, and aadA1.In1, the class 1 integron found in the multidrug resistance plasmidR46, is also located in a putative res site and belongs to theIn4 group. In1 has a shorter internal deletion than In28 and hasalso lost one end. Additional integrons with structures relatedto In4 were also found in databases, and most of them had alsolost either one end or internal regions or both. Tn610 belongsto thisgroup.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The integrons found in clinical isolates of gram-negative bacteria generally contain one or more integrated cassettes thateach include an antibiotic resistance gene, and a large numberof gene cassettes containing different resistance genes have beenidentified (15, 17, 18, 42). Though integrons belongingto three classes have been found in clinical and environmentalstrains of multidrug-resistant bacteria (15, 42, 48), class1 integrons predominate. Despite enormous variation in both thenumber and the identity of the cassettes associated with any individualintegron isolate, integrons belonging to integron class 1 haveidentical or nearly identical integrase genes (intI1). Furthermore,class 1 integrons are present in many of the earliest multidrug-resistantplasmids isolated. The plasmids NR1 (R100), which is the sourceof Tn21, and pSa were both isolated in Japan, NR1 in the late1950s (35, 55) and pSa prior to 1968 (56). Both are nowknown to contain a class 1 integron (9, 29, 48-50). R46, R751,R1033, and R388, plasmids from resistant strains isolated in Europeduring the 1960s and early 1970s, are also known to contain class1 integrons (9, 20, 36, 41, 48, 50). Indeed, it ispossible that that class 1 integrons may have already been presentor even widely distributed in bacteria prior to the introductionof antibiotics as human therapeutics (1, 54) and subsequentlymoved into human pathogens. The variety of backbone structurespresent in class 1 integrons (8, 16, 36, 41) also suggestsan evolutionary history for these elements that is far longerthan the 50 years of extensive antibioticuse.

In addition to the intI1 gene, encoding the site-specific recombinase (32) that is responsible for cassette insertion (11),class 1 integrons also include the attI1 site (37, 43) intowhich the cassettes are incorporated and a promoter, P_c, thatdirects transcription of the cassette-encoded genes (12). Thesethree features are found in a module of 1.36 kb known as the 5'-conservedsegment (5'-CS) (20, 48). The 5'-CS is bounded at the innerend by attI1 and at the outer end by IRi, which is a 25-bp sequencethat is found as an inverted repeat, IRt, at the other end ofclass 1 integrons (8, 20, 36, 41). The 5'-CS or intI1module is found in all class 1 integrons and is generally followedby a variable region that consists of an array of one or moregene cassettes. To the right of the last cassette, or adjoiningthe 5'-CS if no cassettes are present, two different sequenceshave been found (Fig. 1). Most of the class 1 integrons studiedto date contain at least part of a region known as the 3'-conservedsegment (3'-CS) (8, 16, 48). The longest 3'-CS segment(2,384 bp) is found in In5 (8). It includes the sul1 gene,conferring resistance to sulfonamides (48, 50); the qacE $Delta$ 1gene, conferring marginal resistance to quaternary ammonium compoundssuch as antiseptics and disinfectants (38); and two open readingframes (ORFs) of unknown function, orf5 and orf6 (36, 48).However, sometimes the 3'-CS is not present. The transposon Tn402is a class 1 integron that does not include the 3'-CS (41),but is likely to represent the ancestor of integrons that do.Tn402, which is found in plasmid R751, is an active transposon(23, 47) that includes a set of three genes tniA, -B, and-Q, that are required for transposition (24, 41). A fourthgene, tniR, encodes a resolvase that is presumed to be involvedin the resolution of the cointegrates that are formed as transpositionalintermediates (24).

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FIG. 1. Structure of the backbones of class 1 integrons. Each integron is bounded by 25-bp inverted repeats, designated IRi and IRt (vertical bars labeled i and t), and includes the 5'-CS (medium line), which begins with IRi, contains the intI1 gene, and ends at the vertical arrow in the attI1 site (narrow open box). This arrow marks the position of integrated cassettes, which are not shown. Parts of the 3'-CS (narrow line) and the tni module (thick line) are found to the right of the vertical arrow. Insertion sequences are shown as open boxes. (a) Tn402 (also called In16 or Tn5090) includes the complete tni module that contains a full set of transposition genes (tniA, -B, and -Q), a resolvase gene (tniR), and a res site (solid box). Tn402 contains an array of three cassettes, dfrB3, orfD, and qacE. (b) In5 includes the 3'-CS, containing qacE $Delta$ 1, a truncated version of the qacE cassette, the sul1 sulfonamide resistance determinant, orf5 and orf6, and part of the tni module. In5 has a single cassette, aacA(IIa). (c) In4 includes two copies of very short regions of the IRt end of the tni module separated by a complete copy of IS6100 and a partial copy consisting of the last 321 bp of IS6100 ( $Delta$ ). The cassette array is aacC1-orfE-aadA2-cmlA1.

The class 1 integrons that contain the 3'-CS appear to have arisen from an ancestor with a Tn402-type backbone by incorporationof the genes (qacE $Delta$ 1, sul1, orf5, and orf6) that make up the 3'-CS.Indeed, the complete qacE gene is part of a gene cassette (42).This structure has become an integral part of the types of class1 integrons that are now widely distributed among plasmids, amongbacterial species and genera, and geographically. However, theclass 1 integrons that include 3'-CS sequences have undergonefurther rearrangements. All of those studied to date have lostpart or all of the tni module and are now transposon derivativesthat are defective in self-transposition. Most have also lostpart of the 2,384-bp region defined as belonging to the 3'-CS.One group, here called In5-type class 1 integrons (Fig. 1b), wereoriginally identified as containing IS1326 and have lost partsof the 3'-CS and of the tni module, presumably due to IS1326-mediateddeletion of DNA adjacent to the insertion sequence (IS) (8).Further members of this group resemble In5 or In0 but have lostIS1326 (27, 41). A second backbone structure (Fig. 1c) hasrecently been found in integron In4, which constitutes the centralregion of transposon Tn1696 (GenBank accession no. U12338)(36). In4 contains one complete copy of the insertion sequenceIS6100 and an adjacent partial copy in the same orientation. TheIS6100 region is flanked by short segments from the outer right-handend (IRt end) of Tn402 and other class 1 integrons, and thesesegments are in inverse orientation. The outer and inner copiescorrespond to the last 152 and 123 bp of Tn402,respectively.

Here, we have examined additional class 1 integrons, In28 and In1. In28 is found within the transposon Tn1403 (28, 53),which was recovered from a clinical strain of Pseudomonas aeruginosawhich was isolated in the United States in 1973-1974 (26) andcontains the IncP-2 plasmid RPL11. RPL11 transfers resistanceto gentamicin, carbenicillin, streptomycin, tetracycline, sulfonamides,chloramphenicol, and mercury (26), while Tn1403 confers resistanceto only carbenicillin, streptomycin, spectinomycin, and chloramphenicol(28, 53). In1 is found in the multidrug resistance plasmidR46, originally from a Salmonella enterica var. Typhimurium clinicalstrain isolated in the United Kingdom prior to 1966 (33). In28and regions adjacent to both In28 and In1 were sequenced, andboth of these integrons were found to be members of the In4 group.The relationships of these integrons to others found in the databasesare alsoreported.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains and plasmids Escherichia coli JM109 [( $Delta$ lac-proAB) supE thi F' (traD36 proAB⁺ lacIq lacZ $Delta$ M15)] was used to propagate plasmid DNA. Plasmidsused in this work are shown in Table 1. Fragments from R388::Tn1403were cloned into either pUC19 (58) or pACYC184 (10) by standardprocedures (45). Plasmids containing the appropriate fragmentswere identified by screening for antibiotic resistance, by restrictionmapping, and by sequencing the fragment ends using a universalprimer. Subclones were also derived from these primary clones.pRMH519 was constructed by SacI digestion and religation of pRMH518.pRMH527 was constructed by digesting pRMH519 with SalI and religating.Bacteria were routinely cultured at 37°C in Luria-Bertani (LB)medium or on LB agar supplemented as appropriate with ampicillin(100 µg ml¹), chloramphenicol (25 µg ml¹), streptomycin (25 µg ml¹), or sulfamethoxazole (25 µg ml¹). Antibiotics were obtained from Sigma.

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TABLE 1. Plasmids

DNA isolation and restriction mapping. Plasmid DNA for restriction analysis and cloning was isolated using an alkaline lysis method (3). Restriction enzymes wereused in accordance with the manufacturers' instructions. Fragmentswere separated by electrophoresis on 1% (wt/vol) agarose gelsand visualized by staining with ethidium bromide. An EcoRI digestof bacteriophage SPP1 (Geneworks) was used as size markers. PlasmidDNA for sequencing was purified using the Magic Minipreps DNApurification system (Promega) or Wizard maxiprep kit(Promega).

DNA sequencing and analysis. The DNA sequence of at least one strand of fragments of Tn1403 cloned in plasmid vectors was determined. Manual DNA sequencingwas performed with a Sequenase 2.0 system (51) as recommendedby the manufacturer (U.S. Biochemicals) using dITP reaction mixturesfollowed by a 30-min incubation with a 1 mM deoxynucleoside triphosphatemix and terminal deoxynucleotidyl transferase (Boehringer-Mannheim).Automated sequencing was performed by the Sydney University/RoyalPrince Alfred Hospital, Sydney, or by the sequencing facilityat the Department of Biological Sciences, Macquarie University,Sydney, on an ABI-Prism 377 sequencer using the Big Dye system.The additional R46 sequence was determined as described by Halland Vockler (20) using M13 clones isolated in the course ofthat original study. DNA sequences were assembled using MacVector6.5 and AssemblyLIGN (Oxford Molecular). GenBank searches wereperformed using the BlastN and FastA programs available throughWebANGIS (Australian National Genomic Information Service). Programsin the GCG Wisconsin package, version 8.1.0, were used via WebANGISGCG to align and analyze DNAsequences.

Nucleotide sequence accession numbers. The In28 nucleotide sequence data reported here have been assigned GenBank accession no. AF313472. The additional sequenceof R46 reported here has been added as GenBank accession no. M95287.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Structure of In28. Tn1403 is a transposon isolated from a clinical strain of P. aeruginosa (28, 53) and confers resistance to carbenicillin,streptomycin, spectinomycin, and chloramphenicol, but not to sulfonamides.The most recent published map indicates the presence of blaP1(PSE-1), cat, aadA, and aphC antibiotic resistance genes (53).An intI1 gene was also shown, and the IRi end of the 5'-CS wassequenced, but the restriction sites characteristic of the 3'-CSare not present, consistent with the absence of sulfonamide resistance.Here restriction fragments that include most of Tn1403 were isolated,and a map of Tn1403 was constructed (Fig. 2). This map differsfrom the published map, as some restriction sites have been added,removed, or relocated. The sequences of In28, the class 1 integronfound in Tn1403, and of the regions adjacent to it were determined(GenBank accession no. AF313472), and the structure of In28is shown in Fig. 2.

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FIG. 2. Map of Tn1403 and In28. (a) Tn1403. The region shown represents Tn1403, with vertical bars representing the inverted repeats, and In28 is shown as a thicker line ending in bars labeled i and t. The extents of the fragments cloned in various plasmids are shown below. Previously sequenced sections are represented by lines: 1, Huovinen and Jacoby (22); 2, Vézina and Levesque (53); and the extent of the sequence obtained here is indicated by a dotted line. (b) Expanded map of In28. Each cassette is indicated by an open box and adjacent filled box that represents the 59-base element (59-be). Other features are as in Fig. 1. Restriction enzyme sites: B, BamHI; Bg, BglII; E, EcoRI; H, HindIII; P, PstI; S, SalI; Sa, SacI; Sp, SphI; X, XhoI.

The backbone structure is related to that of In4 (36), though the cassettes are different. In28 includes the 1.36-kb 5'-CSthat contains the weak variant of the P_c promoter (TGGACA-17 bp-TAAGCT)rather than the strong (TTGACA-17 bp-TAAACT) version found inIn4, and does not include the 19-bp duplication in attI1. The5'-CS is followed by an array of three gene cassettes, blaP1,cmlA1, and aadA1. The presence of the cmlA1 cassette indicatesthat chloramphenicol resistance is in fact conferred by an effluxmechanism rather than by a chloramphenicol acetyltransferase (Cat).The blaP1 cassette is identical to the previously reported blaP1(PSE-1) cassette (GenBank accession nos. Z18955 and M69058)(22) and confers resistance to carbenicillin and ampicillin.The cmlA1 cassette sequence differs from the prototype in In4(GenBank accession no. U12338) at four positions (three aminoacid changes). The aadA1 cassette confers resistance to streptomycinand spectinomycin and differs at two positions (G732C and C759T)from the prototype aadA1a sequence (GenBank accession no. X12870),but these differences do not result in any amino acidchanges.

To the right of the cassettes, the first 433 bp of the 3'-CS are also present and are adjoined by IS6100. Thus, compared toIn4, both the internal 123-bp copy of the IRt end and the regionof the 3'-CS that contains orf5, orf6, and the sul1 gene are missing.Beyond IS6100 lies the same short segment of 152 bp from the IRtend of the tni module that is present in In4. In28 does not includethe partial copy of IS6100 found in In4. Because this direct duplicationis readily lost from cloned fragments (36), its absence wasconfirmed by DNA-DNA hybridization using digests of R388::Tn1403.The 321-bp PstI fragment created by the presence of the duplicationwas not detected (data notshown).

The sequence of Tn1403 flanking In28 revealed the presence of a 5-bp duplication (boxed in Fig. 3), indicating that In28 reachedits current location by transposition. In28 was located upstreamof the tnpR gene in the resI region of the res site of the transposonthat forms the backbone of Tn1403 (Fig. 3). The sequence to theleft of In28 is identical to that of a short region of Tn1403published previously (GenBank accession no. M59035) (53),and the regions to the left and right are identical to the correspondingregions of a transposon from a multidrug-resistant Pseudomonasstrain isolated from an apple orchard (46). This transposonalso contains a class 1 integron in the same position.

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FIG. 3. Sequence surrounding In28. The Tn1403 sequences flanking In28 have been joined together (bases 195 to 73 of GenBank accession no. M59035 plus bases 6357 to 6452 of AF313472) to reconstitute the res site, and the 5 bp duplicated by insertion of In28 are boxed. This sequence is aligned with the res regions of Tn501 (bases 4750 to 4532 in Z00027), Tn1721 (bases 359 to 160 in K01724), and Tn1696 (bases 3562 to 3669 and 12005 to 12116 in U12338) and the extents of the three components of the res site, determined experimentally for Tn1721 by Hall and Halford (21) and Rogowsky et al. (44), are indicated. The 5-bp duplication in Tn1696 is also boxed.

Structure of In1. We have previously reported that a segment of IS6100 abuts the right-hand end of the region of the 3'-CS present in In1 (16),which is found in the IncN plasmid R46. In In1, only the first2,197 bp of the 3'-CS are present, as opposed to 2,239 bp in In4,and the internal copy of 123 bp from the IRt end of the tni moduleis not found. This suggests that a deletion extending from theleft-hand boundary of IS6100 to base 2198 of the 3'-CS has occurred.The PstI restriction site expected for the right-hand portionof IS6100 is not present in the map of R46 (7), and IS6100appears to be interrupted by an IS26 (IS46) element. The sequenceof this region of R46 has recently been completed (R. Woodgate,personal communication; GenBank accession no. AF117344). Onlythe first 298 bp of IS6100 are present, and they are followedby a complete IS26 (Fig. 4b). The remainder of IS6100 and the152-bp IRt end appear to have been lost, as they are not foundelsewhere in R46 (R. Woodgate, personal communication).

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FIG. 4. Backbone structures of In4-like class 1 integrons and of Tn610. The structures shown are (a) integrons for which the complete sequence is available and both terminal IRs are present; (b) completely sequenced integrons that lack one of the terminal IRs; (c) integrons for which the sequence does not extend far enough to determine if one or both terminal IRs are present; and (d) Tn610. Features shown are as in Fig. 1, and (IS26) indicates that IS26 is found adjacent to the boundary shown. The sources for the sequences used are: In4, GenBank accession no. U12338; In28, AF313472; pHCM1, http://www.sanger.ac.uk/Projects/S_typhi/; DT104, AF071555 and AF261826; In1, M95287 and AF117344; pCG4, AF164956; pACM1, U90945 and AF107205 plus standard 3'-CS (predicted to be present from available restriction maps); A. baumannii In, AJ289190; Tn610, X53653.

The sequence adjacent to the IRi end of R46 was extended and added to that in GenBank accession no. M95287. It includesa gene, designated resP, encoding a resolvase-like protein. Avariant of this resolvase has previously been identified in aderivative of plasmid TP120, which is a relative of R46 (14).In1 is located upstream of resP in the region where the cognateres site would be expected to befound.

Structure of other class 1 integrons. Searches of bacterial sequences present in the databases revealed several additional examples of class 1 integrons with backbonestructures that contain IS6100 and are related to that of In4.Only one of these includes a complete structure extending froman IRi end to an IRt end in the correct orientation (Fig. 4a).It is found in plasmid pHCM1 from a multidrug-resistant Salmonellaenterica serovar Typhi strain and is part of a transposon witha backbone structure closely related (greater than 99.9% identical)to that of Tn1696. The integron is in precisely the same positionas In4 in Tn1696, with the same 5-bp duplication flanking it.In this integron, the internal 123-bp copy of the IRt end is present,but it abuts an unknown sequence, and none of the 3'-CS is present.A possible explanation for this configuration is that a deletionarising at IRt has extended into a previously unidentified cassette.The partial duplication of IS6100 is not present in thisintegron.

Two further examples resemble In1 in that one of the ends of the integron has been lost (Fig. 4b). One of these is the integronin pCG4 from Corynebacterium glutamicum (GenBank accession no.AF164956), which has lost the outer 152-bp copy of IRt, presumablydue to a deletion arising at the right-hand end of IS6100. Thebackbone of the In in pCG4 is otherwise identical to the In4 backbone,except that it lacks the partial copy of IS6100.

The second, from the chromosomal multidrug resistance locus of S. enterica var. Typhimurium DT104, was compiled from GenBankaccession nos. AF071555 and AF261826 (4, 5). It haslost the IRi end and the first 915 bp of the 5'-CS and the partialcopy of IS6100, but is otherwise identical toIn4.

In two further cases (Fig. 4c), the available sequence is incomplete. The sequenced region of plasmid pACM1 from Klebsiellaoxytoca (40) (compiled from GenBank accession nos. U90945and AF107205 and the standard 3'-CS sequence) does not extendto either outer end, but the configuration to the right of thecassette array differs from that in In4 only in that the partialcopy of IS6100 ( $Delta$ in Fig. 4) is missing. In the second case, anintegron found in Acinetobacter baumannii, the 3'-CS is missingand the left-hand end of IS6100 abuts the first 53 bp of the oxa3cassette (39). The right-hand end has been truncated, apparentlyby insertion of IS26 or an IS26-mediated deletion, and only thefirst 14 bp of the 152-bp IRt end fragment remain. The availablesequence does not extend to the IRi end, and it remains to beestablished if this ispresent.

A copy of IS6100 with the 123-bp segment of the tni module adjacent to it is also found in the transposon TnSF1 from Shigellaflexneri (GenBank accession no. AF188331). TnSF1 appears tobe derived from Tn21 and has a class 1 integron in the same positionas In2 in Tn21. This integron seems to have acquired a large blockof extra sequence, including the IS6100/IRt feature, resultingin a complex structure (not shown in Fig. 4).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We have previously shown (8) that one group of class 1 integrons that contain sequences derived from the 3'-CS have backbonestructures related to that of In5. Here, further examples of class1 integrons that may also contain the 3'-CS but have a differentbackbone structure related to that of In4 (36) have been identified.In4 has the longest portion of the 3'-CS found in members of thisIn4-like group and is the only one that includes a partial copyof IS6100 in addition to the complete copy. Though the originof the complex arrangement of IS6100 and IRt ends found in In4remains a matter for speculation, In4 appears to be ancestralto the other integrons that contain IS6100, and all other membersof the group can be viewed as having derived from it. For example,the direct duplication of IS6100 sequences could have been lostby RecA-dependent homologous recombination. Several further differencesare likely to be due to deletions initiated either at the right-handend of the IS6100, leading to loss of the outer IRt end of theintegron, or at the left-hand end of the IS, leading to internaldeletions.

Deletions initiated at the left-hand end have led to loss of the internal 123-bp IRt fragment and different lengths of the3'-CS in In1 and In28, and in the A. baumannii integron, the deletionextends into the cassette array. In the pHCM1 integron, the 3'-CSis also missing, but the deletion appears to have been initiatedat the internal IRt end. Insertion of IS26 or IS26-mediated deletionhas also played a part in shaping these integrons. Tn610 (Fig.4d), a transposon isolated from Mycobacterium smegmatis that confersresistance to sulfonamides (31), is another relative. Tn610is made up of two copies of IS6100 flanking a sequence that consistsof bp 334 to 1333 of the 5'-CS joined to bp 454 to 1663 of the3'-CS. It includes all but the first 4 bp of the sul1 gene. Tn610may well have arisen from an In4-like integron, but in this casepart of the intI1 gene has been lost (presumably due to insertionof the left-hand copy of IS6100) and an internal deletion hasled to loss of part of attI1 and the beginning of the 3'-CS. Asa consequence, Tn610 is no longer an active integron, as it isunable to incorporate genecassettes.

Further examples of the In4-like family of class 1 integrons were identified from published restriction maps. For example,one appears to be present in the IncN plasmid N3 (6), and asmall amount of available sequence confirms this. Part of IS6100and the 152-bp IRt fragment are found where they would be expected,adjacent to the EcoRI restriction-modification genes in N3 (2).Another IncN plasmid, R15, includes the appropriate configurationof restriction sites within a transposon, Tn2353 (13), and Tn2353could be a further relative of Tn1696. Both N3 and R15 are fromShigella strains isolated in Japan prior to 1964 (57).

Most of the In4-like class 1 integrons and integron remnants described here are located on plasmids. A few (In4, In28, andthe integron from S. enterica serovar Typhi) are found withina transposon that is located on a plasmid. Only the DT104 integronis located within the bacterial chromosome of the original isolate,and this is presumably a result of the incorporation of extrachromosomalDNA (e.g., a plasmid) into the S. enterica DT104 chromosome (4).Members of this In4-like group have also been recovered from awide variety of bacterial species. Most are from gram-negativebacteria, but pCG4 is from C. glutamicum and Tn610 was recoveredfrom M. smegmatis. Granted that integrons of this group are foundmostly on plasmids, it is perhaps not surprising that they areso broadlydisseminated.

Though integrons belonging to both the In5-like and In4-like groups are unable to mobilize themselves, having lost some orall of the tni genes, they nonetheless appear to move readily.The sequences flanking them are diverse (8, 16), indicatingpast movement, and only two of the In4-like integrons describedhere, In4 and the pHCM1 integron, are located in the same DNAcontext. If the two outer ends (IRi and IRt) are intact and inthe correct orientation, movement is presumably accomplished whentni genes are present in the same cell to complement the defect.Transposition of Tn402, and presumably also of the tni-deficientIn5-like and In4-like integrons, resembles transposition of theclosely related mercury resistance transposon Tn5053 (24, 25)in that it is constrained by stringent target site specificity,with the target being a res site recognized by a resolvase (23,34). In28, like In4, is located within a res site recognizedby the resolvase encoded by the backbone transposon (Fig. 3).This location presumably interferes with the normal transpositionprocess for Tn1403 and Tn1696. Indeed, cointegrates formed ontransposition of Tn1403 are not resolved (53). The IRi end ofIn1 is also adjacent to a plasmid gene, here called resP, encodinga resolvase-like protein and may be located within the cognateres site. A resolvase-like protein is encoded by a gene near theIRi end of the pCG4 integron (Fig. 5). Indeed, genes that encoderesolvases are also found adjacent to the IRi end of most class1 integrons (Fig. 5). Tn402 (not shown in Fig. 5) is an exception(52).

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FIG. 5. Locations of resolvase genes adjacent to class 1 integrons. Integrons (a) found in transposons and (b) found in plasmids. Open bars labeled i and t indicate the outer IRi and IRt ends of the integron. ( $-$ ) indicates that the outer IRt is not present, and (?) indicates that the sequence of this region has not been determined. The genes encoding resolvases or resolvase-like proteins are shown by thick arrows and are labeled tnpR for transposon genes, resP for plasmid genes, and res for the DT104 gene, whose origin is not known. Other genes and open reading frames are shown by thin arrows. The res sites (solid boxes) are shown only where their locations and extents have been determined experimentally or can be deduced by comparison with an experimentally determined res site (21, 30, 44). The sources of the sequences are: Tn1403/In28, AF313472 and M59035; Tn1696/In4, U12338; Tn1412/In32, L36547; Tn21/In2, AF071413; R46/In1, M95287; pVS1/In0, U10456 and U49101; pSa/In6, U303471; pMG7, S78872; pCG4, AF164956; and DT104, AF071555 and AF261826.

It is clear that class 1 integrons with the In4-like backbone structure described here or with an In5-like backbone describedpreviously (8) are widely distributed. Both types are foundamong integrons from early clinical isolates of multidrug-resistantstrains, indicating that the differences may have arisen priorto the introduction of most antibiotics for extensive therapeuticuse. However, sulfonamides were in use for over 10 years beforethe first use of penicillins, and selection for class 1 integronscontaining the 3'-CS, and hence the sul1 gene, may have occurredin that time span. In4-like class 1 integrons are found in a varietyof plasmids and transposons as well as in bacterial chromosomesand clearly change their location relatively easily, despite havingdispensed with the tni genes. Their location becomes fixed onlywhen one of the outer ends, IRi or IRt, is lost. They are alsofound in many different bacterial species, presumably as a resultof their association with plasmids ortransposons.

	ACKNOWLEDGMENTS

We thank Cassandra Vockler for determining the R46sequence.

S.R.P. was supported by a grant from the Australian National Health and Medical Research Council. S. enterica serovar Typhisequence data were produced by the S. enterica serovar Typhi sequencinggroup at the Sanger Centre and can be obtained from http://www.sanger.ac.uk/Projects/S_typhi/.

	FOOTNOTES

^* Corresponding author. Mailing address: CSIRO Molecular Science, Sydney Laboratory, PO Box 184, North Ryde, NSW 1670, Australia.Phone: 61-2-9490 5162. Fax: 61-2-9490 5005. E-mail: ruth.hall{at}molsci.csiro.au.

Present address: Freehills Carter Smith Beadle, MLC Centre, Sydney, NSW 2000,Australia.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Akiba, T., K. Koyama, and Y. Ishiki. 1960. On the mechanism of the development of multiple-drug-resistant clones of Shigella. Jpn. J. Microbiol 4:219-227.
2.	Bhagwat, A. S., B. Johnson, K. Weule, and R. J. Roberts. 1990. Primary sequence of the EcoRII endonuclease and properties of its fusions with $beta$ -galactosidase. J. Biol. Chem. 265:767-773[Abstract/Free Full Text].
3.	Birnboim, H. C., and J. Doly. 1979. A rapid alkaline extraction procedure for screening recombinant plasmid DNA. Nucleic Acids Res 7:1513-1523[Abstract/Free Full Text].
4.	Boyd, D. A., G. A. Peters, L.-K. Ng, and M. R. Mulvey. 2000. Partial characterization of a genomic island associated with the multidrug resistance region of Salmonella enterica Typhymurium DT104. FEMS Microbiol. Lett 189:285-291[CrossRef][Medline].
5.	Briggs, C. E., and P. M. Fratamico. 1999. Molecular characterization of an antibiotic resistance gene cluster of Salmonella typhimurium DT104. Antimicrob. Agents Chemother. 43:846-849[Abstract/Free Full Text].
6.	Brown, A. M. C., G. M. Coupland, and N. S. Willetts. 1984. Characterization of IS46, an insertion sequence found in two IncN plasmids. J. Bacteriol. 159:472-481[Abstract/Free Full Text].
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