Involvement of H-NS in Transpositional Recombination Mediated by IS1

doi:10.1128/JB.183.8.2476-2484.2001

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Journal of Bacteriology, April 2001, p. 2476-2484, Vol. 183, No. 8
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.8.2476-2484.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Involvement of H-NS in Transpositional Recombination Mediated by IS1

Yasuyuki Shiga,¹ Yasuhiko Sekine,¹ Yasunobu Kano,² and Eiichi Ohtsubo¹^,^*

Institute of Molecular and Cellular Biosciences, The University of Tokyo, Bunkyo-ku, Tokyo 113-0032,¹ and Department of Molecular Genetics, Institute of Molecular and Cellular Biology for Pharmaceutical Sciences, Kyoto Pharmaceutical University, Yamashina-ku, Kyoto 607-8412,² Japan

Received 27 November 2000/Accepted 30 January 2001

	ABSTRACT

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IS1, the smallest active transposable element in bacteria, encodes a transposase that promotes inter- and intramolecular transposition.Host-encoded factors, e.g., histone-like proteins HU and integrationhost factor (IHF), are involved in the transposition reactionsof some bacterial transposable elements. Host factors involvedin the IS1 transposition reaction, however, are not known. Weshow that a plasmid with an IS1 derivative that efficiently producestransposase did not generate miniplasmids, the products of intramoleculartransposition, in mutants deficient in a nucleoid-associated DNA-bindingprotein, H-NS, but did generate them in mutants deficient in histone-likeproteins HU, IHF, Fis, and StpA. Nor did IS1 transpose intermolecularlyto the target plasmid in the H-NS-deficient mutant. The hns mutationdid not affect transcription from the indigenous promoter of IS1for the expression of the transposase gene. These findings showthat transpositional recombination mediated by IS1 requires H-NSbut does not require the HU, IHF, Fis, or StpA protein in vivo.Gel retardation assays of restriction fragments of IS1-carryingplasmid DNA showed that no sites were bound preferentially byH-NS within the IS1 sequence. The central domain of H-NS, whichis involved in dimerization and/or oligomerization of the H-NSprotein, was important for the intramolecular transposition ofIS1, but the N- and C-terminal domains, which are involved inthe repression of certain genes and DNA binding, respectively,were not. The SOS response induced by the IS1 transposase wasabsent in the H-NS-deficient mutant strain but was present inthe wild-type strain. We discuss the possibility that H-NS promotesthe formation of an active IS1 DNA-transposase complex in whichthe IS1 ends are cleaved to initiate transpositional recombinationthrough interaction with IS1transposase.

	INTRODUCTION

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IS1 is an insertion element present in chromosomes and plasmids of enteric bacteria (for a review, see reference 38). IS1(768 bp long) carries imperfect terminal inverted repeats (IRLand IRR) that are about 30 bp long (17, 40). IS1 mediatesthe formation of cointegrates between the IS1-carrying plasmidand a target plasmid in which two copies of IS1 are duplicatedat the two junctions in direct orientation (10, 39). Thiselement encodes two open reading frames, insA and B'-insB (16,32, 33). Transcription occurs from a promoter present in theleft-terminal region (IRL) preceding insA (31). A translationalframeshift occurs in the $-$ 1 direction at the AAAAAAC (A₆C) sequencein the overlapping region between the two open reading frames,producing the InsA-B'-InsB transframe protein, IS1 transposase(7, 49). Unless frameshifting occurs, IS1 produces InsA proteinfrom insA which can bind to the IRs (51, 74) and inhibitstransposition (30, 75). An IS1 mutant (IS1-31) with a singleadenine insertion at the frameshifting site efficiently producestransposase and therefore can frequently transpose and mediatecointegration (49). The plasmid with this IS1 mutant generatesminiplasmids, the deletion products generated by intramoleculartransposition (50, 51), as well as IS1 circles consistingof the entire IS1 sequence and a sequence 6 to 9 bp long whichappears as a spacer between the IRL and IRR of IS1 (45).

The transposition and cointegration mediated by IS1 are believed to be initiated by the step in which each strand of the donormolecule is cut at the 3' end of IS1, yielding a pair of 3'-OHtermini which are transferred to the target molecule. IS1 transposaseinduction of the SOS response is dependent on the IS1 ends, indicatingthat SOS induction is caused by transposase-mediated DNA cleavagesat the IS1 ends (26). IS1 circles are transposed to target plasmidsat a very high frequency owing to the presence of transposase,and the SOS response is induced in cells containing IS1 circles(53). These IS1 circles appear to act as intermediates leadingto simple insertion into the target DNA via the cleavage of thecircles, thereby inducing the SOSresponse.

The transposition activity of transposable elements is mediated by various host factors. Histone-like proteins (or DNA chaperones),such as HU and integration host factor (IHF), function in thetransposition reaction of some bacterial transposable elementsin vivo, in vitro, or both (for reviews, see references 25 and28). Of these histone-like proteins, IHF binds to the ends ofIS1 and to sites within the major hot-spot region for the insertionof IS1 in the target plasmid pBR322 (11). Host factors requiredfor IS1 transposition, however, have yet to be identified. Wepresent findings which show that a nucleoid-associated protein,H-NS, is required for transposition of IS1 but that the otherhistone-like proteins, HU, IHF, Fis, and StpA, are not. H-NS appearsto be important for transposase-induced cleavages at the IS1 ends.Its role in the transpositional recombination mediated by IS1is discussed based on the results of the analysis of the functionaldomains of H-NS.

	MATERIALS AND METHODS

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Escherichia coli K-12 strains and plasmids. The strains used are listed in Table 1. Plasmids used were pSEK117, pSEK131 (48), pSEK1831 (46), pKY6 (72), pSEK80(47), pYS6, pYS7, pYS10T, pYS30, pSEK131 $Delta$ HS (see below), pMC1403(2), pCM101 (30), and pSTV28 (Takara). pSEK131 and pYS10Thave the pUC-type replication origin. pSEK80 has the R100-typereplication origin. pSTV28 and its derivatives (pYS6 and pYS7)have the p15A-type replication origin.

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TABLE 1. E. coli K-12 strains used

Small-scale preparation of plasmid DNA was performed as described previously (14). The alkaline lysis method (43) wasused to prepare the plasmid DNA for cloning and nucleotidesequencing.

Media. L broth and L-rich broth (73) were used. The L-agar plates contained 1.5% (wt/vol) agar (Eiken) in L broth. Antibioticswere added to the L-agar plates when necessary, at 100 µg of ampicillin(Wako)/ml, 30 or 150 µg of chloramphenicol (Sigma)/ml, 30 µg ofkanamycin (Sigma)/ml, or 20 µg of spectinomycin (Sigma)/ml.

Enzymes and H-NS protein. Restriction endonucleases (BamHI, EcoRI, MluI, PstI, PvuII, and SalI from Takara and BsrGI, BspHI, BstEII, HindIII, NsiI,SapI, and XmnI from New England Biolabs), bacterial alkaline phosphatase,and T4 DNA ligase (Takara) were used in the buffers recommendedby the suppliers. H-NS protein purified by the method of Tanakaet al. (61) was provided by T. Mizuno (NagoyaUniversity).

Oligonucleotides. The oligonucleotide primers used are listed in Table 2. These primers were synthesized chemically in an Oligo1000M DNA synthesizer(Beckman).

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TABLE 2. Primers used

PCR. PCR was performed as described previously (45). For the analysis of the generation of miniplasmids, the total plasmid DNAwas prepared from each E. coli strain harboring pSEK131 as describedpreviously (14), and PCR was performed with the total plasmidDNA template (200 ng) and a pair of primers, p5 and p6 (50 pmoleach; Table 2), in 50 µl of Cetus buffer with 2.5 U of Ex TaqDNA polymerase (Takara) under the following thermal cycling conditions:94°C for 2 min followed by 25 cycles of 94°C for 1 min, 65°C for1 min, and 72°C for 3 min. PCR products were electrophoresed ina 1% agarosegel.

Plasmid construction. pYS6 carrying the hns gene was constructed by replacing the HindIII-BamHI segment in pSTV28 with the HindIII-BamHI fragmentbearing the hns gene from plasmid pKY6. pYS7 carrying a mutatedhns gene was constructed by replacing the BsrGI-BamHI segmentof the hns gene in plasmid pYS6 with the BsrGI-BamHI fragmentmutated by PCR using primers p7 and p8 (Table 2).

Two plasmids, pNS17 carrying mini-IS1 and pKEN200T carrying the IS1 transposase gene, were constructed first to obtain pYS10T.pNS17 was constructed by replacing the PstI-BstEII fragment fromIS1 in pSEK17, a pUC18 derivative (48), with the NsiI-BstEIIfragment bearing the chloramphenicol resistance (Cm^r) gene, which was amplified by PCR with pHSG398, a pUC-based Cm^r plasmid (59), as the template and with primers p1 and p2 (Table2). pKEN200T was constructed by replacing the SalI-BspHI regionin the polylinker sequence of pKEN100 (a p15A-based kanamycinresistance [Km^r] plasmid with the araC gene and promoter-operator region of thearaBAD operon of Salmonella enterica serovar Typhimurium [47])with the SalI-BspHI fragment bearing the transposase gene obtainedby PCR with pSEK1451 (a pUC119 derivative carrying an IS1 mutant[IS1-37] with a guanine insertion in the A₆C sequence and encodinga mutant transposase which promotes transposition as efficientlyas the wild-type transposase [48]) as the template and withprimers p3 and p4 (Table 2). Lastly, the HindIII fragment bearingboth the transposase gene placed under the arabinose promoterand the araC gene of pKEN200T was inserted in the HindIII siteof pNS17, yieldingpYS10T.

pYS30 was constructed by insertion of the HindIII fragment bearing the IS1 transposase gene and the araC gene of pKEN200Tinto the HindIII site of pHSG398. pSEK131 $Delta$ HS was constructed byligation of the pSEK131 DNA digested with HindIII and SapI.

Nucleotide sequencing. Nucleotide sequences were determined by the dideoxynucleotide method (34, 44) as described previously (47).

Transposition assay. Plasmid pYS10T was introduced by transformation into strains CSH26 and CU211, both already harboring pSEK80. The transformantswere grown for 16 h at 37°C in L-rich broth containing 0.2% (wt/vol)arabinose or 0.2% (wt/vol) glucose. Plasmid DNAs were electroporatedinto JE6638(polA) cells in a Gene Pulser (Bio-Rad). Cells wereplated on an L-agar plate containing 20 µg of spectinomycin/mlto obtain spectinomycin-resistant (Sp^r) transformants with pSEK80 and on an L-agar plate containing20 µg of spectinomycin/ml and 150 µg of chloramphenicol/ml toobtain Sp^r Cm^r transformants with pSEK80 that had an insertion of mini-IS1 ora cointegrate between pSEK80 and pYS10T. The transposition orcointegration frequency was calculated by dividing the numberof Sp^r Cm^r transformants by the number of Sp^rtransformants.

Gel retardation assay. Plasmid pSEK117 DNA (0.5 µg) digested with several restriction enzymes was incubated at room temperature for 20 min with anappropriate amount of H-NS in a reaction mixture containing 10mM Tris-HCl (pH 7.5), 1 mM EDTA, 80 mM NaCl, 10 mM $beta$ -mercaptoethanol,and 4% (vol/vol) glycerol. Samples obtained were immediately electrophoresedin a 4% polyacrylamide gel. The gel was stained with ethidiumbromide to detect protein-DNAcomplexes.

SOS induction assay. E. coli strains CSH26 sulA::lacZ and YS28 were transformed with a pYS plasmid. The transformants were grown overnight at 37°Cin L broth. The cultures were then diluted 100-fold with freshmedium without glucose and grown at 37°C to an optical densityat 600 nm of 0.4. After the addition of arabinose (final concentration,0.2% [wt/vol]), the cultures were grown for another 3 h. The specificactivities of $beta$ -galactosidase were determined as described previously(36).

Assay for promoter activity specified by IS1. CSH26 and CU211 were transformed by pMC1403 (a derivative of pBR322 with a lacZ gene lacking its promoter) or pCM101 (a pMC1403derivative having the 5' portion of IS1 [the 1-to-208 region basedon the coordinates given to IS1] cloned in frame with the promoter-lesslacZ gene). Promoter activities were measured as described previously(53).

	RESULTS

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Intramolecular IS1 transposition in mutants deficient in various histone-like proteins. IS1-31, an IS1 derivative with an insertion of 1 bp in the translational frameshifting site, efficiently mediates the productionof miniplasmids, which are deletion products generated by intramoleculartransposition (50, 51). The necessity of the histone-likeproteins HU and IHF for intramolecular transposition was examinedusing pSEK131, a pUC119 derivative with IS1-31. HU is composedof two homologous polypeptides, HU-1 and HU-2, encoded by thehupB and hupA genes, respectively (21, 23), and IHF is composedof two components, IHF $alpha$ and IHF $beta$ , encoded by the himA and hipgenes, respectively (9, 35). Miniplasmids were generatedfrom pSEK131 in a hupA hupB double mutant deficient in HU andin a himA hip double mutant deficient in IHF as well as in theisogenic wild-type strain (Fig. 1A, lanes 1 to 3). For cell growth,IHF is reported to compensate for the absence of HU, indicatingthat there is functional redundancy between IHF and HU (20).However, miniplasmids were generated in a hupB hupA himA triplemutant (Fig. 1A, lane 4), which indicates that neither HU norIHF is required for intramolecular IS1 transposition.

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FIG. 1. Generation of miniplasmids from pSEK131. (A) Ethidium bromide-stained agarose gel (0.7%) showing miniplasmids in various E. coli strains harboring pSEK131. Lane 1, YK1100 (wild type [wt]); lane 2, YK1340 (hupA hupB); lane 3, YK2920 (himA hip); lane 4, YK2741 (himA hupA hupB); lane 5, YK4122 (wt); lane 6, YK4124 (hns); lane 7, YK4137 (hns hupA hupB); lane 8, YK4205 (hns himA hip); lane 9, YK5246 (stpA); lane 10, YK5244 (stpA hns); lane 11, RZ4500 (wt); lane 12, MDW246 (fis); lane 13, CSH26 (wt); lane 14, CU211 (hns); lane 15, KT1008 (wt); lane 16, KT1004 (rpoS); lane 17, KT1008 hns (hns); lane 18, KT1004 hns (rpoS hns). Positions of pSEK131 (monomers [M] and dimers [D]) and several kinds of miniplasmids are indicated. ccc and oc indicate covalently closed circular and open circular DNA molecules, respectively. Note that miniplasmids of pSEK131 were generated in the hns wild-type strains (+) but not in the hns mutant strains ( $-$ ). (B) Ethidium bromide-stained agarose gels (1%) showing PCR-amplified fragments from miniplasmids of pSEK131. PCR was performed with (a) the total plasmid DNA prepared from the same E. coli strains as those used above (lanes 1 to 18); (b) the total plasmid DNA prepared from strains CU241 (wt; lane 1) and CU242 ( $Delta$ hns::Km^r; lane 2) and from the CU241 derivatives with an hns mutation in the N- or C-terminal domain, HM12 (hns12; lane 3), HM52 (hns52; lane 4), and HM60 (hns60; lane 5); and (c) the total plasmid DNA prepared from the H-NS-deficient strain YK4124 harboring plasmid pYS6 with the wild-type hns gene (lane 2), plasmid pYS7 with the hns gene mutated in the central domain (lane 3), or pSTV28 without the hns gene (lane 1). The DNA fragments marked with $alpha$ indicate PCR fragments from pSEK131, and small fragments marked with $beta$ indicate those from the most abundant miniplasmids of pSEK131. Molecular sizes of linear marker DNA fragments are shown on the side of the gel. Note that PCR fragments from miniplasmids were generated in the hns mutant strain ( $-$ *) with a mutation in the N- or C-terminal domain but not in the one with a mutation in the central domain.

Miniplasmids were generated in a Fis-deficient mutant as well as in the isogenic wild-type strain (Fig. 1A, lanes 11 and 12),indicating that Fis is not required for the intramolecular transpositionreaction. Miniplasmids, however, were not generated in an H-NS-deficientmutant, YK4124 (hns-2), but were generated in the wild-type strain(Fig. 1A, lanes 5 and 6). Moreover, miniplasmids were not generatedin a mutant [CU211( $Delta$ hns::Km^r)] with a mutation in another hns allele (Fig. 1A, lane 14). Furthermore,no miniplasmids were generated in a mutant deficient in both H-NSand HU or in a mutant deficient in both H-NS and IHF (Fig. 1A,lanes 7 and 8). These findings indicate that H-NS is requiredfor the IS1-mediated intramolecular transpositionreaction.

IS3 is a representative member of the IS3 family, which is distinct from the family to which IS1 belongs (38). IS3 encodesorfA and orfB and produces three proteins, OrfA, OrfB, and OrfAB.The OrfAB transframe protein is transposase, which is producedby $-$ 1 translational frameshifting between orfA and orfB (46).IS3-1, an IS3 derivative with a guanine insertion in the translationalframeshift site leading to the in-frame alignment of orfA andorfB, generates miniplasmids at a high frequency (46). Miniplasmidswere generated from plasmid pSEK1831, a pUC118 derivative withIS3-1, in mutants deficient in HU, IHF, or Fis and even in themutant deficient in H-NS (data not shown). This shows that theseproteins are not important for the IS3-mediated intramoleculartranspositionreaction.

The presence or absence of miniplasmids in the total plasmid DNA prepared from the various pSEK131-carrying strains used abovewas also examined by PCR with a pair of primers that hybridizeto the IRL and the IRR and prime DNA synthesis toward the outsideof IS1. The PCR yielded a 3.3-kb fragment representing the parentalplasmid pSEK131 and several small fragments representing miniplasmids,of which those generating a 1.3-kb fragment appeared to be themost abundant (Fig. 1B, panel a). Such small fragments were notamplified by PCR with the total plasmid DNA prepared from theH-NS-deficient mutants but were amplified by PCR with the totalplasmid DNA from the other mutants (Fig. 1B, panel a). This confirmsthe results above, showing that H-NS is required for the intramolecularIS1 transpositionreaction.

Further evidence of the involvement of H-NS in IS1-mediated intramolecular transposition. As stated above, no miniplasmids were generated in the H-NS-deficient mutant. H-NS has been shown to modulate the transcriptionof many genes (for reviews, see references 1 and 64), butthe hns mutation did not affect transcription from the indigenouspromoter of IS1 that is located in the left-terminal region andis responsible for the expression of the transposase gene (datanot shown). This shows that H-NS does not mediate expression ofthe transposase gene in IS1-31 and indicates that H-NS is directlyinvolved in the transpositionreaction.

The E. coli StpA protein is an intraspecies homologue of H-NS and substitutes for H-NS in some biological reactions (52,69, 76). Miniplasmids were generated in an stpA mutant (Fig.1A and B, lanes 9) but not in an stpA hns double mutant (Fig.1A and B, lanes 10). This shows that StpA is not required forintramolecular transposition but that H-NSis.

The stationary phase-specific sigma factor $sigma$ ^s encoded by the rpoS gene accumulates even in the logarithmic-growth phase inH-NS-deficient mutant cells (71). This accumulation of $sigma$ ^s may be responsible for the lack of generation of miniplasmidsfrom pSEK131 in the H-NS-deficient mutant. However, miniplasmidswere not generated from pSEK131 in an rpoS hns double mutant orin an hns single mutant (Fig. 1A and B, lanes 17 and 18), butthey were generated in an rpoS single mutant (Fig. 1A and B, lanes16). This is evidence that the unusual accumulation of $sigma$ ^s is not responsible for the failure of intramolecular transpositionin the H-NS-deficientmutant.

It is known that hns mutants tend to accumulate mutations (29). To disprove the possibility that a second-site mutation(s)which may have occurred in the hns mutant is responsible for thefailure of intramolecular IS1 transposition, plasmid pYS6, whichcarries the wild-type hns gene, was introduced into the H-NS-deficientmutant and the generation of miniplasmids from pSEK131 was examinedby PCR. Miniplasmids were generated in the H-NS-deficient mutantharboring both pSEK131 and pYS6 (Fig. 1B, panel c, lane 2) butnot in the mutant harboring both pSEK131 and the vector plasmidpSTV28 with no hns gene (Fig. 1B, panel c, lane 1). This showsthat the hns gene carried by pYS6 complemented the mutated hnsgene, resulting in the generation of miniplasmids, and that anypossible second-site mutations are not responsible for the failureof intramolecular IS1 transposition in the H-NS-deficientmutant.

H-NS requirement in IS1-mediated intermolecular transposition. The necessity for H-NS in IS1-mediated intermolecular transposition was examined using plasmid pYS10T with mini-IS1, in whichthe transposase-coding region was replaced with the Cm^r gene as the donor. In this plasmid, the transposase gene wasplaced in the region downstream of the arabinose-inducible promoter(Fig. 2A). It was introduced into the wild-type strain (CSH26)or the H-NS-deficient mutant (CU211) that harbored the targetplasmid pSEK80 with the spectinomycin resistance (Sp^r) gene. The plasmid DNA prepared from cells bearing both the donorand target plasmids was electroporated into cells of strain JE6638(polA1), in which the donor plasmid pYS10T, a pUC18 derivative,cannot replicate and the target plasmid pSEK80, a derivative ofplasmid R100, can. Cm^r Sp^r transformants were obtained at a frequency of 1.4 × 10⁴ per target plasmid molecule upon electroporation of the plasmidDNA prepared from the wild-type strain grown in the presence ofarabinose (Table 3). Gel electrophoresis and cleavage by relevantrestriction enzymes showed that the plasmids from 77% of the Cm^r Sp^r transformants were target plasmids, with an insertion of mini-IS1,and that those from the rest of the transformants were cointegrates,with two copies of mini-IS1 at the junctions between the donorand target plasmid sequences. No Cm^r Sp^r transformants were obtained upon electroporation of the plasmidDNA from the H-NS-deficient strain, even when grown in the presenceof arabinose. (The frequency [<1.4 × 10⁶ per target plasmid molecule] was at least 100-fold lower thanthe frequency for the wild-type strain [Table 3].) This showsthat H-NS is required not only for intramolecular transpositionbut for the intermolecular transposition of IS1 as well.

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FIG. 2. Structures of pYS10T (A) and pYS30 (B). pYS10T carries mini-IS1, which has an IRL and an IRR (closed triangles) and the chloramphenicol resistance gene (Cm^r) in place of the transposase gene. The transposase gene was placed in the region downstream of the promoter of the araBAD operon (Para; open triangle), whose expression is controlled by the araC gene product. Ap^r, ampicillin resistance gene. pYS30 carries the Para-driven transposase gene. The origin of replication of the pUC plasmid is shown by a closed circle.

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TABLE 3. Transposition frequency of mini-IS1 on plasmid pYS10T

Identification of sites preferentially bound by H-NS in the IS1-carrying plasmid. The site(s) bound by H-NS in pSEK117 was examined using a gel retardation assay. pSEK117, the parent of pSEK131, carries wild-typeIS1 instead of the mutant IS1-31 in pSEK131. pSEK117 was usedin this assay because it does not generate miniplasmids, whichcomplicate the assay. The gel retardation assay using the pSEK117plasmid DNA digested with a set of restriction enzymes showedthat H-NS preferentially bound to three fragments (those labeled1, 3, and 5 in Fig. 3) but did not bind to any others, includingthe two fragments with the IS1 sequence (those labeled 4 and 6in Fig. 3), indicating that IS1 has no H-NS-binding site withinits sequence. (Note that an excess amount of H-NS protein causedretardation of all the DNA fragment bands due to the nonspecificDNA-binding ability of H-NS [data not shown].) The gel retardationassay using the pSEK117 plasmid DNA digested with another setof restriction enzymes showed that four fragments (those labeled1', 3', 4', and 6' in Fig. 3) were preferentially bound by H-NS.Of these retarded fragments, one (4') has the IRR region of theIS1 sequence as well as the sequence neighboring it. This meansthat at least one H-NS-binding site is present in the sequenceneighboring the IRR of IS1, because the IS1 sequence has no H-NS-bindingsite.

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FIG. 3. (A) Ethidium bromide-stained acrylamide gels (4%) showing the results of the gel retardation assay with H-NS and restriction fragments derived from pSEK117. (a) Restriction fragments digested with BspHI, EcoRI, PstI, SalI, and XmnI and (b) those digested with BspHI, MluI, PvuII, and XmnI. Fragments were incubated with H-NS protein at the indicated concentrations (pmol/µl). Numbers refer to fragments whose positions are shown in panel B. (B) Restriction maps of pSEK117 and pTP4 (a derivative of pUC119 with a cloned fragment [18]). The restriction fragments from pSEK117 are numbered in order of size. Restriction sites: B, BspHI; E, EcoRI; H, HindIII; M, MluI; Ps, PstI; Pu, PvuII; S, SalI; Sa, SapI; X, XmnI. The bla gene is shown with a thick arrow. ori is the replication origin of pUC119. The region in pTP4 which differs from that in pSEK117 is shown by broken lines. An HaeIII restriction map of pTP4 is depicted. The restriction fragments of pSEK117 and pTP4 preferentially bound by H-NS are indicated by hatched or dark boxes. Restriction fragments indicated by the dark boxes required a greater amount of H-NS protein for retardation than those indicated by the hatched boxes. pSEK131 $Delta$ HS has a deletion of the HindIII-SapI fragment (dotted lines) which borders the IRR sequence in pSEK117. (C) An ethidium bromide-stained agarose gel (0.7%) showing the production of miniplasmids from pSEK131 (lane 1) and pSEK131 $Delta$ HS (lane 2) in YK4122. For further details, see the legend for Fig. 1.

Plasmid pSEK117 is a derivative of pUC119. Jordi et al. (18) performed a gel retardation assay with plasmid pTP4, a pUC119derivative with a cloned fragment, and showed that some restrictionfragments were bound by H-NS. Retarded fragments with the pUC119sequence could be identified, as shown in Fig. 3B. This, togetherwith the above results, allowed for the identification of theDNA segments with an H-NS-binding site(s), one of which is locatedin the region neighboring the IRR of IS1 (Fig. 3B).

To see whether the H-NS-binding site(s) in the sequence neighboring the IRR of IS1 is important for the intramolecular IS1transposition, plasmid pSEK131 $Delta$ HS, a pSEK131 derivative with adeletion of the segment with the binding site(s) (Fig. 3B), wasexamined for the generation of miniplasmids. pSEK131 $Delta$ HS was ableto generate miniplasmids (Fig. 3C), showing that the H-NS-bindingsite(s) in the region neighboring IS1 is not important for theintramolecular transpositionreaction.

Analysis of the functional domain of H-NS that affects IS1 transposition. The previous mutational analysis of hns indicated that H-NS consists of three distinct domains, the N-terminal, central, andC-terminal regions, which are responsible for transcriptionalrepression, dimerization and/or oligomerization, and DNA-binding,respectively (62, 63). To determine which domain of H-NS isimportant for IS1 transposition, the generation of miniplasmidsfrom pSEK131 in three mutants with a mutation in the hns geneon the chromosome was examined by PCR. Mutant strain HM12 hasa missense mutation in the proximal end region of hns which producesan H-NS protein with a mutated N-terminal domain, causing lossof the ability to repress the transcription of proV but retainingthe DNA-binding activity (63). Miniplasmids were generated inHM12 harboring pSEK131 as well as in the isogenic wild-type strainCU241 harboring pSEK131 (Fig. 1B, panel b, lanes 1 and 3), showingthat an amino acid substitution in the N-terminal domain of H-NSdoes not affect IS1 transposition. This may support the idea thatthe N-terminal domain of H-NS is not important for IS1 transposition.Mutant strains HM52 and HM60 have missense and amber mutations,respectively, in the distal end region of hns which produce anH-NS protein with a mutated or truncated C-terminal domain, causingloss of the DNA-binding activity (63). Miniplasmids were generatedin each mutant strain harboring pSEK131 (Fig. 1B, panel b, lanes4 and 5), showing that neither an amino acid substitution nortruncation in the C-terminal domain of H-NS affects IS1 transposition.This indicates that the C-terminal domain is not important forIS1transposition.

The mutants with a mutation in the N- or C-terminal domain of H-NS which were used in the above experiments have been shownnot to impair dimer formation of H-NS (63). Therefore, to determinewhether the central domain of H-NS responsible for dimer formationis important for IS1 transposition, the generation of miniplasmidsfrom pSEK131 in the H-NS-deficient mutant YK4124 harboring plasmidpYS7 with a mutated hns gene in the central domain was examinedby PCR. The mutated hns gene has a missense mutation (the 30thcodon, CUG for leucine, to CCG for proline) causing loss of thedimer-forming activity of the H-NS protein as well as the repressionof transcription from the proV and bgl promoters (62). Miniplasmidswere not generated in YK4124 harboring both pSEK131 and pYS7 (Fig.1B, panel c, lane 3) or in YK4124 harboring both pSEK131 and thevector plasmid pSTV28 with no hns gene (Fig. 1B, panel c, lane1), but they were generated in YK4124 harboring both pSEK131 andpYS6 with the hns gene (Fig. 1B, panel c, lane 2). This showsthat the central domain of H-NS is important for IS1transposition.

Lack of induction of the SOS response by IS1 transposase in the H-NS-deficient mutant. IS1 transposase induces the SOS response by way of transposase-induced cleavages at the IS1 ends (26). The SOS responsein cells harboring pYS plasmids with mini-IS1 was therefore examinedusing an E. coli strain with an SOS gene, sulA, fused with thelacZ gene. $beta$ -Galactosidase activity in the H-NS-deficient andwild-type strains that harbored no plasmid and were grown in thepresence of mitomycin C, a drug known to induce the SOS response,was significantly increased compared to that in the strains grownin the absence of mitomycin C (Table 4). $beta$ -Galactosidase activityin the H-NS-deficient strain harboring pYS10T with the arabinose-inducibletransposase gene (Fig. 2A) was not increased in the presence ofarabinose, whereas it was increased in the wild-type strain harboringpYS10T (Table 4). These findings suggest that the ends of IS1are not cleaved in the H-NS-deficient strain and therefore thereis no induction of the SOS response. $beta$ -Galactosidase activitywas not increased in the presence of arabinose in the H-NS-deficientstrain harboring pYS30 (Table 4), which has the arabinose-inducibletransposase gene but lacks IR sequences in mini-IS1 (Fig. 2B),as was also the case for the H-NS-deficient or wild-type strainharboring no plasmid (Table 4), supporting the argument describedabove. $beta$ -Galactosidase activity, however, was increased to someextent in the presence of arabinose in the wild-type strain harboringpYS30. This increase may be the result of transposase action onchromosomal copies of IS1.

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TABLE 4. SOS responses induced by transposase and mini-IS1

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We showed that in vivo the intramolecular transposition mediated by IS1 does not require HU, IHF, or Fis and that the intramoleculartransposition mediated by IS3, which is distinct from IS1, doesnot require these host proteins. Histone-like proteins (or DNAchaperones) are involved in the transposition of certain transposonsas well as in many site-specific recombination systems. The HUprotein is required in an early step in phage Mu transpositionin vitro (4, 5, 56) and in vivo (15, 19). HU is thoughtto promote the formation of a tight DNA bend in the end regionwhich facilitates the communication of Mu A monomers during complexassembly by binding specifically to sites within the region betweentwo Mu A-binding sites in the Mu left end (27). IHF stimulatesthe Mu DNA strand transfer reaction in vitro by binding at thetranspositional enhancer (57, 58). IHF modulates Tn10 transpositionin vivo and in vitro; IHF stimulates Tn10 excision and forcestransposon end-target DNA interactions into a constrained pathwaythat yields only unknotted intratransposon inversion circles (3,54). IHF binds to the ends of $gamma$ $delta$ , a Tn3 family element, cooperativelywith transposase and stimulates transpositional immunity of $gamma$ $delta$ (67, 68). Fis is required for various site-specific recombinationsystems, and HU and IHF act in some of these systems as well (fora review, see reference 12). These proteins are thought to promotethe formation of the nucleoprotein structures which facilitatesynapsis of the DNA strands required for site-specific recombination.IS1 and IS3, which were shown here to require none of the histone-likeproteins (HU, IHF, and Fis) for their transposition in vivo, arethought to form a nucleoprotein complex that is different fromthe complexes of the other elementsdiscussed.

We demonstrated that the intra- and intermolecular transposition mediated by IS1 requires H-NS, a protein abundant in E. coliwhich has a molecular mass of approximately 15.6 kDa (55). H-NSbinds to DNA in a relatively nonspecific fashion but preferentiallybinds to curved double-stranded DNA (41, 70, 77). H-NS constrainsnegative supercoils, thereby affecting DNA topology, and modulatesthe transcription of many genes (for reviews, see references 1and 64). Mutations in the hns gene caused an increase in transcriptionof the Mu transposase gene, leading to an increase in the Mu transpositionrate, and the depletion of H-NS probably caused destabilizationof the Mu repressor-DNA complex which keeps the transposase genetranscriptionally inactive (8). To our knowledge, no othercases in which H-NS positively regulates the DNA recombinationreaction have been reported. The rate of spontaneous chromosomaldeletions and an inversion of a DNA element with the fimA promoterare stimulated in hns mutants (24, 29), but in these casesH-NS is supposed to negatively regulate the DNA recombinationreaction. Note that the positive role of H-NS in the transpositionalrecombination mediated by IS1 is the only example of a histone-likeprotein that is essential for the transposition of the transposableelement in vivo, except for HU, which is involved in Mu transposition.The role of H-NS in IS1 transposition may therefore shed lighton a novel function of H-NS.

We showed that the N-terminal and C-terminal domains of H-NS, which are responsible for the repression of the proV promoterand DNA binding, respectively, are dispensable for intramolecularIS1 transposition. Dispensability of the DNA-binding domain mayalso be supported by the fact that the IS1 sequence is not preferentiallybound by H-NS. We then showed that the central domain of H-NS,which is responsible for the dimerization of the H-NS protein(62), is indispensable for intramolecular IS1 transposition.These results lead us to conclude that the ability of H-NS toform a dimer is important for IS1 transposition. The transpositionreaction of IS1 should require the formation of an IS1 DNA-transposasecomplex in which both IRs are held closely together by transposasefor subsequent reactions such as end cleavage and strand transfer.We postulate that H-NS interacts with IS1 transposase to forman active DNA-transposase complex for IS1 transposition. In thisconnection, it is noteworthy that the fimA promoter inversionand the bgl gene silencing for which the C-terminal DNA-bindingdomain of H-NS is dispensable are thought to be regulated throughprotein-protein interactions with other molecules at the fimAinvertible element and the bgl promoter (6, 63). AlthoughH-NS regulates DNA recombination positively in the IS1 systembut negatively in the fimA system, H-NS may be involved in thesesystems by a common protein-protein interactionmechanism.

We showed here that the SOS response was not induced in the H-NS-deficient strain, which is strong evidence that H-NS hasan important role in DNA cleavage at the IRs owing to the actionof transposase. An IS1 circle with a spacer sequence of 6 to 9bp has been shown to transpose to target plasmids at a very highfrequency because of transposase (53). This transposition wasaccompanied by removal of the spacer sequence in the IS1 circleand by duplication of a sequence at the target site. IS1 circlesappear to act as intermediates leading to simple insertion intothe target DNA via IS1 circle cleavage, which efficiently inducesthe SOS response. Interestingly, IS1 circle transposition didnot require H-NS (53), although IS1 transposition did. We assumethat when the IS1 circle, in which both IRs are intrinsicallyclosely located, serves as the donor, an active DNA-transposasecomplex is formed even in the absence of H-NS but that when IS1serves as the donor, H-NS is essential for the formation of theactive complex in which DNA cleavage occurs at theIRs.

We found that as in the wild-type strain, IS1 circles transpose preferentially to AT-rich regions in the H-NS-deficient strains.In the H-NS-deficient strain, however, IS1 circles transpose evento non-AT-rich regions (53). These observations led us to assumethat H-NS participates in the step involving the target DNA molecule.The interaction of H-NS with the IS1 transposase protein may alsobe important for target capture and/or formation of a nucleoproteincomplex consisting of IR DNA, target DNA, andtransposase.

	ACKNOWLEDGMENTS

This research was supported by a grant-in-aid for scientific research from the Ministry of Education, Science, Sports, andCulture ofJapan.

We thank K. Tanaka, T. Horiuchi, W. Reznikoff, and C. Ueguchi for kindly providing us with the E. coli strains used in thisstudy. We also thank T. Mizuno for the gift of purified H-NSprotein.

	FOOTNOTES

^* Corresponding author. Mailing address: Institute of Molecular and Cellular Biosciences, The University of Tokyo, Yayoi 1-1-1,Bunkyo-ku, Tokyo 113-0032, Japan. Phone: 81-3-5841-7852. Fax:81-3-5841-8484. E-mail: eohtsubo{at}ims.u-tokyo.ac.jp.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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