Bacterial SOS Checkpoint Protein SulA Inhibits Polymerization of Purified FtsZ Cell Division Protein

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Journal of Bacteriology, August 1998, p. 3946-3953, Vol. 180, No. 15
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Bacterial SOS Checkpoint Protein SulA Inhibits Polymerization of Purified FtsZ Cell Division Protein

Dorina Trusca,¹ Solomon Scott,² Chris Thompson,¹ and David Bramhill¹^,^*

Department of Enzymology¹ and Department of Immunology,² Merck Research Laboratories, Rahway, New Jersey 07065-0900

Received 6 February 1998/Accepted 29 May 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Cell division of Escherichia coli is inhibited when the SulA protein is induced in response to DNA damage as part of the SOScheckpoint control system. The SulA protein interacts with thetubulin-like FtsZ division protein. We investigated the effectsof purified SulA upon FtsZ. SulA protein inhibits the polymerizationand the GTPase activity of FtsZ, while point mutant SulA proteinsshow little effect on either of these FtsZ activities. SulA didnot inhibit the polymerization of purified FtsZ2 mutant protein,which was originally isolated as insensitive to SulA. These studiesdefine polymerization assays for FtsZ which respond to an authenticcellular regulator. The observations presented here support thenotion that polymerization of FtsZ is central to its cellularrole and that direct, reversible inhibition of FtsZ polymerizationby SulA may account for division inhibition.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The bacterial SOS response to DNA damage represents one of the first examples of what has become known as checkpoint regulation(for a recent review, see reference 40). The sulA gene was firstidentified as a factor required for SOS-mediated division inhibition(16) and was found independently to be a suppressor of lon mutants(15). Transcription of the sulA gene is induced as part of theSOS response in Escherichia coli cells (21, 28). Elevatedlevels of the SulA division inhibitor are sufficient to causedivision inhibition (22).

The target of SulA is thought to be the FtsZ protein (3, 19, 27). FtsZ plays a central role in bacterial division,forming a structural element at the division site (for reviews,see references 6, 11, 26, and 36). Although the aminoacid sequence of FtsZ includes only a short segment with a highdegree of sequence homology to tubulins, there is a remarkablesimilarity between the structures of these two proteins (25,31). Purified FtsZ has GTPase activity (9, 29, 34) andcan polymerize to form protofilaments which closely resemble theprotofilaments in microtubules (12). FtsZ normally becomes localizedto the division site as one of the earliest detected events incell division (5). However, when SulA is induced, FtsZ failsto localize to the division site (3).

Several lines of evidence point to a direct interaction between SulA and FtsZ. FtsZ stabilizes SulA in vivo (23), and purifiedSulA binds to FtsZ in vitro (19). Also, wild-type SulA interactswith FtsZ in the yeast two-hybrid system, while mutant SulA proteinsdo not. Most SulA-resistant FtsZ point mutations abolish interactionwith SulA in the two-hybrid system (20).

Diverse conditions have been found to support polymerization of FtsZ in vitro; however, most of these studies were performedeither at or below neutral pH (7, 12, 30) or in the presenceof calcium (42) at levels significantly higher than that normallyfound in the cell (8, 13).

We devised conditions that allowed quantitation of FtsZ polymerization in the presence of DEAE-dextran and used these assaysto test the effect of SulA on polymerization. The results presentedin this report indicate that SulA binding to FtsZ directly inhibitsthe polymerization of FtsZ.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Reagents. Chemicals and reagents were obtained from Sigma unless otherwise stated. DEAE-dextran (Sigma 9885; average molecular weightof 500,000). GTP and deoxynucleoside triphosphates for PCR reactionswere purchased from Boehringer, [ $alpha$ -³²P]GTP was obtained from Dupont-NEN, Tris buffer (pH 7.4) was fromBioWhittaker, IPTG (isopropyl- $beta$ -D-thiogalactopyranoside) was fromNational Laboratory Source, Syto-17 came from Molecular Probes,and Permount was obtained from Fisher. Restriction enzymes werepurchased from New England Biolabs; the DNA polymerases for PCRand the QuickChange site-directed mutagenesis kit were from Stratagene.

Strains and plasmids. E. coli strains BL21(DE3) [F ompT hsdS_B (r_B m_B) gal dcm (DE3)] and HMS174(DE3) [F recA1 hsdR(r_K12 m_K12⁺) Rif^r (DE3)] (39) were obtained from Novagen and were used as expressionhosts for genes cloned under T7 promoter control (the lambda prophagecarries the T7 RNA polymerase expressed from the lacUV5 promoter).The recombination-deficient strain DH5alpha (recA1) (18), whichlacks any T7 RNA polymerase, was used as the initial cloning hostfor all subcloning and mutagenesis studies.

Plasmids were obtained from Novagen. The pBR322-derived pET11a (10) confers ampicillin resistance and allows cloning ofgenes downstream of the T7 promoter overlapped by the lac operatorto provide regulation by IPTG, while the pACYC184-derived pLysSplasmid (38) confers chloramphenicol resistance and providesa low level of the T7 lysozyme, which inhibits the T7 RNA polymerasestoichiometrically, thereby reducing the expression of genes clonedin pET11 vectors prior to induction with IPTG (used for PrtA-SulAexpression). SulA fusions were constructed in a derivative ofpET11a into which a portion of the Staphylococcus protein A genewas inserted, allowing in-frame fusion to the C terminus of proteinA for any protein initiating with a methionine codon overlappingan NdeI site (19a). Mutant derivatives of PrtA-SulA and FtsZwere constructed with the QuickChange site-directed mutagenesiskit as described by the manufacturer, starting with the appropriatepET11 clone. Primer pairs used to introduce the mutations were5'-GGTCAGCAATCGCACTGGCAACTCTGG-3' and 5'-CCAGAGTTGCCAGTGCGATTGCTGACC-3'for SulA62H and 5'-GGTCAGCAATCGAGCTGGCAACTCTGG-3' and 5'-CCAGAGTTGCCAGCTCGATTGCTGACC-3'for SulA62S. To change FtsZwt to FtsZ2, the primers 5'-CGTGGACTTTGCAGGCGTACGCACCGTAATG-3'and 5'-CATTACGGTGCGTACGCCTGCAAAGTCCACG-3' were used. Each cloneand mutant derivative were confirmed by using fluorescent dideoxyterminator sequencing on an ABI377 DNA sequencing machine.

Purification of protein A-SulA fusion proteins. Strain HMS174(DE3)(pLysS) was transformed with a pET11 derivative encoding the fusion to protein A of wild-type SulA or mutantSulA. Cells were grown in minimal medium (33) to an opticaldensity at 600 nm (OD₆₀₀) of 0.5, induced by the addition of IPTGto a final concentration of 1 mM, and grown at 37°C for 2.5 h(for PrtA-SulAwt and PrtA-SulA62H) or at 22°C overnight (for PrtA-SulA62S).Cells were harvested and resuspended in buffer A (10 mM Tris-Cl,pH 8; 10% glycerol; 1 mM dithiothreitol; 1 mM EDTA, 150 mM KCl)to which lysozyme was added to a final concentration of 200 µg/ml.Cells were frozen in liquid nitrogen, thawed, and centrifugedat 40,000 rpm in a 45 Ti rotor for 1 h at 4°C to remove debris.To this extract solid ammonium sulfate was added (0.25 g/ml ofextract) to precipitate the PrtA-SulA fusion. Ammonium sulfatepellets were redissolved in buffer B (20 mM Tris-Cl, pH 7.4; 1mM dithiothreitol; 20% glycerol), conductivity was adjusted tobe equivalent to 125 mM NaCl, and then the samples were loadedonto a Q Sepharose fast-flow column (Pharmacia). Protein was elutedby applying a gradient of 125 to 500 mM NaCl in buffer B. Fractionscontaining the fusion protein were pooled and loaded onto an immunoglobulinG (IgG)-Sepharose column (Pharmacia) equilibrated with TST buffer(50 mM Tris-Cl, pH 7.6; 150 mM NaCl; 0.05% Tween 20). The columnwas washed with 10 bed volumes of TST buffer then with 2 bed volumesof 5 mM ammonium acetate (pH 5.0). PrtA-containing fractions wereeluted with 0.1 M glycine-HCl (pH 3), and fractions were neutralizedimmediately following elution by the addition of a predeterminedvolume of 1 M Tris base and then verified to be at a pH of 7.4.

FtsZ polymerization assays. Wild-type and mutant FtsZ protein was spun at 22,260 × g for 20 min at 4°C in a TLA-100.2 rotor in a Beckman TL-100 ultracentrifugeimmediately prior to reaction assembly to remove any preexistingpolymers. Reactions were assembled on ice and contained 100 mMTris-Cl (pH 7.4), 1.5 mM magnesium acetate, 50 mM KCl, 1 mM GTP,and 2 µM FtsZwt or FtsZ2 in a final volume of 200 µl. Reactionswere initiated by the addition of DEAE-dextran, incubated for10 min at 37°C, and then spun at 22,260 × g for 20 min at 37°C.Pellets were resuspended in 200 µl of 100 mM Tris-Cl (pH 7.4).To both supernatant and resuspended pellets, 20 µl of 4× sodiumdodecyl sulfate (SDS) sample buffer (0.25 M Tris-Cl, pH 6.8; 8%SDS; 40% glycerol; 20% 2-mercaptoethanol) was added and then themixture was heated at 95°C, uncovered, for 10 min. Aliquots wereloaded onto 10% polyacrylamide Tris-glycine-SDS resolving gels(Bio-Rad). Gels were Coomassie blue stained, destained, scannedwith a Molecular Dynamics densitometer, and quantified by usingImageQuant software. Dilution series of known amounts of FtsZin the gels were used as internal standards.

Affinity copurification of PrtA-SulA and FtsZ. FtsZ proteins were centrifuged prior to reaction assembly as described above. Reactions were assembled exactly as for thepolymerization assays, except that DEAE-dextran was omitted. Whereindicated, FtsZ was present at 4 µM and PrtA-SulA fusions werepresent at 2 µM. After 15 min at 37°C, 200-µl reaction mixtureswere loaded onto IgG columns (0.5-ml bed volume), equilibratedin reaction buffer plus 1 mM GTP, washed in the same buffer, andeluted as described above for the PrtA-SulA fusions. Electrophoresisand densitometric analysis was done as described for the sedimentationassay (except that dilutions of PrtA-SulA standards were usedin estimating PrtA-SulA).

GTPase assay. FtsZ proteins were centrifuged prior to reaction assembly as described above for the polymerization assays. The assays (50-µlfinal volume) contained 100 mM Tris-Cl (pH 7.4), 1.5 mM magnesiumacetate, 50 mM KCl, 0.075 µCi of [ $alpha$ -³²P]GTP, and 0.1 mM GTP. Reactions were usually initiated by theaddition of 2 µM FtsZwt or FtsZ2. However, when the effects ofPrtA-SulA fusion proteins were being monitored, a 5-min preincubationof the FtsZ and PrtA-SulA fusion was carried out in the absenceof GTP, and the reactions were then initiated by addition of GTP.Incubation was carried out in a 96-well plate from which 3.5-µlaliquots were withdrawn at specific time points and transferredto a second plate containing 3.5 µl per well of a quenching mix(2 mM GDP, 0.2% SDS, 20 mM EDTA, 30% glycerol), allowing timepoint data to be obtained at 15-s intervals (typically at 0, 0.25,0.5, 0.75, 1, 1.25, 1.5, 1.75, 2, 4, 6, and 20 min). From eachquenched time point, a 1-µl sample was spotted onto PEI celluloseF thin-layer chromatography plastic sheets (EM Science); eachsheet was dried, then washed for 10 min in methanol, and thendried again and developed in 1 M formic acid and 0.5 M LiCl. Thesheets were exposed in a phosphor screen cassette and quantitatedwith a Storm 860 phosphorimager (Molecular Dynamics). The resultsare expressed as the total amount of GTP converted to GDP in a50-µl reaction.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

FtsZ polymerization. Purified FtsZ protein can be induced to form extensive polymers at a pH of 6.0 or lower, and DEAE-dextran has been used atpH 6.5 to induce FtsZ polymer formation (12). Limited polymerizationhas been observed at or above neutral pH by electron microscopy(12, 30). We tested whether DEAE-dextran will also inducepolymerization of FtsZ at pH 7.4, a more physiological pH forcells of E. coli. We used a sedimentation assay to monitor theextent of polymer formation. Figure 1A shows the effect of titratingDEAE-dextran into an FtsZ solution. At approximately equal massratio of FtsZ to DEAE-dextran there is efficient recovery of FtsZin the pellet. The level of polymers remained essentially constantfrom 5 min to at least 20 min when the reactions contained 1 mMGTP, though after longer times reduced polymerization was seencorrelating with depleted GTP levels (data not shown). The polymerizationof FtsZ dependent on DEAE-dextran is inefficient in the absenceof GTP (20 to 45% of full reaction) or magnesium (30 to 50%),but when GDP is present in place of GTP, polymerization is 30to 60% of that seen with GTP.

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FIG. 1. Titration of DEAE-dextran into FtsZ sedimentation assay. (A) SDS-polyacrylamide gel analysis of the supernatant and pelleted FtsZ protein with increasing levels of DEAE (final concentrations of 0, 3.125, 6.25, 12.5, 25, 50, 100, 200, and 400 µg/ml, respectively, in lanes 1 to 9). The gel lanes are arranged so that the corresponding supernatant and pellet at a specific level of DEAE are vertically aligned. (B) Same as in panel A, but with FtsZ2 mutant protein in place of wild type. (C) Densitometric scans of the gels in the top two panels were used to determine the fraction of FtsZ sedimented and then plotted as a function of the amount of DEAE-dextran added as described in Materials and Methods.

FtsZ2 characterization. The FtsZ2 mutant was originally isolated in a screen seeking ftsZ alleles that conferred resistance to the SulA division inhibitor(2). The mutation was introduced into the pET11-FtsZ expressionplasmid by site-directed mutagenesis. By using the pET11-FtsZ2plasmid in the expression host BL21(DE3), the FtsZ2 protein wasoverexpressed and purified for comparison with the wild-type FtsZ.Its purification was made possible by a procedure identical tothat used for the wild-type FtsZ protein (7).

Polymerization of FtsZ2 and wild type was compared at different DEAE-dextran concentrations (Fig. 1B). DEAE-dextran was essentialto induce significant polymerization of FtsZ2 under these conditions.However, FtsZ2 required significantly lower concentrations ofDEAE to induce polymerization than did wild-type FtsZ protein(Fig. 1C).

The ability of FtsZ2 to hydrolyze GTP was compared with that of wild-type FtsZ at the permissive and restrictive temperaturesfor ftsZ2 mutant growth. The GTPase activity of FtsZ2 was at least200-fold lower than that of wild-type FtsZ measured at 30°C andeven less active at 42°C (Fig. 2). The lower panel (Fig. 2B; notethe very different x and y scales compared to Fig. 2A) shows thatFtsZ2 did exhibit GTPase activity above background. The FtsZ2GTPase activity was reduced at 42°C, at which temperature ftsZ2mutants are not viable (2).

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FIG. 2. (A) GTPase of FtsZ2 compared with wild-type FtsZ at 30 and 42°C. (B) Replotted detail (note axis changes) of FtsZ2 at 30 and 42°C, extending the time to 60 min. Each FtsZ protein (Zwt or Z2) was present as 2 µM, and the assay was performed as described in Materials and Methods.

Polymer structures. The nature of the polymers formed by FtsZ and FtsZ2 under these conditions was investigated by electron microscopy of negativelystained samples (Fig. 3). The predominant form of FtsZ polymersis a tube with a diameter of about 20 nm. Sheets and miniringsof FtsZ resembling those reported previously (12) were alsoseen. The relationship between these structures is suggested bythe appearance of numerous tubules, which seem to be either partiallydisrupted or else incompletely formed. These structures seem toexhibit a helical arrangement of the protofilaments in the tubules.A plausible explanation of these observed images is that thereis a tubule formed from a pair of FtsZ protofilaments (most likelyparallel to one another, as in the sheets) that are wrapped helically,as indicated by the diagram in Fig. 3 (inset). The structuresobserved for FtsZ2 mutant protein were indistinguishable fromthose formed by wild-type FtsZ, although FtsZ2 showed somewhatfewer sheets than did wild-type FtsZ. Though less abundant, thepolymers of FtsZ formed in the absence of GTP or magnesium orwhen GDP replaced GTP resembled the various forms seen with GTP(data not shown).

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FIG. 3. Electron micrographs of FtsZ polymers induced by DEAE-dextran, each at a magnification of ×59,000. (A to D) Wild-type FtsZ, illustrating tubules (A), protofilaments aligned vertically (B), and minirings (C and D, arrowheads). (E and F) FtsZ2 showing miniring (E) and tubules (F), with inset diagram of proposed tubule structure represented as one light and one dark protofilament. Polymerization reactions were done as described in Materials and Methods with FtsZ proteins present at 5 µM. Scale bar, 100 nm.

SulA fusions and mutants. To determine whether our polymerization assay at pH 7.4 reflects the cellular conditions, we decided to investigate the effectsof SulA protein on the activity of FtsZ. Initial attempts to isolateSulA protein were hampered by its poor solubility. We found thata fusion of part of the Staphylococcus protein A (PrtA) to theamino terminus of SulA resulted in a soluble PrtA-SulA fusionthat was easily purified by IgG-affinity column chromatography.Two null mutant forms of SulA were also made as PrtA-SulA fusionsby site-directed mutagenesis of the wild-type fusion construct.These mutants had replaced the arginine residue at position 62of the wild-type SulA with either histidine (PrtA-SulA62H) orserine (PrtA-SulA62S). The function of each fusion construct wastested by two methods to confirm that the wild-type SulA domainretained its biological activity and that the mutant forms weredefective. First, the concentration of IPTG which induced expressionof lethal levels of each protein was examined. The lowest levelof IPTG tested (0.0078 mM) was sufficient to induce significantkilling of cells expressing the wild-type PrtA-SulA, while growthof cells expressing the PrtA-SulA62H or PrtA-SulA62S toleratedIPTG at up to 0.25 mM (Fig. 4).

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FIG. 4. Toxic expression of PrtA-SulA fusions. Strain HMS174(DE3) was transformed with 0.5 µg of the indicated plasmid DNA: pET11-PrtASulAwt (wt), pET11-PrtASulA62H (62H), or pET11-PrtASulA62S (62S). The transformed cells were grown for 2 h at 37°C and then diluted in twofold steps in a 96-well plate. From each dilution 10-µl aliquots were spotted onto each of a series of 10 plates containing Luria-Bertani medium plus ampicillin (50 µg/ml) and 0, 0.0078, 0.0156, 0.0234, 0.0312, 0.0468, or 0.0625 mM IPTG. After incubation overnight at 37°C, colonies were counted for each IPTG concentration. The transformation efficiency was determined relative to that achieved with no IPTG and is plotted as the surviving fraction.

Second, the ability to induce filamentation when expressed in cells was examined. Figure 5 shows that cells expressing PrtA-SulAare blocked in division, resulting in filamentous growth, whereascontrols which express the mutant SulA fusion proteins are normalrods.

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FIG. 5. Effect of PrtA-SulA alleles on cell division. The cloned SulA alleles are as indicated; "none" refers to the vector lacking SulA. All panels show cells after IPTG-induced expression of the plasmid-encoded gene. Strain HMS174(DE3) was transformed with pET11a, pET11-PrtASulAwt, pET11-PrtASulA62H, and pET11-PrtASulA62S plasmids. One colony from each plate was inoculated into minimal medium (33) and 50 µg of ampicillin per ml at 37°C, then grown to an OD₆₀₀ of 0.2, and then induced with 0.5 mM IPTG for 4 h. Cells from 0.5-ml samples of each well were harvested, washed with 100 mM NaCl in 5 mM Tris-Cl (pH 7.4), and resuspended in 0.5 ml of water with 10 µM Syto-17 red fluorescent dye. Aliquots (10 µl) were spread on polylysine-coated glass slides and fixed with Permount as coverslips were mounted. Slides were examined with a Zeiss Axiovert inverted stage microscope with a ×100 oil immersion objective lens and a rhodamine fluorescence filter set. Exposure was for 4 s on ISO 400 film.

SulA inhibits FtsZ GTPase. An earlier report by Higashitani et al. (19) failed to detect any effect of a maltose binding protein-SulA fusion proteinon FtsZ GTPase activity. Since the PrtA-SulA fusion proteins carrya smaller additional domain (ca. 14 kDa), we considered it importantto investigate their effects on the GTPase activity of purifiedFtsZ protein. Each purified PrtA-SulA protein was preincubatedwith wild-type FtsZ protein prior to measuring GTPase activity(Fig. 6). Wild-type PrtA-SulA showed a significant level of inhibitionof FtsZ GTPase activity. In contrast, neither the PrtA-SulA62Hnor the PrtA-SulA62S mutant proteins exhibited an effect on GTPaseactivity. Preincubation of FtsZ led to a lag in its subsequentGTPase activity.

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FIG. 6. Effects of PrtA-SulA on FtsZ GTPase activity. The indicated PrtA-SulA fusion (5 µM) was each preincubated with 2 µM FtsZ for 5 min before the addition of GTP to the assay. The assays were followed for 20 min, withdrawing and quenching samples for analysis. The GTPase assay was done as described in Materials and Methods.

SulA inhibits FtsZ polymerization. The effect of the PrtA-SulA proteins on polymerization of FtsZ induced by DEAE-dextran was examined. Wild-type PrtA-SulA wasa potent inhibitor of FtsZ polymerization (Fig. 7), whereas thetwo mutants, PrtA-SulA62H and PrtA-SulA62S, did not inhibit FtsZpolymerization. Since the FtsZ2 mutant was originally isolatedas SulA insensitive, the effect of PrtA-SulA on FtsZ2 polymerizationwas compared with that of the wild type. Again, the results parallelthe in vivo observations; although polymerization of the wild-typeFtsZ protein was inhibited, there was only minimal effect on theFtsZ2 mutant (Fig. 7).

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FIG. 7. Effects of PrtA-SulA fusion proteins on FtsZ polymerization. Wild-type FtsZ (Z) or FtsZ2 (Z2) was present where indicated at a fixed concentration of 2 µM. Increasing amounts of wild-type PrtA-SulA protein (wt) or indicated mutant SulA fusion proteins (62S and 62H) were preincubated with FtsZ or FtsZ2 for 5 min at 37°C before polymerization was initiated by the addition of DEAE-dextran to 100 µg/ml. The sedimentation assay was then done as described in Materials and Methods. The results have been normalized to facilitate comparison of the data for FtsZ2 (95% sedimented in the absence of any SulA) and wild-type FtsZ (86% sedimented in the absence of any SulA).

Polymerization reactions in the presence of PrtA-SulA fusions were also examined by electron microscopy (data not shown).Wild-type FtsZ formed hundreds of tubules per grid square in thepresence of either SulA mutant fusion; these tubules were indistinguishablefrom the polymers formed in the absence of SulA in number andform. This finding contrasted dramatically with the complete absenceof visible polymers in the presence of equimolar wild-type PrtA-SulA,where at least a dozen grid squares were examined in each duplicategrid from four independent experiments. As judged by electronmicroscopy, FtsZ2 polymerization was not affected even by wild-typeSulA. The FtsZ2 structures observed were indistinguishable fromthose seen in the absence of SulA.

Polymerization was distinctly more sensitive to SulA than was GTPase to SulA (Fig. 8). It required stoichometric levels ofSulA (2 µM) to inhibit FtsZ GTPase activity, suggesting that a1:1 complex may be formed and implying that the affinity may onlybe in the 1-µM range. In contrast, polymerization of 2 µM FtsZwas inhibited 50% by PrtA-SulA at concentrations as low as 0.3to 0.5 µM, a finding corresponding to one-quarter or fewer SulAmolecules per FtsZ molecule. The affinity estimate from the GTPasestudies suggests that the actual number of SulA molecules activelyinvolved in the inhibition of FtsZ polymerization may be considerablylower than one per four FtsZ molecules.

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FIG. 8. Direct comparison of the effects of PrtA-SulA fusion proteins on FtsZ polymerization and on FtsZ GTPase activity. The wild-type PrtA-SulA fusion was titrated into reactions for GTPase or polymerization; in each case reactions were initiated by the addition of FtsZ wild-type protein. The assays were performed as described in Materials and Methods.

The order of addition of SulA to the polymerization reaction was investigated to ascertain whether SulA can cause the disassemblyof intact FtsZ polymers. SulA was either preincubated with FtsZbefore addition of DEAE-dextran or SulA was added last, afterthe DEAE-dextran; in either case it was inhibitory. Indeed, whenpolymers of FtsZ had already formed, the addition of equimolarSulA caused a rapid depolymerization within 5 min of its additionto FtsZ (data not shown). Shorter times could not readily be monitoredby the sedimentation assay, so this depolymerization might bemuch more rapid.

SulA interaction with FtsZ. Direct binding of the PrtA-SulA fusion to FtsZ was confirmed by affinity column chromatography. FtsZ and PrtA-SulA were mixedin the reaction buffer at 37°C for 15 min and subsequently passedover an IgG-Sepharose column which bound the PrtA-SulA fusion,presumably via the protein A domain. After the column was washed,the PrtA-SulA and any bound FtsZ were eluted and quantified bydensitometry of SDS-polyacrylamide gels versus standards. Alldetectable PrtA-SulA fusion protein was bound by IgG, regardlessof the SulA allele. Table 1 shows that the affinity column bearingwild-type SulA retained a significant amount of FtsZ, whereasno FtsZ was detected in the bound fractions when one of the mutantSulA alleles replaced the wild type. The extensive wash step makesthis method prone to underestimating the true extent of complexformation. It cannot be concluded that the mutant SulA proteinsfail to bind FtsZ but rather that any interaction is much weakerthan that of FtsZ with wild-type SulA. It was also seen that FtsZ2mutant protein bound to SulA to give a yield very similar to thatof wild-type FtsZ. This appears somewhat paradoxical in view ofthe ability of FtsZ2 to polymerize in the presence of SulA, butit is in agreement with a report that these two proteins can interactin the yeast two-hybrid system (20).

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TABLE 1. Affinity copurification of SulA and FtsZ^a

The interaction between the FtsZ2 mutant protein and SulA provided a way to determine whether SulA can bind efficiently toFtsZ subunits within the polymer. We tested whether PrtA-SulAwas cosedimented with the FtsZ2 polymer. Such cosedimentationshould be more sensitive for detecting interaction than is theaffinity copurification procedure since there is no wash stepas the polymers are sedimented through a solution containing SulAprotein. Despite the sensitivity of the method, cosedimentationof SulA dependent on FtsZ was not detectable with a variety ofratios of SulA either to wild-type FtsZ or to mutant FtsZ2 protein(Table 1). The level of SulA cosedimenting with FtsZ2 polymersprovides the most sensitive detection method since polymerizationis affected little even by excess SulA. In such FtsZ2 assays,as little as 2% of the input level (2 µM) of SulA could have beenmeasured in the pellet, but none was detected above the backgroundlevel (1%) of soluble protein trapped within the pellet of FtsZ2polymer. This suggests that the SulA protein does not bind tightlyto polymerized FtsZ2 protein along the entire length of the polymer.The possibility that SulA binds specifically to one or both endsof the FtsZ polymer is not excluded.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The results presented here document the inhibition of FtsZ polymerization by SulA, which likely leads directly to the arrestof cell division. Wild-type and mutant forms of these two proteinshave been compared in vitro and in vivo, providing evidence insupport of this notion.

Fusions of SulA protein were used to circumvent solubility problems encountered with the native protein. The SulA fusion proteinswere all tested for biological function in blocking cell division.Only the wild-type SulA fusion was a potent division inhibitor.Inhibition of FtsZ polymerization was observed only for the fusionsof the functional wild-type SulA protein and not for the mutantSulA proteins. This correlates with our in vivo results. The inabilityof the wild-type SulA to inhibit the FtsZ2 protein is consistentwith the selection used to isolate the ftsZ2 allele as SulA resistant.

Two extreme possibilities might be considered for the cellular role of FtsZ: (i) GTPase or signaling associated with GTP andGDP binding is the critical aspect of FtsZ function in the cell,or (ii) the ability to polymerize is the most crucial factor forFtsZ function during division. The properties of FtsZ2 supportthe idea that FtsZ acts as a polymer in the cell. FtsZ2 exhibitsa low level of GTPase activity, as low as or lower than the GTPaseactivity of the SulA-inhibited wild-type FtsZ protein. If GTPaseactivity were the primary requirement for FtsZ function, thenthe ftsZ2 mutant should be expected to resemble a loss-of-functionmutation. In contrast, FtsZ2 is fully capable of polymerizationunder our assay conditions even when SulA is present. If polymerizationis the crucial property of FtsZ, then the ftsZ2 mutants shouldbe able to divide. The phenotypes of ftsZ2 mutants best fit arole for the polymer.

Although mutants bearing a single copy of the ftsZ2 gene are not viable, it requires only a modest increase in expressionof FtsZ2 to grow at permissive temperature (4). If the levelof expression were increased even by sevenfold, then the correspondingstrains expressing increased wild-type FtsZ protein would be expectedto form filaments and minicells (41), whereas this is not reportedto be the case (4). Reducing wild-type FtsZ levels by morethan two- or threefold results in filamentous growth (14). Thus,despite the 200-fold reduction in the amount of FtsZ2 GTPase,the mutant protein is capable of almost wild-type function indivision at 30°C. These observations are not readily compatiblewith a primary function for FtsZ as a GTPase.

The extremely low level of FtsZ2 GTPase activity is intriguing. The structure of the Methanococcus jannaschii FtsZ protein(25), together with the high amino acid identity, suggests thata simple threading of the E. coli FtsZ amino acid sequence mayprovide a plausible approximation to the structure of the E. coliFtsZ protein. Such a model would place the FtsZ2 mutation (asparticacid 212 to glycine) at the opposite end of the FtsZ protein fromthe GTP-binding site. It is possible that this amino acid changecauses an overall alteration in the conformation of FtsZ, therebyaffecting the GTPase activity of the protein. However, a secondpossibility is suggested by a comparison of FtsZ with the structureof the tubulin polymer determined by electron diffraction (31),where the equivalent residue is in close proximity with the nucleotide-bindingsite of the neighboring tubulin molecule in the protofilament.The similarities between FtsZ and tubulin at the level of molecularstructure and also in their protofilament arrangement at lowerresolution (12) suggest that similar contacts might occur betweenFtsZ promoters in a protofilament. Thus, it is possible that theaspartic acid at position 212 may provide or stabilize part ofthe active site of the neighboring FtsZ subunit. The GTPase sitesin the Ras-GAP and Rho-GAP complexes (35, 37) provide a precedentfor this type of interaction.

The FtsZ2 protein copurified with SulA as an affinity ligand, with a yield almost as high as when wild-type FtsZ copurifiedwith SulA. This observation provides direct biochemical confirmationof the FtsZ2-SulA interaction detected by the yeast two-hybridsystem (20). Despite the affinity copurification of FtsZ2 proteinwith SulA, we did not detect significant cosedimentation of SulAwith FtsZ2 polymers, a less-stringent condition in that it omitsany wash step.

There are several possible explanations for this apparent discrepancy. First, SulA may interact preferentially with unpolymerizedFtsZ rather than the bulk FtsZ polymer. In this case SulA wouldshift the equilibrium between the FtsZ polymer and free FtsZ monomerby depleting the level of monomer to form a SulA-FtsZ complex.However, this hypothesis cannot easily explain why substoichiometriclevels of SulA were able to inhibit FtsZ polymerization so dramatically.

A second possibility is that SulA binds to an FtsZ subunit at one end of the polymer so as to destabilize that end and therebyfavor depolymerization. Such a site might plausibly overlap oneof the two contact surfaces of FtsZ involved in polymerization,so that it is only accessible at one end of the polymer but isexposed on each FtsZ monomer. This might explain the sensitivityof FtsZ polymerization to substoichiometric levels of SulA andalso the rapid depolymerization of FtsZ induced by addition ofSulA. The limits of detection in our assays allow the possibilitythat SulA interacts with one or both ends of the polymer. Thepossibility of active depolymerization of FtsZ by SulA was firstsuggested by in vivo results (3).

Inhibition of FtsZ GTPase requires stoichiometric levels of SulA, suggesting that a 1:1 complex of FtsZ and SulA may be responsiblefor the reduced level of GTPase. Such a SulA-FtsZ complex is consistentwith the binding data. The inhibition of the polymerization assayby substoichiometric levels of SulA may not be due to a differentkind of SulA-FtsZ interaction but may reflect the difference inthe sensitivity of the measurements. The conditions of the sedimentationassay did not lead to detectable sedimentation of DnaB hexamers(M_r of 300,000 for the hexamer [data not shown]), so that it seemslikely that the FtsZ polymers which readily sediment consist ofmore than six protomers of FtsZ. In such a case, one SulA moleculeper 10 or more FtsZ molecules may be sufficient to disrupt detectablepolymers in the sedimentation assay. In agreement with this approximatesize limit, no significant assemblies of FtsZ were observed byelectron microscopy when SulA was present, but where FtsZ miniringsof approximately 15 to 20 FtsZ promoters are readily detectedby electron microscopy.

This discussion would be incomplete without considering the contrast between our observations of SulA inhibition of FtsZ GTPaseactivity and those of an earlier report (19) in which no effectof SulA on GTPase was seen. Several explanations might be considered.First, the differences in GTPase reaction conditions may explainthe different observations. Second, the larger maltose bindingprotein fusion partner used in the earlier study may account forthe differences; perhaps it allows binding of SulA to FtsZ buthinders a second interaction that mediates the inhibitory effectof SulA. Finally, we noted that the GTPase activity of FtsZ issignificantly less sensitive to SulA than is the polymerizationof FtsZ. The experiments of Higashitani et al. (19) may haveused SulA at a concentration which is too low to cause significantinhibition of FtsZ GTPase.

Earlier studies had identified the ability of DEAE-dextran to promote the polymerization of FtsZ (12, 30). These observationshave been extended by the present study to provide a quantitativebiochemical assay at a physiological pH. The behavior of wild-typeand mutant FtsZ and SulA proteins argues that the DEAE-dextranpolymerization assay reflects at least some of the important cellularconditions. Nevertheless, caution is required since this is adifferent situation from that in the bacterial cell.

While DEAE-dextran represents an artificial condition, we speculate that it may mimic the effects of a factor which normallynucleates or stabilizes FtsZ polymers in the cell. Such a factoris expected to be located in the inner membrane and may be a knowndivision protein, such as the recently identified ZipA protein(17). It is plausible that FtsZ does not polymerize efficientlyunder physiological conditions without a positively charged factorto nucleate or stabilize the polymeric form. It is noteworthythat the cytoplasmic domains of most Fts proteins carry a significantnet positive charge. Although none of the other Fts proteins isessential for localizing FtsZ to a ring, the stability or frequencyof the FtsZ rings is reduced in mutants affected in a number offts genes (1, 24, 32).

The availability of a purified FtsZ polymerization assay which responds to authentic cellular regulators provides a powerfultool for future studies of the molecular mechanisms of divisionand its control.

	ACKNOWLEDGMENTS

We thank D. Pompliano, J. Kozarich, and I. Singer for their support of this work and Xiling Yuan for the DNA sequencing toconfirm constructs.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Enzymology, Building 80Y-325, Merck Research Laboratories, 126 East LincolnAvenue, Rahway, NJ 07065-0900. Phone: (732) 594-6092. Fax: (732)594-5878. E-mail: david_bramhill{at}merck.com.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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	ALL ASM JOURNALS

1.	Addinall, S. G., E. Bi, and J. Lutkenhaus. 1996. FtsZ ring formation in fts mutants. J. Bacteriol. 178:3877-3884[Abstract/Free Full Text].
2.	Bi, E., and J. Lutkenhaus. 1990. Analysis of ftsZ mutations that confer resistance to the cell division inhibitor SulA (SfiA). J. Bacteriol. 172:5602-5609[Abstract/Free Full Text].
3.	Bi, E., and J. Lutkenhaus. 1993. Cell division inhibitors SulA and MinCD prevent formation of the FtsZ ring. J. Bacteriol. 175:1118-1125[Abstract/Free Full Text].
4.	Bi, E., and J. Lutkenhaus. 1992. Isolation and characterization of ftsZ alleles that affect septal morphology. J. Bacteriol. 174:5414-5423[Abstract/Free Full Text].
5.	Bi, E. F., and J. Lutkenhaus. 1991. FtsZ ring structure associated with division in Escherichia coli. Nature 354:161-164[Medline].
6.	Bramhill, D. 1997. Bacterial cell division. Annu. Rev. Cell Dev. Biol. 13:395-424[Medline].
7.	Bramhill, D., and C. M. Thompson. 1994. GTP-dependent polymerization of Escherichia coli FtsZ protein to form tubules. Proc. Natl. Acad. Sci. USA 91:5813-5817[Abstract/Free Full Text].
8.	Chang, C. F., H. Shuman, and A. P. Somlyo. 1986. Electron probe analysis, X-ray mapping, and electron energy-loss spectroscopy of calcium, magnesium, and monovalent ions in log-phase and in dividing Escherichia coli B cells. J. Bacteriol. 167:935-939[Abstract/Free Full Text].
9.	de Boer, P., R. Crossley, and L. Rothfield. 1992. The essential bacterial cell-division protein FtsZ is a GTPase. Nature 359:254-256[Medline].
10.	Dubendorff, J. W., and F. W. Studier. 1991. Controlling basal expression in an inducible T7 expression system by blocking the target T7 promoter with lac repressor. J. Mol. Biol. 219:45-59[Medline].
11.	Erickson, H. P. 1997. FtsZ, a tubulin homologue in prokaryote cell division. Trends Cell Biol. 7:362-368. [Medline]
12.	Erickson, H. P., D. W. Taylor, K. A. Taylor, and D. Bramhill. 1996. Bacterial cell division protein ftsZ assembles into protofilament sheets and minirings, structural homologs of tubulin polymers. Proc. Natl. Acad. Sci. USA 93:519-523[Abstract/Free Full Text].
13.	Gangola, P., and B. P. Rosen. 1987. Maintenance of intracellular calcium in Escherichia coli. J. Biol. Chem. 262:12570-12574[Abstract/Free Full Text].
14.	Garrido, T., M. Sanchez, P. Palacios, M. Aldea, and M. Vicente. 1993. Transcription of ftsZ oscillates during the cell cycle of Escherichia coli. EMBO J. 12:3957-3965[Medline].
15.	Gayda, R. C., L. T. Yamamoto, and A. Markovitz. 1976. Second-site mutations in capR (lon) strains of Escherichia coli K-12 that prevent radiation sensitivity and allow bacteriophage lambda to lysogenize. J. Bacteriol. 127:1208-1216[Abstract/Free Full Text].
16.	George, J., M. Castellazzi, and G. Buttin. 1975. Prophage induction and cell division in E. coli. III. Mutations sfiA and sfiB restore division in tif and lon strains and permit the expression of mutator properties of tif. Mol. Gen. Genet. 140:309-332[Medline].
17.	Hale, C. A., and P. A. J. de Boer. 1997. Direct binding of FtsZ to ZipA, an essential component of the septal ring structure that mediates cell division in E. coli. Cell 88:175-185[Medline].
18.	Hanahan, D. 1983. Studies on transformation of Escherichia coli with plasmids. J. Mol. Biol. 166:557-580[Medline].
19.	Higashitani, A., N. Higashitani, and K. Horiuchi. 1995. A cell division inhibitor SulA of Escherichia coli directly interacts with FtsZ through GTP hydrolysis. Biochem. Biophys. Res. Commun. 209:198-204[Medline].
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