Constitutive Septal Murein Synthesis in Escherichia coli with Impaired Activity of the Morphogenetic Proteins RodA and Penicillin-Binding Protein 2

doi:10.1128/JB.183.14.4115-4126.2001

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Journal of Bacteriology, July 2001, p. 4115-4126, Vol. 183, No. 14
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.14.4115-4126.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Constitutive Septal Murein Synthesis in Escherichia coli with Impaired Activity of the Morphogenetic Proteins RodA and Penicillin-Binding Protein 2

Miguel A. de Pedro,¹^,^* William D. Donachie,² Joachim-Volker Höltje,³ and Heinz Schwarz³

Centro de Biología Molecular "Severo Ochoa," Consejo Superior de Investigaciones Científicas-Universidad Autónoma de Madrid, Campus de Cantoblanco, 28049 Madrid, Spain¹; Institute of Cell and Molecular Biology, The University of Edinburgh, Edinburgh EH9 3JR, Scotland²; and Max-Planck Institut für Entwitcklungsbiologie, D-7400 Tübingen, Germany³

Received 20 February 2001/Accepted 27 April 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The pattern of peptidoglycan (murein) segregation in cells of Escherichia coli with impaired activity of the morphogeneticproteins penicillin-binding protein 2 and RodA has been investigatedby the D-cysteine-biotin immunolabeling technique (M. A. de Pedro,J. C. Quintela, J.-V. Höltje, and H. Schwarz, J. Bacteriol. 179:2823-2834,1997). Inactivation of these proteins either by amdinocillin treatmentor by mutations in the corresponding genes, pbpA and rodA, respectively,leads to the generation of round, osmotically stable cells. Innormal rod-shaped cells, new murein precursors are incorporatedall over the lateral wall in a diffuse manner, being mixed uphomogeneously with preexisting material, except during septation,when strictly localized murein synthesis occurs. In contrast,in rounded cells, incorporation of new precursors is apparentlya zonal process, localized at positions at which division hadpreviously taken place. Consequently, there is no mixing of newand old murein. Old murein is preserved for long periods of timein large, well-defined areas. We propose that the observed patternsare the result of a failure to switch off septal murein synthesisat the end of septation events. Furthermore, the segregation resultsconfirm that round cells of rodA mutants do divide in alternate,perpendicular planes as previously proposed (K. J. Begg and W.D. Donachie, J. Bacteriol. 180:2564-2567,1998).

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The peptidoglycan (murein) sacculus is the principal stress-bearing and shape-maintaining element of the cell wall and playsan essential role in bacterial morphogenesis. Growth of Escherichiacoli occurs by periodic alternation of elongation and divisionevents (2, 14). Newborn cells elongate and then divide atmidcell once the chromosome is replicated and the initial mass(length) is doubled (17, 20). Cell elongation demands theconcomitant enlargement of the sacculus, and cell division requiresthe formation of a transverse septum at its center (2, 14,40).

Elongation and septation of the sacculus require insertion of new precursors by the concerted action of murein biosyntheticand hydrolytic enzymes (25, 39, 46). Among the former, penicillin-bindingproteins (PBPs) are of particular interest as the enzymes thatactually polymerize monomeric subunits and cross-link the resultingnew strands to the preexisting murein (15, 36, 48, 52).In E. coli, PBP2 and -3 have well-defined morphogenetic roles.PBP3 is specifically and absolutely required for septal mureinsynthesis. Inhibition of PBP3 activity blocks septation and leadsto filament formation. Impairment of PBP2 activity leads to thegeneration of pleiomorphic, spherical cells (3, 18, 22,41, 48, 49, 53, 55, 57, 58, 61). Enzymaticallyboth proteins have DD-transpeptidase activities in vitro, butno transglycosylase activity has been reliably demonstrated foreither of them (26, 56). To be fully functional, PBP2 apparentlyrequires an active RodA protein (26). Impairment of either RodAor PBP2 leads to similar phenotypes. However, the enzymatic activityof RodA remains to be identified. Because the activities of bothPBP2 and RodA are needed to keep the rod-like morphology of thecell, they are thought to be required for side wall murein synthesisduring elongation of the cell wall (3, 11, 13).

Amdinocillin is a $beta$ -lactam antibiotic that binds with high affinity and specificity to PBP2. The effects of amdinocillin aregenerally attributed to its inhibitory action on PBP2, but thepossibility of additional effects cannot be totally discounted(27, 43, 50). Inhibition of PBP2 by amdinocillin leads toimportant alterations in murein composition and rate of synthesis.Upon addition of amdinocillin, the rate of murein synthesis isreduced by about 50%, but the rate of growth and division remainsconstant for roughly one doubling in cell mass. Therefore, theamount of murein per cell drops to about one-half the normal value.Concomitantly cells become spherical, cell division is blocked,large multinucleated cells are generated, and viability is lost(11, 12, 31, 37, 47, 50). Spherical cells are alsogenerated by mutations in the genes pbpA and rodA (coding forPBP2 and RodA, respectively). Thermosensitive mutations in bothgenes (pbpA45 and rodA52) were first obtained by using amdinocillinresistance as the selective criterion. At the restrictive temperature(42°C) both pbpA(Ts) and rodA(Ts) strains are viable, resistantto amdinocillin, and have a round cell morphology (28, 29,37, 51, 55). At permissive temperatures (30°C), the rodA(Ts)mutant has normal morphology, but the pbpA(Ts)strain has a near-sphericalshape in stationary-phase culture (45). Inactivation of eitherrodA or pbpA results in round cells that are unable to grow anddivide in rich medium, although these round cells are viable inminimal medium. Both kinds of deletion mutants can, however, growand divide well in rich medium if the level of FtsA and FtsZ divisionproteins is increased. This can result from either an increasein the copy number of these genes (on plasmid vectors) or mutationsthat increase transcription of these two genes (6). Divisionof rounded cells is efficient but abnormal in several respects(4, 6, 51, 55). The larger-than-normal diameter of thecell impedes formation of a complete FtsZ ring as required fornormal septation (1, 7, 35, 54). Polymerization of FtsZat the future division site leads instead to partial rings, whichare nevertheless able to direct a lateralized invagination ofthe envelope (19, 28, 64). Progressive invagination eventuallyleads to cell separation. Interestingly, successive divisionsseem to occur in perpendicularly alternating planes (4, 65).In addition, pbpA(Ts) mutants have a tendency to divide irregularlyto give cells of different sizes (45).

Because PBP3 and PBP2 plus RodA are apparently involved in discrete morphological events, it has been proposed that togetherwith additional proteins (such as FtsW, a close homologue of RodA)(9, 32, 57), each could be part of murein biosyntheticcomplexes active at alternating periods of the cell cycle (38).In these models, PBP3-containing complexes would be active exclusivelyat the septation period and PBP2-containing ones would be activeduring the elongation phase of cell growth or both elongationand division (3, 8, 10, 13, 16). An implication ofsuch models is that murein synthesized upon PBP2 impairment shouldbe made by complexes that are normally committed to septationand therefore should have the properties of septal murein (51).

Application of a new method to the analysis of murein segregation in E. coli (16) confirmed and complemented previous resultsthat support "two-complex" models (8, 10, 40, 60, 62,63). According to our interpretation, during cell elongation,new precursors are inserted in a diffuse fashion into the cylindricalpart of the sacculus, but not at the polar caps, which do notundergo further expansion. However, shortly before septation actuallystarts, a strongly localized murein biosynthetic activity is triggeredat the putative division site in an FtsZ-dependent process. Activationof septal murein synthesis (SMS) results in the generation ofa ring of all-new murein around the cell, which in time developsinto a circumferential invagination that is completed to formtwo new poles. Inhibition of cell division at any stage laterthan FtsZ ring formation leads to the generation of a ring ofnew murein, which grows for a defined period of time and thenstops, generating an annular zone of new and inert murein. Thestudies of murein segregation suggest therefore some kind of periodicactivation and inactivation of a septal murein biosynthesis complex,whose activity may alternate, or overlap, with that of complexesinvolved in lateral wall synthesis, which could in turn be directedby the PBP2 and RodAproteins.

We were therefore interested in studying murein segregation in strains with impaired activity of the PBP2 and RodA proteins.The mode of insertion of new materials under conditions in whichcell wall growth is exclusively directed by septation complexescould be substantially different from that in normal cells andcould help to explain the way in which viable dividing sphericalcells areformed.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains and growth conditions. The E. coli strains used in this work were MC6RP1 (K-12 F dra drm leuA lysA proA thi thr) (44), SP4500 [K-12 F his pro purB thi mtl xyl galK lacY rpsL pbpA45(Ts)], SP5211 [K-12F his pro purB thi mtl xyl galK lacY rpsL rodA52(Ts)] (51), andKJB24 [K-12 IN(rrnD-rrnE)1 rodA^Sui(Am) ddlB::Tn5] (4). Cultures were routinely grown in Luria-Bertani(LB) medium (34) at the appropriate temperature in gyratorywater baths. Growth was monitored by measuring the optical densityof the cultures at 550 nm (OD₅₅₀).

D-Cysteine labeling of murein. Labeling was performed as described previously (16). Flasks containing appropriate volumes of prewarmed medium were inoculated(OD₅₅₀, $approx$ 0.03) from overnight cultures of the selected bacterialstrain and incubated until they had reached an OD₅₅₀ of $approx$ 0.06.At that moment, D-Cys was added to the cultures to a final concentrationof 100 µg/ml, and cultures were further incubated for three doublingsin cell mass as determined by measuring the OD₅₅₀. To remove D-Cys,cultures were centrifuged (5 min, 20,000 × g) at the temperatureused for growth, resuspended into an equal volume of D-Cys-freemedium prewarmed at the growth temperature, centrifuged againas described above, and finally resuspended in the medium appropriatefor each experiment. Cultures were further processed accordingto the specific requirements of individualexperiments.

Purification, biotinylation, immunolabeling, and observation of sacculi. Sacculi were purified, reduced with NaH₄B, biotinylated at the free thiol groups, and immunolabeled for either epifluorescenceor electron microscopy exactly as described previously (16).Observation and photographic work were performed with the sameinstruments used before (Zeiss Axioplan fluorescence microscopefitted with a 100×/1.3 Neofluar objective and a Philips CM10 transmissionelectron microscope at an acceleration voltage of 60kV).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Effect of amdinocillin on murein segregation in E. coli MC6RP1. Cultures of E. coli MC6RP1 labeled with D-Cys were transferred to prewarmed D-Cys-free medium containing amdinocillin at 1µg/ml. At increasing chase times, 25-ml samples were removed,and murein was purified and prepared for immunoelectron microscopyand immunofluorescence microscopy. Upon addition of amdinocillin,E. coli cells are able to complete the ongoing round of cell division,but are unable to complete any further divisions (11, 12,47). Sacculi from nonchased cells (Fig. 1A) showed a homogeneousand dense distribution of gold grains over their surface. Sacculifrom cells chased for one mass doubling time already showed clearsigns of rounding. Most of them presented a gold grain-free pole,indicating that a division had taken place after the removal oflabel (Fig. 1B). After a longer chase (Fig. 1C), all sacculi hadacquired aberrant shapes. Most were either pear shaped (with theolder pole closing the small end of a conical section closed onthe other side by a hemisphere) (Fig. 1C¹) or hourglass shaped (Fig. 1C²). Only a few were actually spherical (Fig. 1C³). Most remarkable was that, in contrast to the observations withfilaments and normal cells (16), large sharply delimited areasof labeled and unlabeled murein were present. The surface areacovered by old (gold marked) and new (gold free) murein was roughlyequal after two doubling times. In all instances, the large areasof all-new murein (unlabeled) appeared in places at which a divisionhad already been completed or a new one had started. The distributionof gold grains in the labeled areas was essentially homogeneous.Interestingly, the hourglass-shaped sacculi had an additionalsmall area free of gold grains in one of the poles (Fig. 1C²), indicative of an early division. Another interesting observationwas that the total number of gold grains per sacculus (256 ± 66grains/sacculus, n = 26) was about one-half of the value for cellsat the beginning of the chase period (452 ± 110 grains/sacculus,n = 18). Because cells do divide once in the presence of the drug,these results indicate that most of the old murein is conservedthroughout the chase period.

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FIG. 1. Immunoelectron microscopy of D-Cys-labeled murein in amdinocillin-treated cells of MC6RP1. Cells from a culture grown for three generations in LB medium supplemented with D-Cys were harvested by centrifugation and transferred to medium without D-Cys, but containing 1 µg of amdinocillin per ml. As a control, an aliquot was transferred to medium with both amdinocillin and D-Cys at the concentrations shown above. At the indicated chase times, samples were removed and further processed for murein purification, biotinylation, immunolabeling, and electron microscopy as described in Materials and Methods. Gold-conjugated (6-nm-diameter grains) protein A was used for the detection of antibodies. (A) Chase time zero. (B) Cells chased for one doubling in cell mass. (C) Cells chased for two doublings in cell mass. The arrowhead indicates a gold-free pole. (D) Control cells incubated for two doublings in cell mass in D-Cys plus amdinocillin. All pictures are at the same magnification.

Fluorescence microscopy of the same sacculus samples gave similar results. In particular, the images corresponding to sacculichased for two doubling times validated the electron microscopyones discussed above. That the shapes shown in the electron microscopypictures (Fig. 1) were by no means rare was clear from pictureslike the one in Fig. 2. Again the labeled (old) murein appearedas a large area of essentially uniform brightness. The shapesof the bright areas clearly corresponded to the gold-labeled onesfound in the electron microscopy pictures.

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FIG. 2. Immunofluorescence microscopy of D-Cys-labeled murein in amdinocillin-treated cells of MC6RP1. Aliquots of the same sacculi purified for the experiment shown in Fig. 1 were subjected to immunofluorescence microscopy for the detection of D-Cys-labeled areas with a fluorescein isothiocyanate-labeled goat anti-rabbit antibody. The picture shows sacculi chased for two doublings in cell mass, corresponding to Fig. 1C. V-shaped and rhomboidal arrowheads indicate sacculi similar to the ones in Fig. 1C¹ and C², respectively. The inset shows selected sacculi from the sample incubated for the same time in D-Cys plus amdinocillin (Fig. 1D).

Murein segregation in the E. coli pbpA(Ts) strain SP4500. The pbpA(Ts) mutant strain SP4500 is amdinocillin resistant and has a round cell morphology at 42°C. To monitor murein segregationat 42°C, cells were first labeled with D-Cys and then chased inD-Cys-free medium before purification of the sacculi. The detailedpattern of segregation could not be as clearly established asthat described above, although it was rather evident that incorporationof new material was essentially a localized event. Large areasof neatly delimited old and new murein were segregated duringthe chase period in accordance with the results for amdinocillin-treatedcells (Fig. 3).

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FIG. 3. Immunoelectron microscopy of D-Cys-labeled murein in cells of the pbpA(Ts) mutant SP4500. Cells from a culture grown for three generations in LB medium supplemented with D-Cys at 42°C were harvested by centrifugation. One sample was immediately subjected to murein purification, and the rest of the cell suspension was transferred to prewarmed medium without D-Cys and further incubated for one and a half generations. Sacculi were purified, biotinylated, and immunolabeled as indicated in Materials and Methods. Gold-conjugated (6-nm-diameter grains) protein A was used for the detection of antibodies. (A) Nonchased sacculi. (B) Sacculi chased for one and a half doublings in mass. All pictures are at the same magnification.

Murein segregation in the E. coli rodA(Ts) mutant SP5211 Cells of the rodA(Ts) mutant strain SP5211 have a normal rod shape at 30°C, which is lost upon transfer to 42°C, resemblingthe morphological change induced by amdinocillin. To investigatemurein segregation in this mutant, cells were labeled with D-Cysat 30°C, and then D-Cys was removed by centrifugation and thecells were resuspended in D-Cys-free medium (prewarmed at 42°C)to initiate the chase period. Sacculi from cells chased at 42°Ckept a rod-like morphology for the first doubling in mass, andup to this point, the segregation of murein corresponded to theobservations in wild-type cells. Septal rings of all-new mureinwere clearly visible in some sacculi, and most of them had onepole without label, indicative of a division event (Fig. 4B).Transition into a round shape was a smoother process than in amdinocillin-treatedcells, probably because SP5211 continues to divide at the restrictivetemperature. As previously observed, once cells start gettingrounded, as in Fig. 4B, septation starts as a localized invaginationand proceeds asymmetrically (Fig. 4C¹). After completion of division, cells were produced with sacculivery much like the ones generated by amdinocillin treatment (Fig.4C² to 4C⁴). Some had one large, densely labeled area and a gold-free one(Fig. 4C² to 4C³), and others had a central belt of gold grains (Fig. 4C⁴). The former represent cells that conserved one of the polesof the initially labeled cell (Fig. 4C¹, labeled pole), whereas the latter correspond to cells that inheriteda new pole after each round of division (Fig. 4C¹, unlabeled pole). Interestingly the latter kind of cells conservemore gold grains than corresponding sacculi from cells chasedfor the same time at 30°C (Fig. 4D). This suggests that dilutionof old lateral wall material with new material was slower in therounding cells. The end result was the accumulation of sacculiwith large delimited areas of all-new and all-old murein, as inthe previous cases. As described above, the distribution of goldgrains in the areas of old murein was rather homogeneous. Cellschased at 30°C behaved like the wild type: that is, polar regionsretained all of their original label, whereas label was progressivelydiluted in the rest of the sacculus, and septal rings of new mureinwere associated with division sites (data not shown).

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FIG. 4. Immunoelectron microscopy of D-Cys-labeled murein in cells of the rodA(Ts) mutant SP5211. Cells from a culture grown for three generations in LB medium supplemented with D-Cys (150 µg/ml) at 30°C were harvested and transferred to D-Cys-free medium prewarmed at 30 and 42°C. Cultures were further incubated at the respective temperature, and after one and two doublings in cell mass, samples were removed and further processed for sacculus purification, biotinylation, immunolabeling, and electron microscopy as indicated in Materials and Methods. Gold-conjugated (6-nm-diameter grains) protein A was used for the detection of antibodies. (A) Sacculi from control, nonchased cells. (B) Sacculi chased for one doubling in cell mass at 42°C. (C) Sacculi chased for two doublings in cell mass at 42°C. (D) Sacculi chased for two doublings in cell mass at 30°C. All pictures are at the same magnification.

Murein segregation in the E. coli rodA° mutant KJB24 Although the RodA protein is required for normal cell shape, it is not strictly essential for cell viability. Null mutantsare viable in minimal medium, in which growth is slow and thecell diameter is small, and plasmids or secondary mutations thatincrease the production of FtsA and FtsZ division proteins allowcell division in the larger cells formed in rich medium. In strainKJB24, a Tn5 insertion in the ddlB gene, immediately upstreamof ftsQ, ftsA, and ftsZ, causes increased transcription of thesegenes and allows the strain to grow and divide well in rich medium(3). Null mutant cells are spherical in shape and have a widerange of sizes, although they keep the ability to divide at thecentral plane of the sphere. A point of particular interest isthat successive division planes are perpendicular to each other(4). The results presented above suggest that disruption ofthe PBP2-RodA system results in localized and continuous synthesisof new murein at the division sites and in conservation of theold murein. Therefore, in strain KJB24, the sacculus of a newlyborn cell should consist of two hemispheres: one made of old mureinand the other made of new murein. After a second round of division,at 90° to the preceding one, each daughter cell should have a90° spherical sector of old murein and 270° of new murein (Fig.5A). To check this prediction, KJB24 was labeled with D-Cys andchased for one and two mass doubling times as described above.Although collapsing and folding of the large spherical sacculiobscured observation in many instances, sacculi with the predicteddistribution of gold grains for the first and the second roundsof division (Fig. 5B and C) were relatively frequent. In the samplechased longer, about 37% of sacculi were one-quarter labeled (Fig.5C6), and about 25% were from cells dividing for the second timeto give one-quarter-labeled sacculi (Fig. 5C4 and C5). Most othersacculi were either folded or oriented in ways that impeded aproper classification. The high proportion of sacculi with thepredicted distribution of label supports the conclusions reachedfrom observations of cell morphology. Incidentally, KJB24 sacculiappeared to be rather fragile, because a considerable proportionof them showed clear signs of degradation (data not shown), possiblybecause of lysis (4).

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FIG. 5. Murein segregation in the rodA° mutant KJB24 as observed by immunoelectron microscopy. Cells from a culture grown for three generations in LB medium supplemented with D-Cys were harvested and transferred to prewarmed D-Cys-free medium. Cultures were further incubated, and after one and two doublings in cell mass, samples were removed and further processed for sacculus purification, biotinylation, immunolabeling, and electron microscopy as indicated in Materials and Methods. Gold-conjugated (6-nm-diameter grains) protein A was used for the detection of antibodies. (A) Hypothetical segregation pattern. (B) Schematic representation of the actual segregation pattern as found in the images shown in panel C. The profile, position, and number of dots were drawn from the real pictures by using digitized images and PhotoShop software. (C) Immunolabeling of D-Cys in selected sacculi after no chase (panel 1) or after chase for one (panels 2 and 3) and two (panels 4 to 7) doublings in cell mass. The numbers in panels B and C correspond. All pictures are at the same magnification.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Previous studies of murein segregation by the D-amino acid labeling technique revealed two features relevant to an understandingof cell wall growth in E. coli. First, the polar caps of the cellsacculus are metabolically inert, and second, at the initiationof septation, there is local activation of murein synthesis atthe future division site, the place at which new poles will begenerated (16). Therefore, it seems quite straightforward topropose a direct relationship between the two phenomena: localizedsynthesis at the division site produces septal (later polar) murein,which is inert either because of some intrinsic property or becauseof topological influences. Investigation of murein segregationupon impairment of PBP2 or RodA function further supports thisidea.

Inhibition of PBP2 by amdinocillin led to a profoundly altered segregation pattern. After one doubling in mass, most sacculiwere slightly ovoid in shape and had gone through a division event.The distributions of gold grains at this stage in amdinocillin-treatedand untreated sacculi were similar. Further incubation of cellswith amdinocillin resulted in the generation of large sacculiwith bizarre morphologies and distribution of gold grains. Mostfrequently, chased sacculi had a distinct conical shape with arelatively narrow apex and a large hemispherical base. The apexand lateral (i.e., conical) areas retained a large proportionof old murein, as indicated by their heavy labeling upon immunodetectionof D-Cys residues. In contrast, the large basal area seems tobe made exclusively of new murein, because no D-Cys was detectedby immunomicroscopy. A significant proportion of cells were apparentlyable to reach a rather advanced stage of a second division roundand generated sacculi in which two units similar to the one describedabove were connected by the wide ends. The connection was oftendisplaced to one side instead of being central as previously described(3, 4). In these sacculi, segregation of old murein in eachhalf-cell followed a pattern similar to the one described abovefor single cells, resulting in sacculi with two large areas oflabeled murein at the former poles separated by a large area ofall-new murein divided by a furrow. Therefore, inhibition of PBP2by amdinocillin results in a modified pattern of murein segregation.In this pattern, most or all of the old murein is conserved intwo equal domains corresponding to the two hemispheres of theoriginal cell and two all-new half-cells are formed between themto generate a pair of sister cells. Thus, each sister cell consistsof two equal hemispheres, one of which consists of all-new mureinand the other of which consists of conserved old murein. Thisis the classical pattern for natural coccal species such as Enterococcusfaecalis (24), in which growth consists entirely of the formationof new cell halves. In Enterococcus and, we believe, in coccalmutants of E. coli, cell division (i.e., the formation of newcell halves) is synonymous with cellgrowth.

According to the measurements of the numbers of gold grains in sacculi at the end of the labeling period and after two massdoublings in the presence of amdinocillin, most of the old mureinseems to be conserved. Indeed, as cells are able to go throughone division event, the amount of grains per sacculus should bearound one-half of the value at the initiation of the chase, whichis remarkably similar to the actual values. Therefore, recyclingseems to have been reduced to a minimum under these conditions.If this were not so, a significant part of the old, labeled mureinshould have been lost (about one-half, assuming a moderate turnoverrate of 30% per generation) (23, 30, 42). The reductionin murein recycling is also consistent with the interpretationthat round cells consist entirely of septal murein. As previouslyreported, septal (polar) murein turns over extremely slowly, ifat all (16, 33).

Because PBP2 is the target for amdinocillin, murein segregation was also studied with the pbpA(Ts) mutant SP4500. However,it is important to realize that the segregation patterns for amdinocillin-treatedcells and the pbpA(Ts) mutant cannot be directly compared becauseof the very different experimental conditions used. Amdinocillin-treatedcells were in a morphological transition to rounded forms andwere the result of a single division event. In contrast, the pbpA(Ts)mutant was spherical, showed a large dispersion in cell size,and could divide more than once, often in an asymmetric way (Fig.3B). Because pbpA(Ts) cells are spherical during the labelingperiod, no "polar" regions can be defined. Evaluation of the numberof divisions a cell has gone through is also uncertain. Dividingcells are very disperse in size, and asymmetric divisions generatean unequal distribution of old and new murein between daughtercells. Nevertheless, old (labeled) and new murein segregated inall instances as large, well-delimited domains on the surfaceof the sacculi, which supports a zonal mode of murein synthesis.This result is consistent with the observations in amdinocillin-treatedcells and reinforces the idea that impairment of PBP2 activitypermanently blocks the diffuse mode of murein growth responsiblefor cell wallelongation.

When the rodA(Ts) mutant SP5211 is transferred to restrictive conditions, the cells undergo a morphological change similarto that observed in amdinocillin-treated wild-type cells (51).However, acquisition of the round shape is more gradual, possiblybecause division continues in spite of cell deformation. Duringthe first doubling in cell mass at the restrictive temperature,murein segregation was similar to that in the wild type or inthe mutant itself at 30°C, except that cells were slightly morerounded (Fig. 4B). However, upon further incubation, sacculi becameprogressively more rounded and had a distribution of label similarto the ones observed in amdinocillin-treated cells. Most sacculihad large areas where new and old murein did not intermix andtherefore appeared as discrete labeled and unlabeled regions (Fig.4C).

The observed patterns of segregation and morphological evolution suggest the following model. In normal cells (Fig. 6A), septationwould occur by the FtsZ-dependent activation of SMS at the potentialdivision site and the concomitant inhibition of lateral wall mureinsynthesis. Upon septum completion, SMS is shut off, murein atthe new poles becomes metabolically inert, and PBP2-promoted lateralwall murein synthesis proceeds until the next division cycle bydiffuse incorporation of precursors all over the cylindrical surfaceof the sacculus (8, 10, 12, 21). The consequences ofamdinocillin treatment depend on the age of individual cells atthe time of drug addition. Elongating but nondividing cells (Fig.6B) complete the ongoing period of lateral wall synthesis, SMSis triggered, and septation proceeds to completion. However, inhibitionof PBP2 activity prevents SMS from being switched off. Becausethe SMS system is localized and makes inert murein, large areasof all-new murein are generated at the new polar regions. Incidentally,a molecular interaction between RodA and the septal peptidoglycansynthetase PBP3 has been proposed on the basis of genetic complementationexperiments (5). Cells that are dividing at the time of drugaddition (Fig. 6C) might be able to switch from septal to lateralwall synthesis before amdinocillin actually blocks PBP2 activity.Lateral wall expansion is started, but because of PBP2 inactivation,the regular rod shape cannot be properly maintained. Cells increasein diameter, and FtsZ assembles as incomplete rings, which arenevertheless competent to trigger SMS (1). The septation eventis started as a lateral furrow, which grows into a bilobed surfaceof new murein for an undefined period of time, generating thepeculiar morphology and segregation pattern shown in Fig. 1C². Thermosensitive mutations in pbpA and rodA or null mutationsin rodA would generate spherical cells by essentially the samemechanism. That is, they would generate such cells by suppressinglateral wall murein synthesis and keeping SMS permanently on.In these mutant spherical cells, each round of SMS would end withthe completion of the new hemispherical sections and, in the absenceof the system for lateral wall synthesis, be succeeded by theimmediate initiation of a new round of SMS. Thus, sacculus growthand cell division would continue essentially in the same way asin natural gram-negative cocci such as Neisseria spp. (59).

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FIG. 6. Diagrammatic representation of the generation of rounded cells by the action of amdinocillin (mecillinam). Dark gray areas show newly synthesized septal murein; Light gray areas show newly made lateral wall murein. L.W.S., lateral wall murein synthesis.

Septation in round E. coli cells, as in Neisseria, is an asymmetric process (3, 4, 59, 64, 65). The analysis ofsacculi reported here shows that septal invagination in sphericalsacculi starts as a lateral furrow that produces a two-lobed sacculus.The lateral furrow then progresses inwards, making the two lobesdeeper until eventually two new spherical cells are released.An essentially identical series of events has been proposed onthe basis of cell morphology and FtsZ ring formation in sphericalcells (1, 64).

Previous studies of the growth and division of rodA° mutants showed that the lack of RodA protein leads to generation of spherical,viable cells, which divided in alternate perpendicular planes(3, 4). The results of murein segregation experiments insuch a strain were consistent with both the proposed mode of celldivision and with the model proposed for growth of the sacculusupon disturbance of the PPB2-RodA system. Based on the assumptionsthat (i) division planes were central and alternated by 90° and(ii) murein synthesis would take place exclusively at the divisionfurrow to generate two new hemispherical half-sacculi (Fig. 5A),cells that had gone through one division during the chase periodshould have sacculi consisting of sharply delimited labeled andunlabeled halves. Likewise, sacculi from cells that have dividedtwice after removal of D-Cys should consist of a 90° sector oflabeled murein and a 270° sector of all-new murein. Sacculi withthe expected distributions of new and old murein were indeed frequentlyfound after appropriate chase times (Fig. 5), a result stronglysupporting bothassumptions.

To summarize, our segregation studies indicate that impairment of PPB2 or RodA function leads to inactivation of cylindricalsacculus extension and permanent activation of the septal mureinbiosynthetic system, which is normally activated for only partof each cellcycle.

	ACKNOWLEDGMENTS

This work was supported by grant PM97-0148 from the PGC, a grant from the CSIC-MPG bilateral cooperation program, and an institutionalgrant from Fundación Ramón Areces to M.A.D.P.

	FOOTNOTES

^* Corresponding author. Mailing address: Centro de Biología Molecular "Severo Ochoa," CSIC-UAM, Facultad de Ciencias UAM, Campusde Cantoblanco, 28049 Madrid, Spain. Phone: (34) 913978083. Fax:(34) 913978087. E-mail: madepedro{at}cbm.uam.es.

This paper is dedicated to J. de la Rosa for the many years of hard work that she has dedicated to our group at Centro deBiología Molecular "SeveroOchoa."

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Addinall, S. G., and J. Lutkenhaus. 1996. FtsZ-spirals and -arcs determine the shape of the invaginating septa in some mutants of Escherichia coli. Mol. Microbiol. 22:231-237[CrossRef][Medline].
2.	Ayala, J. A., T. Garrido, M. A. de Pedro, and M. Vicente. 1994. Molecular biology of bacterial septation, p. 73-101. In J. M. Ghuysen, and R. Hakenbeck (ed.), Bacterial cell wall. Elsevier, Amsterdam, The Netherlands.
3.	Begg, K. J., and W. D. Donachie. 1985. Cell shape and division in Escherichia coli: experiments with shape and division mutants. J. Bacteriol. 163:615-622[Abstract/Free Full Text].
4.	Begg, K. J., and W. D. Donachie. 1998. Division planes alternate in spherical cells of Escherichia coli. J. Bacteriol. 180:2564-2567[Abstract/Free Full Text].
5.	Begg, K. J., B. G. Spratt, and W. D. Donachie. 1986. Interaction between membrane proteins PBP3 and RodA is required for normal cell shape and division in Escherichia coli. J. Bacteriol. 167:1004-1008[Abstract/Free Full Text].
6.	Begg, K. J., A. Takasuga, D. H. Edwards, S. J. Dewar, B. G. Spratt, H. Adachi, T. Ohta, H. Matsuzawa, and W. D. Donachie. 1990. The balance between different peptidoglycan precursors determines whether Escherichia coli cells will elongate or divide. J. Bacteriol. 172:6697-6703[Abstract/Free Full Text].
7.	Bi, E. F., and J. Lutkenhaus. 1991. FtsZ ring structure associated with division in Escherichia coli. Nature 354:161-164[CrossRef][Medline].
8.	Botta, G. A., and J. T. Park. 1981. Evidence for involvement of penicillin-binding protein 3 in murein synthesis during septation but not during cell elongation. J. Bacteriol. 145:333-340[Abstract/Free Full Text].
9.	Boyle, D. S., M. M. Khattar, S. G. Addinall, J. Lutkenhaus, and W. D. Donachie. 1997. ftsW is an essential cell-division gene in Escherichia coli. Mol. Microbiol. 24:1263-1273[CrossRef][Medline].
10.	Burman, L. G., J. Raichler, and J. T. Park. 1983. Evidence for diffuse growth of the cylindrical portion of the Escherichia coli murein sacculus. J. Bacteriol. 155:983-988[Abstract/Free Full Text].
11.	Canepari, P., G. Botta, and G. Satta. 1984. Inhibition of lateral wall elongation by mecillinam stimulates cell division in certain cell division conditional mutants of Escherichia coli. J. Bacteriol. 157:130-133[Abstract/Free Full Text].
12.	Canepari, P., C. F. Di Stefano, M. M. Lleo, and G. Satta. 1993. Peptidoglycan synthesis and its fine chemical composition in dividing and not dividing Klebsiella pneumoniae cocci. New Microbiol. 16:165-170[Medline].
13.	Canepari, P., C. Signoretto, M. Boaretti, and L. Del Mar. 1997. Cell elongation and septation are two mutually exclusive processes in Escherichia coli. Arch. Microbiol. 168:152-159[CrossRef][Medline].
14.	Cooper, S. 1991. Bacterial growth and division. Academic Press, Inc., San Diego, Calif.
15.	Denome, S. A., P. K. Elf, T. A. Henderson, D. E. Nelson, and K. D. Young. 1999. Escherichia coli mutants lacking all possible combinations of eight penicillin binding proteins: viability, characteristics, and implications for peptidoglycan synthesis. J. Bacteriol. 181:3981-3993[Abstract/Free Full Text].
16.	de Pedro, M. A., J. C. Quintela, J.-V. Höltje, and H. Schwarz. 1997. Murein segregation in Escherichia coli. J. Bacteriol. 179:2823-2834[Abstract/Free Full Text].
17.	Donachie, W. D. 1968. Relationship between cell size and time of initiation of DNA replication. Nature 219:1077-1079[CrossRef][Medline].
18.	Donachie, W. D. 1993. The cell cycle of Escherichia coli. Annu. Rev. Microbiol. 47:199-230[Medline].
19.	Donachie, W. D., S. Addinall, and K. Begg. 1995. Cell shape and chromosome partition in prokaryotes, or why E. coli is rod-shaped and haploid. Bioessays 17:569-576[CrossRef][Medline].
20.	Donachie, W. D., K. J. Begg, and M. Vicente. 1976. Cell length, cell growth and cell division. Nature 264:328-333[CrossRef][Medline].
21.	Garcia del Portillo, F., and M. A. de Pedro. 1991. Penicillin-binding protein 2 is essential for the integrity of growing cells of Escherichia coli ponB strains. J. Bacteriol. 173:4530-4532[Abstract/Free Full Text].
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