Visualization of Penicillin-Binding Proteins during Sporulation of Streptomyces griseus

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J Bacteriol, April 1998, p. 2125-2132, Vol. 180, No. 8
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Visualization of Penicillin-Binding Proteins during Sporulation of Streptomyces griseus

Jiang Hao and Kathleen E. Kendrick^*

Department of Microbiology, Ohio State University, Columbus, Ohio 43210

Received 10 November 1997/Accepted 2 February 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

We used fluorescein-tagged $beta$ -lactam antibiotics to visualize penicillin-binding proteins (PBPs) in sporulating cultures ofStreptomyces griseus. Six PBPs were identified in membranes preparedfrom growing and sporulating cultures. The binding activity ofan 85-kDa PBP increased fourfold by 10 to 12 h of sporulation,at which time the sporulation septa were formed. Cefoxitin inhibitedthe interaction of the fluorescein-tagged antibiotics with the85-kDa PBP and also prevented septum formation during sporulationbut not during vegetative growth. The 85-kDa PBP, which was thepredominant PBP in membranes of cells that were undergoing septation,preferentially bound fluorescein-6-aminopenicillanic acid (Flu-APA).Fluorescence microscopy showed that the sporulation septa werespecifically labeled by Flu-APA; this interaction was blockedby prior exposure of the cells to cefoxitin at a concentrationthat interfered with septation. We hypothesize that the 85-kDaPBP is involved in septum formation during sporulation of S. griseus.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Sporulation of Streptomyces species is characterized by the formation of chains of uninucleoidal, unicellular spores by growthfrom multinucleoidal, branched, filamentous cells. Two distinctivefeatures of streptomycete sporulation are its reproductive natureand the requirement for extensive growth during differentiation.Cytological events during sporulation include the growth of specializedfilaments, termed aerial (5) or sporogenic (23) hyphae, whichare the sites of spore formation; partitioning of copies of thechromosome in these hyphae; massive and relatively synchronousseptation to form the spore compartments; and maturation of thespores by thickening of the walls and rounding up of the sporecompartments.

The conversion of specialized, reproductive hyphae into chains of spores implicates peptidoglycan synthesis as an importantpathway that is likely to respond to temporal and spatial regulatorysignals. Penicillin-binding proteins (PBPs) catalyze the terminalsteps in the synthesis of peptidoglycan and are targets of inhibitionby $beta$ -lactam antibiotics. Two major classes of PBPs have been described(10): low-molecular-weight PBPs that have carboxypeptidase andtranspeptidase activities in vitro and are typically responsiblefor cleaving the terminal D-Ala from pentapeptide chains of nascentpeptidoglycan, and high-molecular-weight PBPs that form the cross-linksbetween neighboring peptide side chains. Within the latter classare two subgroups. The bifunctional class A PBPs act as both transpeptidasesand transglycosylases (10), whereas the class B PBPs containa transpeptidase domain and at least one additional "module" ofcontroversial function. Ishino and Matsuhashi (17) have suggestedthat the class B PBPs have transglycosylase activity mediatedby the N-terminal domain, but a recent study (12) suggests thatthe N-terminal domain may act as an intramolecular chaperone toassist in folding the C-terminal transpeptidase module. Most,if not all, of the low-molecular-weight PBPs are not essentialfor cell growth under standard laboratory conditions (41). Someof the high-molecular-weight PBPs are at least somewhat redundant(32, 40, 42), whereas others appear to be essential (25,41).

The essential PBPs include those required for septum formation during cell division. In only three bacteria is there convincingevidence of the identity of the septum-specific PBP. In Escherichiacoli, FtsI (PBP3) is necessary for septation (37) and may alsobe required for assembly of the septation site (32). Certain $beta$ -lactam antibiotics preferentially inhibit the activity of FtsI(37). C-terminal truncation of PBP2B, the homolog of FtsI inBacillus subtilis, leads to filamentation; this protein appearsto be required for septum formation during vegetative growth (41).Two FtsI homologs have been identified in Pseudomonas aeruginosa.One of these, PBP3, is encoded by a gene that lies within thecell division cluster and is depleted in the stationary phase;the other, PBP3x, is not essential and accumulates during thestationary phase (25, 26).

Although phylogenetic (21) and structural (11, 18, 19, 36) studies have led researchers to propose that streptomycetePBPs may be the progenitors of the serine $beta$ -lactamases that inactivate $beta$ -lactam antibiotics, little work has been published on the physiologicalfunction of PBPs from these bacteria. Early studies of Streptomycessp. strain R61 demonstrated that $beta$ -lactam antibiotics that inhibitedtranspeptidation in membrane preparations also prevented germinationof spores or growth (7). Other researchers have surveyed thePBPs of several Streptomyces species and noted relationships betweensome PBPs and the growth phase (16, 28). Several PBPs wereidentified in vegetative cells and mature spores of Streptomycesgriseus, but none were correlated with a specific function (1).The physiological role of one streptomycete PBP has been suggestedby the work of Paradkar et al. (31), who showed that pcbR, withinthe cephamycin biosynthetic gene cluster of Streptomyces clavuligerus,could be disrupted in a non-cephamycin-producing mutant but notin the producing parent strain. Disruption of the pcbR gene ledto twofold-less resistance to $beta$ -lactam antibiotics, and immunologicalanalysis showed that synthesis of PcbR, a PBP of 57 kDa, was increasedduring the antibiotic production phase. The authors suggestedthat PcbR was a low-affinity PBP that augmented resistance to $beta$ -lactam antibiotics in the $beta$ -lactam-producing strain. The roleof this PBP in peptidoglycan synthesis remains to be determined.

Because streptomycete sporulation is marked by dramatic changes in cell shape, several PBPs are likely to be required duringthe life cycle. For example, distinct PBPs (or altered activitiesof existing PBPs) might be necessary for growth by apical extension(13, 27), branch formation during vegetative growth and atthe earliest stage of sporulation to generate sporogenic hyphae,septum formation during growth and differentiation, and sporematuration. Since sporulation and vegetative septa have distinctfates, it is conceivable that different PBPs are responsible forseptation at these stages of the life cycle. To begin to understandthe roles of PBPs in the Streptomyces life cycle, we have usedfluorescence microscopy to visualize PBPs during sporulation andhave identified a likely candidate for a PBP involved in septationof S. griseus.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Media and growth of the organism. To determine the effect of $beta$ -lactam antibiotics on growth and sporulation, cultures were inoculated into sporulation medium(SpM) (20) by dilution (2 × 10⁴) from a primary culture grown in SpM for 2 to 5 days at 30°C.At this time the primary culture comprised mature spores. To inducesporulation by phosphate starvation, the primary culture was diluted(10² to 10³) into glucose-ammonia minimal medium containing 1% casein hydrolysate(HyCase SF; Sigma Chemical Co., St. Louis, Mo.) (20) and grownto an absorbance of 3, at which time phosphate was removed fromthe culture (20). The $beta$ -lactam antibiotics were added at thetime of transfer to the phosphate-free medium. The number of cellsthat had developed thick walls, which was used to approximatesporulation efficiency, was measured by determining the viablecount of cultures after exposure to ultrasound for 10 min (23).

Microscopy, photography, and image processing. Samples were prepared for fluorescence microscopy by combining 0.1 ml of culture with 100 µM fluorescein (Flu)-labeled $beta$ -lactamin a microcentrifuge tube and incubating the mixture for 20 minat 30°C. In some cases the cells were exposed to a $beta$ -lactam antibioticfor 20 min at 30°C prior to two washes with 1.5 ml of 0.85% NaCl(saline) and exposure to the Flu- $beta$ -lactam. Then the samples werewashed twice with 1.5 ml of saline and suspended in 0.1 ml ofsaline for microscopy. An identical sample of cells was combinedwith 5 µl of 1 mg of propidium iodide per ml and held at roomtemperature for 10 min. Cells were centrifuged and washed twicewith saline and then resuspended in 0.1 ml of saline. Sampleswere viewed with a Zeiss Axioskope microscope equipped for fluorescenceand phase-contrast photomicroscopy. To view the Flu label, a Fluisothiocyanate filter set was used, whereas a rhodamine filterset was used for viewing of propidium iodide-treated samples.Images were captured as TIFF files that were subsequently cropped,magnified, and adjusted in brightness and intensity with CorelPhoto Paint to resemble the viewed sample as closely as possible.For the dual fluorescent labels, the individual TIFF files weresuperimposed by using Corel Photo Paint. Each image was importedinto Corel Draw for labeling and printed with a Tektronix Phaser450 dye sublimation printer. Phase-contrast photomicrographs weremade by using Kodak TMax 400 film; then the prints were scannedand processed as described above.

For electron microscopy, 1.5 ml of culture was combined with 1.5 ml of 8% glutaraldehyde. The mixture was centrifuged, andthe cells were suspended in 1 ml of 4% glutaraldehyde in 0.1 Msodium cacodylate, pH 7.2, and held at 4°C overnight. Cells wereprocessed for thin sectioning as described by Kwak and Kendrick(23). Thin sections were viewed and photographed with a PhilipsCM12 transmission electron microscope. The prints were scannedand processed as described above.

Preparation of membranes. All membrane preparation steps were carried out at 4°C. The procedure of Buchanan and Ling (4) was used, with slight modifications.Fifty milliliters of culture was harvested by centrifugation,washed once in 50 mM Tris-HCl (pH 7.5) containing 1 M KCl, suspendedin 1 ml of 50 mM Tris-HCl (pH 7.5)-1 mM phenylmethylsulfonyl fluoride,and disrupted by two passages through a French press at 18,000lb/in². After centrifugation at 20,000 × g for 30 min, the supernatantwas centrifuged at 100,000 × g for 1 h in a Beckman L8-M ultracentrifuge.The supernatant was discarded, the pelleted material was suspendedin 3 ml of extraction buffer, and centrifugation was repeated.The material in the pellet was dissolved in extraction bufferto a protein concentration of 10 to 20 mg/ml (8) and eitherused immediately or stored at $-$ 70°C.

For routine treatment with Flu- $beta$ -lactam conjugates, 100 µg of protein was combined with at least 50 µM Flu- $beta$ -lactam in a finalvolume of 12 µl. The mixture was incubated for 20 min at 30°C.This was sufficient Flu-6-aminopenicillanic acid (Flu-APA) andreaction time to achieve a concentration between 2.6- and 5-foldgreater than the K_d (as calculated from the experimental datashown in Fig. 7) for those PBPs that bound Flu-APA. The reactionwas stopped by addition of an equal volume of double-strengthsodium dodecyl sulfate-polyacrylamide gel electrophoresis samplebuffer (24), and the reaction mixture was boiled for 5 min andapplied to a sodium dodecyl sulfate-polyacrylamide gel (24).After electrophoresis, the gel was viewed with a Molecular DynamicsStorm imaging device. The relative levels of PBPs were measuredby using the quantitation software provided by the manufacturer.This imaging system detects emissions centered at 560 nm and thereforecannot detect very low levels of Flu-tagged PBPs. To confirm thatwe were able to detect all of the Flu-tagged PBPs by this method,we employed Western immunoblot analysis with anti-Flu antibodiesconjugated to alkaline phosphatase and detected proteins boundto Flu-tagged 7-aminocephalosporanic acid (Flu-ACA) or Flu-APAby using a chemiluminescent substrate according to the manufacturer'sinstructions (Vistra ECF; Amersham, Buckinghamshire, United Kingdom).This method, which amplified the Flu signal and permitted detectionby chemiluminescence at 560 nm, showed no additional PBPs in oursample. Since the direct detection of Flu-tagged PBPs gave betterresolution and was more rapid than the Western immunoblot approach,we used the former method for routine analysis.

To label the cells with Flu-APA prior to denaturing gel electrophoresis, 100 µM Flu-APA was added to an induced culture andincubation was continued for 15 min. The reaction was quenchedby adding 1,000-fold excess APA, and the cells were processedas described above.

Synthesis of Flu-ACA and Flu-APA. Flu conjugates of APA and ACA were prepared by the method of Galleni and coworkers (9), as modified by Popham and Setlow(34). When the mixed isomer of Flu was used, the conjugateswere purified by thin-layer chromatography on silica gel G (Whatman)in 80% (vol/vol) acetonitrile in water and detected by fluorescence.The regions of the silica gel that contained the fluorescent conjugates,both of which migrated with an R_f of 0.72, were scraped from theplate into 1.5-ml microcentrifuge tubes, combined with 400 µlof water, and centrifuged at 15,000 rpm for 2 min. The supernatantwas transferred to a new tube and centrifuged for 5 min. The supernatantwas collected, dried in a vacuum centrifuge (Savant, Farmingdale,N.Y.) at room temperature, and dissolved in 50 µl of 50 mM Tris-HCl,pH 7.5. This solution was stored at $-$ 20°C in the dark and wasstable for at least 1 month. The concentration of conjugate wasestimated by measuring its absorbance at 494 nm, assuming thatthe extinction coefficient of the conjugate was identical to thatof Flu ( $varepsilon$ ₄₉₄ = 71,000 cm¹ M¹).

To confirm their identities, 20 ng of each purified sample was analyzed by negative ion electrospray mass spectrometry witha Perkin-Elmer Sciex API-300 mass spectrometer. The preparationof Flu-APA had an average mass of 688.2 ± 1.7 (expected valueof 688.0), and that of Flu-ACA had a mass of 743.0 (expected valueof 743.9). The reaction mixture was also tested for antibioticactivity by bioautography of the thin-layer chromatogram. Sufficientsoft Luria-Bertani agar containing either E. coli (ATCC 25922)or Staphylococcus aureus (ATCC 29213) to cover the surface ofthe thin-layer plate was overlaid, and the plate was incubatedovernight at 37°C. APA (R_f = 0.30), ACA (R_f <0.05), and Flu-APAdid not inhibit either indicator organism, but S. aureus was sensitiveto Flu-ACA. No other fluorescent spots inhibited growth of eitherorganism.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Effects of $beta$ -lactam antibiotics on growth and sporulation. To identify PBPs that were required for morphogenesis of S. griseus, we first surveyed several $beta$ -lactam antibiotics for theireffects on vegetative growth and sporulation. Cultures of thewild-type strain, S. griseus NRRL B-2682, that were growing exponentiallyin SpM (20) were exposed to 50 µg of $beta$ -lactam antibiotic perml when they reached an A₅₀₀ of 1.0 to 1.1. In this medium, theuntreated wild-type strain grew with a doubling time of 1.5 to1.75 h, entered the transition to stationary phase at an A₅₀₀of approximately 5 to 6 (Fig. 1), and formed chains of spores10 h later. Cultures were monitored for growth, cell morphology,and the development of resistance to sonication that occurs whenthe spore compartments acquire thick walls. This normally happensshortly after the completion of septation (23).

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FIG. 1. Effect of $beta$ -lactam antibiotics on growth. S. griseus NRRL B-2682, growing exponentially in SpM (A₅₀₀ = 1), was subdivided into four cultures and left untreated (×) or exposed to 50 µg of cefoxitin ( $black-triangle$ ), cefotaxime ( $bullet$ ), or penicillin V ( $open circle$ ) per ml. The arrow indicates the time at which sporogenic hyphae were evident, and the arrowhead shows when free spores were first visible.

Four penicillins (penicillin V, carbenicillin, benzylpenicillin, and ampicillin) affected the cells during vegetative growth,but the effect was most pronounced with penicillin V. After theaddition of penicillin V, the culture underwent an additionaldoubling before the mycelia formed clumps. Dispersed growth resumed8 h later (Fig. 1) and culminated in the production of sporesto the same extent as the untreated culture.

Among nine cephalosporins and their precursor, ACA, seven had no visible effect on vegetative growth or sporulation, whereascefoxitin, cephalosporin C, and cefotaxime prevented completesporulation without significantly affecting vegetative growth(Fig. 1). The magnitude of inhibition of spore formation was assessedby measuring the development of sonication-resistant units atconcentrations of each drug up to 100 µg/ml. Cefoxitin had themost dramatic effect (Fig. 2), inhibiting complete maturationof the spores at 6 µg/ml, reducing spore formation at 24 µg/ml,and reducing the total viability by 4 orders of magnitude at 100µg/ml. Cefotaxime inhibited spore formation by 60% at 1 µg/ml;the extent of inhibition increased to 80% at 50 µg/ml. ACA showedlittle effect until the concentration exceeded 24 µg/ml (Fig.2). The complex pattern of inhibition by cefoxitin (and perhapsalso cefotaxime) suggests that this drug had more than one targetin sporulating cells.

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FIG. 2. Dose-response curve for inhibition of sporulation by $beta$ -lactam antibiotics. An exponentially growing culture of S. griseus (A₅₀₀ = 1) in SpM was divided into 3-ml aliquots that were placed in 18- by 150-mm culture tubes containing the indicated concentration of cefoxitin ( $bullet$ ), cefotaxime ( $open circle$ ), or ACA (×). After incubation for an additional 4 days, the cultures were treated with ultrasound, diluted, and plated for viability. The values (in sonication-resistant units [sru] per ml) are averages ± standard deviations of duplicate experiments, each assayed in duplicate. The concentration of sonication-resistant units for each antibiotic at 0.6 µg/ml was identical to that of an untreated culture.

When spores were plated on SpM agar that contained 50 µg of cefoxitin per ml, colonies formed with an efficiency equal tothat of spores plated in the absence of the drug and producedaerial hyphae but did not sporulate. Likewise, spores inoculatedinto liquid SpM initiated growth with equal efficiency in thepresence or absence of 24 µg of cefoxitin per ml. At this concentration,cefoxitin altered the morphology of cells only after their entryinto the transition phase: the hyphae in cultures treated withcefoxitin from 6 to 50 µg/ml showed bulges, adjacent to the growingtips, that were more prevalent at the higher concentrations ofcefoxitin. Only rarely was there more than one bulge per filament.Bulges first appeared in the treated cultures at the same time(20 h) that the control culture was beginning to form sporogenichyphae. As incubation continued, the distance between the bulgeand the tip increased (Fig. 3).

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FIG. 3. Formation of bulges by S. griseus exposed to 50 µg of cefoxitin per ml. A culture of S. griseus that had been grown as described in the legend to Fig. 1 was left untreated (A) or treated with 50 µg of cefoxitin per ml (B), and incubation was continued for 10 h. The swollen tips of branches in panel A are sporogenic hyphae; the bulges are evident in panel B. Bar, 10 µm.

Sporulation was also blocked by cefoxitin and cefotaxime when the drugs were added to cultures of S. griseus that had beeninduced to sporulate by phosphate starvation. Electron microscopicexamination of sporulating cultures that had been exposed to cefoxitinduring 12 h of induction confirmed that this antibiotic inhibitedseptation. At 50 µg/ml, cefoxitin completely prevented progressionof septation past the initial stage (Fig. 4D). An electron-denselayer that was continuous with the peptidoglycan in the hyphalwall was evident within the regularly spaced, small septal invaginations.Cefoxitin at 6 µg/ml interfered with but did not prevent septation.The septa in this case were rather diffuse and irregularly shaped,but the spore walls still underwent thickening (Fig. 4E), andthe rectangular cells were resistant to ultrasound. The effectof cefoxitin was specific to sporulation since vegetative hyphaecontained apparently normal septa (Fig. 4C). Cefotaxime at 12µg/ml permitted complete septation (Fig. 4F), but the septa wereirregularly shaped and the thick-walled spore compartments didnot separate into individual cells even after prolonged incubation(4 days) or treatment with ultrasound.

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FIG. 4. Effects of cefoxitin and cefotaxime on septation. Cultures of S. griseus were grown vegetatively (C) or induced to sporulate by phosphate starvation (A, B, and D to F) for 10 or 12 h in the presence or absence of the indicated $beta$ -lactam antibiotic. (A) Untreated culture at 10 h of starvation. (B) Untreated culture at 12 h of starvation. (C) Culture treated with 50 µg of cefoxitin per ml in vegetative growth. (D) Culture treated with 50 µg of cefoxitin per ml after phosphate starvation for 12 h. (E) Culture treated with 6 µg of cefoxitin per ml for 12 h. (F) Culture treated with 20 µg of cefotaxime per ml for 12 h. Arrowheads indicate sporulation septa. VS, vegetative septum. Bar, 0.5 µm.

Visualization of binding in situ. Because massive, synchronous septation occurs in the sporogenic hyphae at 10 h of sporulation of S. griseus when induced byphosphate starvation (Fig. 4) (23), we reasoned that the PBP(s)required for septation may be present at a relatively high concentrationin the sporogenic hyphae at this time. We examined sporulatingcultures by fluorescence microscopy to determine whether the Flu-conjugated $beta$ -lactam antibiotics Flu-APA and Flu-ACA could be visualized uponinteraction with their target PBPs. During vegetative growth therewas substantial autofluorescence, but no localization of eitherFlu-APA or Flu-ACA was evident. Early in sporulation, neitherFlu- $beta$ -lactam bound noticeably to the cells. At 10 h of sporulation,Flu-APA bound to sites distributed at regular intervals throughthe sporogenic hyphae (data not shown). Most of these zones offluorescence did not completely transect individual sporogenichyphae. Since electron microscopic observations had shown thatthe majority of the septa were still forming at this time (Fig.4), these zones may correspond to nascent septa. Flu-tagged "ladders"were evident at 12 h (Fig. 5A and G), shortly after the completionof septation (23). The "rungs" of these ladders lay betweenthe nucleoids, consistent with their localization to the sporulationsepta (Fig. 5A). Inspection of the same sample by phase-contrastmicroscopy showed the sporulation septa as thin, dark bands atintervals within the swollen sporogenic hyphae (Fig. 5B); thesebands coincided with the zones stained by Flu-APA. This samplealso showed that spore-bearing hyphae formed not only by growthfrom new branches (23) but also by extension from existing hyphaltips (Fig. 5B). By examining this and other samples, we estimatedthat hyphal regions undergoing septation comprised no more than25% of the biomass at 12 h of induction. Although Flu-APA localizedonly at septation sites, Flu-ACA bound to both the sites of septationand the walls of the sporogenic hyphae (Fig. 5C). When cells weretreated with 6 µg of cefoxitin per ml during induction, subsequentbinding of Flu-APA and Flu-ACA to the septa was blocked (cf. Fig.5C and D and Fig. 5G and H). A higher concentration of cefoxitinwas required to prevent binding of Flu-ACA to the hyphal walls(cf. Fig. 5C to F).

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FIG. 5. Visualization of PBPs by fluorescence microscopy. Cells of S. griseus that had been induced to sporulate for 12 h in the presence or absence of cefoxitin were exposed to Flu-conjugated $beta$ -lactams. (A) Flu-APA and propidium iodide. (B) Phase-contrast micrograph of the sample shown in panel A. (C) Flu-ACA. (D) Cefoxitin (6 µg/ml), then Flu-ACA. (E) Cefoxitin (20 µg/ml), then Flu-ACA. (F) Cefoxitin (60 µg/ml), then Flu-ACA. (G) Flu-APA. (H) Cefoxitin (6 µg/ml), then Flu-APA. Arrowheads in panels A, C, and G point to examples of Flu-tagged "ladders" in sporogenic hyphae. Arrowheads in panel B point to sporulation septa. The arrows marked "N" in panel A point to nucleoids stained with propidium iodide; in panel B, those marked "Br" point to sporogenic hyphae that emerged from new branches and those marked "E" point to sporogenic hyphae that formed by extension of preexisting vegetative hyphae. The arrows marked "W" in panel C point to Flu-ACA-labeled hyphal walls. Bar, 2 µm. The color version of this figure can be viewed at http://www.biosci.ohio-state.edu/~kek/html/j_bacteriol_1998.html.

Identification of PBPs in membrane preparations. The formation of abundant septa at 10 h of sporulation of S. griseus would be expected to require an increase in the activityof septum-specific PBPs. Moreover, the specificity of Flu-APAfor the sporulation septa suggested that biochemical studies withthis reagent might permit us to identify a septum-specific PBP.Incubation of Flu-APA with membrane preparations from vegetativeand sporulating cultures of S. griseus revealed three PBPs, allof relatively high molecular weights. The largest of these (140kDa) decreased at least threefold in intensity, ultimately toa barely detectable level, during the first 12 h of sporulation(Fig. 6). An 85-kDa PBP that was present during vegetative growthincreased 1.5-fold during the first 4 h of sporulation, at whichtime the sporogenic hyphae had begun to form (23). By 10 h,the 85-kDa PBP signal had increased threefold, coincident withthe onset of septum formation. At 12 h, when complete septa wereevident, the amount of signal was approximately fourfold greaterthan that during vegetative growth (Fig. 6). The third PBP (66kDa) was present at a low level during growth and sporulation.In addition to these three high-molecular-weight PBPs, three lower-molecular-weightPBPs were faintly evident when membranes were treated with Flu-ACA.One (60 kDa) was detectable only in membranes from sporulatingcells (Fig. 6). We classified these proteins as PBPs because thebands were absent from membranes that were not exposed to Flu-ACA(in contrast to 75- and 30-kDa autofluorescent proteins), theydisappeared entirely when the membranes were incubated with 50µg of cefoxitin per ml followed by Flu-ACA, and they were alsodetectable by immunoblot with anti-Flu antibodies.

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FIG. 6. Identification of PBPs after denaturing polyacrylamide gel electrophoresis. PBPs were labeled with Flu-ACA or Flu-APA in membranes prepared from vegetative hyphae (Veg) or cells induced to sporulate for 4, 10, or 12 h prior to separation of proteins by denaturing gel electrophoresis. Cells induced to sporulate for 10 h were treated with 100 µM Flu-APA, and then membranes were prepared and proteins were separated as described above. Arrowheads point to PBPs of the indicated molecular masses (in kilodaltons). In the absence of treatment with either Flu- $beta$ -lactam, membrane preparations showed two inherently fluorescent proteins of 75 and 30 kDa.

The affinity of Flu-APA for the 85-kDa PBP was also evident after labeling the cells at 10 h of sporulation and examinationof the PBPs in membrane samples (Fig. 6). The pattern of labelingwas similar to that seen in vitro, with the 85-kDa PBP predominatingunder these conditions. Titration of the PBPs by the additionin vitro of increasing concentrations of Flu-APA confirmed thatthe 85-kDa PBP preferentially bound Flu-APA, followed by the 66-and 140-kDa PBPs (Fig. 7). Binding of the 85-kDa PBP to Flu-APAin vivo was inhibited approximately 90% by 6 µg of cefoxitin perml (data not shown).

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FIG. 7. Preferential interaction of Flu-APA with the 85-kDa PBP. Increasing concentrations of Flu-APA were incubated for 15 min with a membrane preparation from a culture of S. griseus that had entered stationary phase (A₅₀₀ = 12) in glucose-ammonia minimal medium supplemented with 1% casein hydrolysate. (Membranes prepared from this culture contained relatively high amounts of the 66- and 140-kDa PBPs, which permitted more accurate quantitation of their levels.) Band intensities were measured as described in Materials and Methods, the background was subtracted, and the results were fit to a hyperbolic curve (one binding site) by using Prism 2.01 (GraphPad, San Diego, Calif.). By this analysis, the relative K_d of the 85-kDa PBP (×) was 2.3- and 2.7-fold lower than that of the 66 ( $open circle$ )- and 140 ( $bullet$ )-kDa PBPs, respectively; the coefficients of determination (r²), which indicate the fit of the data to the equation, were 0.9694 (66-kDa PBP), 0.9892 (85-kDa PBP), and 0.9602 (140-kDa PBP).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The technique of detection of PBPs by coupling $beta$ -lactam antibiotics to Flu was developed by Galleni and colleagues (9).We have applied this technique to the visualization of streptomycetePBPs in situ. The success of this method may reflect the relativeabundance of certain PBPs during sporulation, when the demandfor septation proteins and enzymes required for spore wall thickeningis expected to be high. Since the stoichiometry between a PBPand its bound Flu- $beta$ -lactam is 1, no signal amplification occursin this system. The visualization of the signal most likely dependson an abundant or highly localized target protein. This methodis therefore probably less sensitive than immunofluorescence microscopy,which detected FtsI at an estimated 100 molecules per cell whenthe protein localized to the midcell (39).

It is noteworthy that Flu-ACA revealed several more PBPs than did Flu-APA. Although we do not know whether Flu-ACA revealsthe full complement of PBPs expressed in S. griseus under theconditions of this study, our results demonstrate the importanceof using more than one labeled $beta$ -lactam compound to detect PBPs.

Our previous studies (23) showed that sporogenic hyphae developed by growth from newly formed branches after induction ofsporulation. Here we have extended this observation, noting thatthe sporogenic hyphae also grew from existing tips of vegetativehyphae. It is not known whether the same occurs during the formationof aerial hyphae during sporulation on a solid surface. The sporogenichyphae that formed by extension of vegetative hyphae were longerand, upon subdivision, generated more spores than those that formedat new branch points. At 12 h of induction, two subpopulationsof cells existed in this culture: old vegetative hyphae and newlyformed sporogenic hyphae, approximately 50% of which were undergoingseptation.

The inhibitory effect of cefoxitin on sporulation of S. griseus was complex. Electron micrographs showed that septum formationprogressed through the earliest stage but no further in the presenceof 50 µg of cefoxitin per ml. Phase-contrast microscopy demonstratedthat this effect was caused by cefoxitin in excess of 20 µg/ml;lower concentrations of cefoxitin resulted in complete but deformedsepta, perhaps because the target PBP was incompletely inhibited.The presence of a layer of peptidoglycan within the small septalingrowth evident in the culture treated with 50 µg of cefoxitinper ml indicated that the inhibited PBP was not necessary to effectthe change in direction of peptidoglycan growth. The peptidoglycanwithin these invaginations is therefore presumably synthesizedeither by a mechanism that does not require the transpeptidaseactivity of the septum-specific PBP or by an additional PBP thatis relatively insensitive to cefoxitin. This result is consistentwith radiolabeling studies with E. coli that suggested that FtsIis responsible for the centripetal extension of peptidoglycanduring septation but not the initiation of septation (29, 40).

Comparison of the in vivo and in vitro effects of cefoxitin showed that a concentration of 6 µg/ml was sufficient to abrogatefluorescence at the septum but not the hyphal walls. This concentrationresulted in greater than 90% inhibition of the 85-kDa PBP andvisibly altered the ultrastructure of the sporulation septa. Evenat 6 µg of cefoxitin per ml, however, the spores still had thickwalls sufficient to withstand sonication. The absence of a strictcorrelation between the concentration of cefoxitin required toblock binding of Flu-APA and that required for a morphologicaleffect is probably a consequence of the rather insensitive methods(electron microscopy and development of resistance to sonication)that are available to assess structural changes during sporulation.

We cannot yet explain the bulges that formed after exposure to cefoxitin during growth. These bulges resembled those describedby several researchers for E. coli cells in which the activityof FtsL (14) or FtsI (the latter in conjunction with PBP2 [2],RodA [3], or soluble lytic transglycosylase [38]) was inhibited.In all of these cases the formation of bulges correlated withthe inhibition of septation. Although comparisons with the resultsfor E. coli would suggest that the bulges in S. griseus markedsites of aborted septation, phase-contrast microscopic examinationsuggested that this was not the case; bands resembling septa wereevident, sometimes traversing the bulge but more commonly immediatelyproximal or distal to the bulge. Moreover, the bulges formed atthe growing tips, which are unlikely to be undergoing vegetativeseptation (22). Bulges always formed during the transition betweenvegetative growth and sporulation in cultures that were growingin sporulation medium, even though cefoxitin had been presentsince inoculation. This observation suggests that there is somethingunique about the hyphal tips at this stage of the life cycle.Since the control culture was beginning to form sporogenic hyphaeat the time that the bulges first appeared, it is conceivablethat these bulges mark the junctions between the preexisting vegetativehyphae and the nascent sporogenic hyphae.

We might reasonably expect that the presence of a $beta$ -lactam antibiotic that targets a septum-specific PBP would slow vegetativegrowth, yet this was not observed. Cultures grew with essentiallyidentical rates (µ = 0.4 ± 0.07 h¹) at concentrations of cefoxitin as high as 24 µg/ml. Microscopicobservations confirmed that septa were present in vegetative hyphaeof a culture growing in the presence of 50 µg of cefoxitin perml. These results suggest that the septum-specific PBP that isthe target of cefoxitin during sporulation either is not accessibleto cefoxitin or is not required for septation during vegetativegrowth. This observation supports the possibility that distinctPBPs are responsible for septation during vegetative growth andsporulation.

The simplest hypothesis to explain our results is that the 85-kDa PBP is involved in septation during sporulation of S. griseus.This PBP showed the greatest affinity for Flu-APA in vitro andwas prominent in membranes from sporulating cells that had beenexposed to Flu-APA in vivo. Flu-APA bound specifically to thesites of sporulation septation, and this binding was inhibitedby cefoxitin at a concentration that interfered with septation.Like the septum-specific PBPs in other bacteria (10, 25, 41),the 85-kDa PBP has a high molecular weight. Nevertheless, theremay be additional PBPs involved in septation. For example, theelectron micrographs suggest that a cefoxitin-insensitive peptidoglycan-synthesizingenzyme deposits the material within the invaginations that markthe earliest stage of septum formation.

At this time we cannot determine whether the 85-kDa PBP band represents one or multiple PBP species. The intensity of fluorescenceof this protein band increased three- to fourfold during the first12 h of sporulation; this may be a consequence of either the enhancedproduction of a single PBP during sporulation or the productionof one 85-kDa PBP during vegetative growth and the subsequentproduction of a different, sporulation-specific 85-kDa PBP. Thegood fit of our data to the single-site hyperbolic equation forbinding of Flu-APA to the 85-kDa PBP is consistent with a singleprotein species, yet we cannot readily explain the presence ofthis PBP during vegetative growth if it is required only duringsporulation. The absence of localized sites of fluorescence inhyphae during vegetative growth and early in morphogenesis maybe attributable to interference from autofluorescence, the relativerarity and asynchrony of vegetative septation, the absence ofthe target PBP in sufficient quantity, or the presence of thetarget PBP(s) in diffuse, unlocalized regions. In light of theresults of Pogliano et al. (32), who suggested that FtsI isrequired not only for synthesis of peptidoglycan at the septumbut also for assembly of the septation sites, one possibilityis that the 85-kDa PBP is required for synthesis of septa duringsporulation as well as placement or assembly of the septationsites during vegetative growth. Cefoxitin may inhibit the formerfunction but not the latter.

Why should a relatively small (three- to fourfold) increase in the binding of the 85-kDa PBP be sufficient to permit visualizationin situ? We suggest that the increased activity of this PBP maybe confined to the sporogenic hyphae. Since the regions of thesporogenic hyphae that are undergoing septation at 12 h of inductioncomprise roughly 20 to 25% of the biomass of this culture, theamount of 85-kDa PBP in this location would actually have increased12- to 20-fold. Once the structural gene for the 85-kDa PBP isisolated, we will be able to determine whether its expressionor activity is spatially regulated, as our hypothesis would predict.

We consider it unlikely that a different PBP, undetectable by our methods, is solely responsible for septum formation, becausethe visible interaction between the sporulation septa and Flu-APAsuggests that the reactive PBP(s) should be relatively abundantand readily bind Flu-APA in vivo and in vitro. At the time ofseptation, the 85-kDa PBP was the predominant PBP labeled by Flu-APAin vivo. We cannot yet rule out the possibility that the 66-kDaPBP is also involved in septation, but its very low level at thetime when sporogenic hyphae were undergoing septation and itssomewhat lower affinity for Flu-APA argue against this possibility.Despite the physiological evidence suggesting that the 85-kDaPBP is involved in septation during sporulation, the definitivetest of our hypothesis requires disruption of its structural gene.Current work is directed toward this goal.

In keeping with the various morphologies assumed by streptomycetes during their complex life cycle, the synthesis of peptidoglycanin these organisms appears to be complex, differing in fundamentalways in vegetative growth, upon entry into the transition phase,and during sporulation. The nature of submerged sporulation byS. griseus dictates that any $beta$ -lactam antibiotic that inhibitedonly septation during spore formation would exert a relativelysmall effect on the development of sonication-resistant structures.This is because in our system the sporogenic hyphae typicallysubdivide into chains of 5 to 20 spores. Related work in our laboratoryindicates that the septum near the base of each sporogenic hyphaand the thick spore walls form even when sporulation septationis prevented (6, 15). From these preliminary results andthe observations presented in this paper, we would expect thatthe absence of sporulation septation would result in a decreasein sonication-resistant units of approximately 1 order of magnitude.This effect is clearly illustrated by our results with cefotaxime.The spore compartments formed but did not separate in culturesexposed to cefotaxime, even after treatment with ultrasound. Becausethe septa in this case were deformed, it is likely that a changein the structure of peptidoglycan in these septa led to a formthat was refractory to subsequent hydrolysis. This proposed actionis consistent with the results of the dose response experiment,which showed that cefotaxime at 50 µg/ml reduced the proportionof sonication-resistant units to approximately 20% of that ofthe untreated culture. Microscopic observations showed that thesonication-resistant units in this culture corresponded to sporechains, comprising 5 to 10 spore compartments, that failed toseparate into individual spores.

To our knowledge, the 140-kDa PBP is considerably larger than others that have been identified in unicellular gram-positiveand gram-negative bacteria. The largest reported to date appearsto be PBP1a of Caulobacter crescentus (30), which has a molecularmass of 130 kDa on the basis of its migration on a denaturingpolyacrylamide gel. The next largest is PBP1 of B. subtilis, whichis approximately 100 kDa on the basis of its amino acid sequencebut migrates on a denaturing polyacrylamide gel as if it wereabout 110 kDa (33). Like S. griseus, other streptomycetes alsocontain PBPs having apparent molecular masses in excess of 120kDa (16, 28). The dramatic decrease in the 140-kDa signalduring the early stages of sporulation implies not only that thisPBP is not involved in spore septation or maturation in S. griseusbut also that the structure of the peptidoglycan differs in youngsporogenic and vegetative hyphae. Sporogenic hyphae, which beginto form from rapidly growing tips during the first 2 to 4 h ofsporulation and complete elongation by approximately 10 h, donot branch as they elongate prior to septation (23). In contrast,vegetative hyphae form branches, generating new growing tips andthereby maintaining exponential growth (13, 27, 35). Itis therefore tempting to speculate that the 140-kDa PBP is requiredfor branch formation. This function, necessary for growth of actinomycetesand perhaps also prosthecate bacteria, might require a PBP thatwould have no homolog in most unicellular bacteria.

	ACKNOWLEDGMENTS

This research was supported by grants from the National Science Foundation (MCB-9210743 and MCB-9632468).

We thank F. R. Tabita for use of the chemiluminescence imager, Scott Taylor and Kathy Wolken for assistance with fluorescenceand electron microscopy, and Tim Vojt for assistance with imageprocessing. David Popham, John Reeve, and Julie Schwedock providedhelpful comments.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, 484 West 12th Ave., Ohio State University, Columbus, OH43210. Phone: (614) 292-1440. Fax: (614) 292-9195 or (614) 292-8120.E-mail: kendrick.1{at}osu.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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1.	Barabás, J., G. Barabás, I. Szabó, M. Veemhuis, and W. Harder. 1988. Penicillin-binding proteins of protoplast and sporoplast membranes of Streptomyces griseus strains. Arch. Microbiol. 150:105-108.
2.	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].
3.	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].
4.	Buchanan, C. E., and M.-L. Ling. 1992. Isolation and sequence analysis of dacB, which encodes a sporulation-specific penicillin-binding protein in Bacillus subtilis. J. Bacteriol. 174:1717-1725[Abstract/Free Full Text].
5.	Chater, K. F. 1993. Genetics of differentiation in Streptomyces. Annu. Rev. Microbiol. 47:685-713[Medline].
6.	Dharmatilake, A. J. Unpublished results.
7.	Dusart, J., M. Leyh-Bouille, and J. M. Ghuysen. 1977. The peptidoglycan crosslinking enzyme system in Streptomyces strains R61, K15 and rimosus. Kinetic coefficients involved in the interactions of the membrane-bound transpeptidase with peptide substrates and $beta$ -lactam antibiotics. Eur. J. Biochem. 81:33-44[Medline].
8.	Ehresmann, B., P. Imbault, and J. H. Weil. 1973. Spectrophotometric determination of protein concentration in cell extracts containing tRNA's and rRNA's. Anal. Biochem. 54:454-463[Medline].
9.	Galleni, M., B. Lakaye, S. Lepage, M. Jamin, I. Thamm, B. Joris, and J.-M. Frère. 1993. A new, highly sensitive method for the detection and quantification of penicillin-binding proteins. Biochem. J. 291:19-21.
10.	Ghuysen, J.-M. 1991. Serine $beta$ -lactamases and penicillin-binding proteins. Annu. Rev. Microbiol. 45:37-67[Medline].
11.	Ghuysen, J.-M. 1994. Molecular structures of penicillin-binding proteins and $beta$ -lactamases. Trends Microbiol. 2:372-380[Medline].
12.	Goffin, C., C. Fraipont, J. Ayala, M. Terrak, M. Nguyen-Distèche, and J.-M. Ghuysen. 1996. The non-penicillin-binding module of the tripartite penicillin-binding protein 3 of Escherichia coli is required for folding and/or stability of the penicillin-binding module, and the membrane-anchoring module confers cell septation activity on the folded structure. J. Bacteriol. 178:5402-5409[Abstract/Free Full Text].
13.	Gray, D. I., G. W. Gooday, and J. I. Prosser. 1990. Apical hyphal extension in Streptomyces coelicolor A3(2). J. Gen. Microbiol. 136:1077-1084[Abstract/Free Full Text].
14.	Guzman, L.-M., J. J. Barondess, and J. Beckwith. 1992. FtsL, an essential cytoplasmic membrane protein involved in cell division in Escherichia coli. J. Bacteriol. 174:7716-7728.
15.	Hao, J. Unpublished results.
16.	Horikawa, S., H. Nakazawa, and H. Ogawara. 1980. Penicillin-binding proteins in Streptomyces cacaoi and Streptomyces clavuligerus. J. Antibiot. 33:1363-1368[Medline].
17.	Ishino, F., and M. Matsuhashi. 1981. Peptidoglycan synthetic enzyme activities of highly purified penicillin-binding protein 3 in Escherichia coli: a septum-forming reaction sequence. Biochem. Biophys. Res. Commun. 101:905-911[Medline].
18.	Joris, B., J. M. Ghuysen, G. Dive, A. Renard, O. Dideberg, P. Charlier, J. M. Frere, J. A. Kelly, J. C. Boyington, P. C. Moews, and J. R. Knox. 1988. The active-site serine penicillin-recognizing enzymes as members of the Streptomyces R61 DD-peptidase family. Biochem. J. 250:313-324[Medline].
19.	Kelly, J. A., O. Dideberg, P. Charlier, J. P. Wery, M. Libert, P. C. Moews, J. R. Knox, C. Duez, C. Fraipont, B. Joris, J. Dusart, J. M. Frere, and J. M. Ghuysen. 1986. On the origin of bacterial resistance to penicillin: comparison of a $beta$ -lactamase and a penicillin target. Science 231:1429-1431[Abstract/Free Full Text].
20.	Kendrick, K. E., and J. C. Ensign. 1983. Sporulation of Streptomyces griseus in submerged culture. J. Bacteriol. 155:357-366[Abstract/Free Full Text].
21.	Kirby, R. 1992. Evolutionary origin of the Class A and Class C $beta$ -lactamases. J. Mol. Evol. 34:345-350[Medline].
22.	Kretschmer, S. 1989. Septation behaviour of the apical cell in Streptomyces granaticolor. J. Basic Microbiol. 29:587-595.
23.	Kwak, J., and K. E. Kendrick. 1996. Bald mutants of Streptomyces griseus that prematurely undergo key events of sporulation. J. Bacteriol. 178:4643-4650[Abstract/Free Full Text].
24.	Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[Medline].
25.	Liao, X., and R. E. W. Hancock. 1995. Cloning and characterization of the Pseudomonas aeruginosa pbpB gene encoding penillin-binding protein 3. Antimicrob. Agents Chemother. 39:1871-1874[Abstract].
26.	Liao, X., and R. E. W. Hancock. 1997. Identification of a penicillin-binding protein 3 homolog, PBP3x, in Pseudomonas aeruginosa: gene cloning and growth phase-dependent expression. J. Bacteriol. 179:1490-1496[Abstract/Free Full Text].
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