Characterization of the Starvation-Survival Response of Staphylococcus aureus

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J Bacteriol, April 1998, p. 1750-1758, Vol. 180, No. 7
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Characterization of the Starvation-Survival Response of Staphylococcus aureus

Sean P. Watson, Mark O. Clements, and Simon J. Foster^*

Department of Molecular Biology and Biotechnology, University of Sheffield, Sheffield, S10 2TN, United Kingdom

Received 17 November 1997/Accepted 20 January 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

The starvation-survival response of Staphylococcus aureus as a result of glucose, amino acid, phosphate, or multiple-nutrientlimitation was investigated. Glucose and multiple-nutrient limitationresulted in the loss of viability of about 99 to 99.9% of thepopulation within 2 days. The remaining surviving cells developedincreased survival potential, remaining viable for months. Aminoacid or phosphate limitation did not lead to the development ofa stable starvation-survival state, and cells became nonculturablewithin 7 days. For multiple-nutrient limitation, the developmentof the starvation-survival state was cell density dependent. Starvationsurvival was associated with a decrease in cell size and increasein resistance to acid shock and oxidative stress. There was noevidence for the formation of a viable but nonculturable stateduring starvation as demonstrated by flow cytometry. Long-termsurvival of cells was dependent on cell wall and protein biosynthesis.Analysis of [³⁵S]methionine incorporation and labelled proteins demonstratedthat differential protein synthesis occurred deep into starvation.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Bacteria in the natural environment are often found under nutrient-limiting conditions. To survive prolonged periods of starvation,many bacteria have developed starvation-survival strategies enablingthem to persist in the environment until conditions become favorablefor growth. The starvation-survival response of non-spore-forminggram-negative bacteria such as Escherichia coli, Salmonella typhimurium,and Vibrio spp. has been well characterized (10, 19, 21),but the responses of non-spore-forming gram-positive bacteriaare less well understood.

A number of gram-negative bacteria, including E. coli and Vibrio cholerae, have been proposed to enter a viable but nonculturable(VBNC) state upon starvation (48). The VBNC state has been definedas a cell which can be demonstrated to be metabolically activewhile being incapable of undergoing the sustained cellular divisionrequired to form a colony on a plate (34). The existence ofthe VBNC state is controversial, since the biochemical parameterswhich define a cell as viable or dead have not been universallyagreed.

Micrococcus luteus is the only gram-positive bacterium for which the starvation survival response has been characterized.It was shown that upon prolonged starvation, M. luteus persistsin a dormant state; cells in this state were unable to form colonieson agar plates (17). The recovery of dormant cells on agar plateswas found to be increased 1,000 to 100,000-fold by incubationin spent growth medium from exponential-phase cells. This ledto the proposal that a recovery pheromone was required to breakdormancy and allow the growth and division of dormant cells (18).To date, this is the only non-spore-forming bacterium for whichthe formation of such a dormant state has been well demonstrated.

In the gram-negative bacteria so far studied, nutrient starvation results in reductive division, giving rise to cells withan altered morphology and an increased long-term survival potential(10, 19, 21). Cells in the starved state also develop generalizedresistance to stresses over and above that of the adaptive responseof growing cells. These stresses include oxidizing agents, heat,near-UV radiation, and acid (10, 19, 21).

Cryptic growth is thought to play an important role in starvation survival. This is defined as the recycling of nutrientsderived from dead cells for the maintenance of a few survivingcells (38). There is also considerable evidence to suggest thatstarved cultures are not static populations. Culture dynamismis indicated from studies with E. coli, where long-term-starvedcells have a competitive advantage in a mixed culture with newlystarved cells (49).

The starvation survival of E. coli, Vibrio spp., and S. typhimurium is dependent on differential protein synthesis (25,39, 44). Bulk protein synthesis is sharply reduced duringstarvation and is associated with the lower expression of proteinsnecessary for exponential growth (30, 39). During the earlyhours of starvation, novel proteins whose continued activity andproduction is required for long-term survival are synthesized(25, 39). There is also evidence that the degradation of existingproteins may be a major source of amino acids utilized for proteinsynthesis during starvation (40).

Staphylococcus aureus is an important, worldwide pathogen, particularly in nosocomial infections (20). Infection of patientsin hospital wards occurs via a number of routes including directcontact (e.g., hand to wound), airborne carriage, and via surfacessuch as indwelling devices (e.g., catheters). These environmentsare frequently nutrient limiting and stressful. Therefore, anunderstanding of the mechanisms of S. aureus starvation survivaland stress resistance is of great interest and may lead to betterclinical practices to prevent the transmission of S. aureus infectionwithin hospitals. In this paper, we describe experiments whichelucidate the conditions required for the formation of a stablestarvation-survival state in S. aureus. The characterization ofthis state is described, and changes in cell morphology, physiologicalstatus, and stress resistance properties are assessed.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Growth and starvation of bacterial cells. S. aureus 8325-4 (29) was grown in a chemically defined medium (CDM) (13). The CDM preparation was amino acid limiting.Glucose- and phosphate-limiting CDM was prepared by lowering theglucose concentration from 1% (wt/vol) to 0.1% and the phosphateconcentration from 0.18 M to 36 mM. Starvation cultures were preparedby the inoculation of CDM to an absorbance at 600 nm (A₆₀₀) of0.01; the medium was then incubated at 37°C with shaking (250rpm). Stationary phase was reached after about 8 to 10 h of incubation.After 18 h of growth, the cultures were transferred to the long-termstarvation temperature and incubated statically. Multiple-nutrient-limitedcells were prepared by harvesting of CDM cultures, after 18 hof growth, by centrifugation (4,000 × g for 10 min at room temperature),and the cells washed twice with an equal volume of phosphate-bufferedsaline (PBS) by repeated centrifugation and resuspension. Thecells were finally resuspended in water to the original culturevolume. All the cultures reached an A₆₀₀ between 3.0 and 5.0,corresponding to 1 × 10⁸ to 5 × 10⁸ CFU ml¹. Viable counts were determined by serial dilution of culturesin PBS, plating on CDM agar (1% [wt/vol] agar), and incubationovernight (37°C). The minimum detection level was 100 CFU ml¹. Results are representative of at least two independent cultures,which showed no more than 10-fold variability between equivalenttime points.

Penicillin G inhibition. Penicillin G was added to starved cultures at 1 µg ml¹ (20 times the MIC). The biological activity of penicillin G in CDM overa 15-day incubation at 37°C decreased only twofold and hence wasstill 10 times the MIC.

Electron microscopy. Samples for examination were pelleted (10,000 × g for 5 min at 4°C), and the supernatant was removed. Standard fixing andstaining techniques were used to prepare cell sections, whichwere examined with a Philips CM-10 electron microscope. Mean celldiameters were calculated from measurements of 50 cells.

Preparation of cells for flow cytometry. The cells were enumerated by flow cytometry after being stained with fluorescein isothiocyanate (FITC)-conjugated human immunoglobulinG (IgG), which binds to surface-associated protein A (6). Samples(1 ml) were washed with PBS and resuspended in 1 ml of PBS containing3% (wt/vol) bovine serum albumin and 15 µg of FITC-conjugatedIgG ml¹. The cell suspension was incubated for 30 min at 37°C and washedthree times in PBS before being subjected to analysis by flowcytometry.

Viable-cell numbers were measured by flow cytometry after staining with rhodamine 123 (Rh123) by a modification of the methodof Diaper et al. (7). Rh123 is accumulated in an energy-dependentfashion, requiring active metabolism. Cell suspensions (1 ml)were washed with PBS and resuspended in 1 ml of PBS containing15 µM Rh123. The suspension was incubated for 30 min at room temperatureand washed three times in PBS. As a negative-staining control,S. aureus cells (1 ml) were incubated with 15 µM carbonyl cyanidem-chlorophenolhydrazone (CCCP) for 10 min and then stained withRh123; 15 µM CCCP was included in all solutions.

Flow cytometry. A Skatron instrument was used for flow cytometry. Sheaf fluid was prepared by filtering distilled water three times througha 0.22-µm-pore-size nitrocellulose membrane. The sheaf fluid pressurewas set at 1 kPa cm¹, and the flow sample rate was set between 1 and 10 ml min¹. Changes in light-scattering properties of the cells were monitoredwith light at a wavelength of between 395 and 440 nm. Narrow-anglelight scattering (NALS) used a gain of 32 and a photomultipliertube setting of 640 V. FITC-conjugated IgG and Rh123 fluorescencewas assessed with an excitation wavelength of 475 to 495 nm, astopband of 510 nm, and an emission wavelength of 520 to 560 nm.A peak at zero fluorescence is due to background noise.

Resistance to stress conditions. Cells during various phases of growth were harvested, washed in PBS, and resuspended at a cell density of about 5 × 10⁶ CFU ml¹. For oxidative stress challenge, 7.5 mM hydrogen peroxide wasadded and the cells were incubated at 37°C. Hydrogen peroxidechallenge was also performed on cells resuspended in their culturesupernatants to which 7.5 mM hydrogen peroxide had been added.For heat challenge, the cells were incubated at 55°C. Acid resistancewas determined at 37°C by resuspension of the cells in CDM whichhad been acidified to pH 2 with HCl. In all cases, changes incell viability were monitored for a 60-min period by serial dilutionin PBS followed by plating onto CDM agar, except for hydrogenperoxide resistance, where the cells were diluted in PBS containing10 mg of catalase ml¹ to inactivate the hydrogen peroxide before plating. UV resistancewas measured by spreading 5 ml of cells on a 15-cm-diameter glasspetri dish, which was then exposed to a Hanovia 30-W mercury lampat a distance of 60 cm. The decrease in cell viability was measuredfor 1 min.

Methionine incorporation rate determination. The cells were grown in glucose-limiting, methionine-free CDM. Samples (1 ml) were removed at various time points and pipettedinto a microcentrifuge tube, which had been prewarmed to 37°Cand which containing 20 µCi of [³⁵S]methionine (SJ235 [Amersham]; 1,200 Ci mmol¹) in 40 µl. The pulse length was adjusted so that the total incorporationwas roughly comparable in all samples. Unlabelled methionine (80µl, 10 mg ml¹) was added to the samples, which were placed on ice. The cellswere pelleted (10,000 × g at 4°C for 3 min), resuspended in 25µl of lysis buffer (10 mM Tris HCl [pH 7.4], 10 mM EDTA, 0.5 mgof lysostaphin per ml, 1 mM phenylmethylsulfonyl fluoride), andrepeatedly freeze-thawed (5 to 10 times) until lysis was visible.For determination of the level of incorporation, proteins wereprecipitated with 5% (wt/vol) trichloroacetic acid at 4°C for15 min and the precipitates were recovered by filtration (Millipore;pore size, 0.45 µm). The filters were washed with 4 ml of 5% (wt/vol)trichloroacetic acid prior to scintillation counting (BeckmanLS1801 scintillation counter).

For samples to be analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE), the appropriate volumeof lysate containing 5 × 10⁴ dpm was added to 6.25 µl of 5× SDS-PAGE loading buffer (10% [wt/vol]SDS, 25% [vol/vol] 2-mercaptoethanol, 50% [wt/vol] sucrose, 0.01%[wt/vol] bromophenol blue) and the volume was made up to 30 µl.These samples were boiled for 3 min and cooled before being subjectedto centrifugation (14,000 × g for 5 min at room temperature) toremove insoluble material and SDS-PAGE (Mini Protean; Bio-Rad)with a 15% (wt/vol) polyacrylamide gel (22). After electrophoresis,the gel was fixed (35% [vol/vol] methanol, 10% [vol/vol] aceticacid) for 60 min. The gel was then incubated in Amplify (Amersham)for 30 min before being dried and visualized by fluorography at $-$ 70°C with Hyperfilm-MP (Amersham).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Effect of nutrient limitation on starvation survival. The kinetics of starvation survival in glucose-, phosphate-, or amino acid-limiting CDM and in water at 37°C were examined(Fig. 1). Cultures limited for glucose or multiple nutrients (waterincubation) showed a very different response from those limitedfor amino acids or phosphate. Glucose- and multiple-nutrient-limitedcultures demonstrated biphasic kinetics: within the first 2 days,about 99 to 99.9% of the cells lost viability; after 2 days, thesurviving population remained relatively constant with only aslight decrease in viability after 25 days. Cultures limited forphosphate or amino acids demonstrated a rapid decrease in viability,becoming nonculturable after 4 and 7 days, respectively (>10⁵-fold drop in viability). The accelerated loss of viability inducedby amino acid and phosphate limitation may be due to the acidificationof the culture supernatant upon starvation, since the pH of thesecultures was found to decrease to 5.5 whereas glucose-limitedcultures remained at pH 7. All cultures lost viability in a temperature-dependentmanner, with higher temperatures resulting in a faster rate ofdeath (Fig. 1 and data not shown). For glucose-limited culturesincubated at 25°C, a 99% drop in viability was observed after7 days, at which point stable population numbers were realized.Cultures limited for multiple nutrients followed the same starvationkinetics as glucose-limited cultures, even if the initial growthwas in phosphate- or amino acid-limiting CDM before the transferto water. Hence, glucose limitation and multiple-nutrient limitationappear to be the most important stimuli involved in the long-termsurvival response of the cells to starvation.

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FIG. 1. Starvation-survival kinetics. Changes in viable counts of S. aureus 8325-4 grown in CDM limiting for glucose at 37°C ( $bullet$ ), glucose at 25°C ( $open circle$ ), phosphate at 37°C ( $black-triangle$ ), amino acids at 37°C ( $black-square$ ), and multiple nutrients by incubation in water at 37°C ( $square$ ) are shown.

Role of cell density in starvation survival. The effect of cell density on the survival of 6-h-post-exponential-phase cells resuspended in either water (Fig. 2a) or spentculture supernatant (Fig. 2b) was examined. Cells resuspendedin water at densities of 5 × 10⁶ CFU ml¹ or below lost viability rapidly, becoming nonculturable after2 days, whereas at higher cell densities, between 0.1 and 0.005%of cells survived prolonged incubation. When cells were resuspendedin spent culture supernatant, they retained culturability overthe 20-day period irrespective of the initial cell density. Stationary-phaseculture supernatants therefore contain sufficient nutrients tomaintain a population of about 10⁶ CFU ml¹.

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FIG. 2. Effect of cell density on the survival of glucose-limited S. aureus cells. Glucose-limited cells (6 h post-exponential phase) were washed and resuspended in either distilled water (a) or filter-sterilized culture supernatant (b) at cell densities of about 5 × 10⁸ ( $bullet$ ), 5 × 10⁷ ( $open circle$ ), 5 × 10⁶ ( $black-triangle$ ), and 5 × 10⁵ ( $black-square$ ) CFU ml¹. Changes in cell viability were determined over a 20-day period.

Cells already subjected to long-term glucose starvation (7 days) also showed a density-dependent survival phenotype. Whenthese cells were washed and resuspended in water at cell densitiesof >10⁶ CFU ml¹, 99 to 99.9% of them died until stable numbers were reached after3 days of incubation at 37°C (data not shown). At lower densities,the cells lost culturability with 2 days. When the cells wereresuspended in long-term-glucose-limited culture supernatants,they survived at all cell densities (data not shown). It thereforeappears that even though cells enter a starvation-survival state,their survival is still dependent on nutrients or factors presentin their culture supernatants or associated with the dead celldebris.

Effect of penicillin G on starvation survival. To elucidate if starved cells are growing and dividing during prolonged incubation, inhibitory concentrations of the cellwall biosynthesis inhibitor penicillin G were incubated with cellsat various stages during starvation (Fig. 3). The addition ofpenicillin G to cultures 8 h after the exponential phase acceleratedthe loss of viability, with the cells becoming nonculturable after11 days, while 0.1% of untreated cells were still viable. Similarresults were observed for 7-day-glucose-limited cultures, wherethe addition of penicillin G resulted in the cells becoming nonculturableafter 10 days, while 10% of cells were still viable in the culturesto which no penicillin had been added. Hence, the addition ofpenicillin G accelerated the rate of death of both postexponentialand starved cells. This suggests that although population numbersare relatively stable, starved cells are still active, exhibitingwall growth and probably division, although at a much lower ratethan exponential-phase cells, which lose viability within a fewhours of penicillin G treatment (data not shown).

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FIG. 3. Effect of penicillin G on survival in glucose-limiting CDM. Penicillin G (1 µg ml¹) was added to cultures either 8 h post-exponential phase ( $bullet$ ) or after 7 days of incubation ( $black-triangle$ ). Open symbols represent cultures to which no penicillin G was added ( $open circle$ , 8 h post-exponential; $triangle$ , 7 days of incubation).

Starvation-survival-associated morphological changes. Electron microscopic examination of glucose-limited cells (incubated at 21°C for 25 days) revealed an altered cell morphologycompared to exponential-phase cells (Fig. 4). At 25°C, long-term-glucose-limitedcells were quite heterogeneous, with a wide variation in cellsize, but they had a reduced average diameter of 0.41 ± 0.08 µmcompared to exponential-phase cells, which had an average celldiameter of 0.69 ± 0.08 µm. Fewer division septa were observed,with only 20% of glucose-starved cells showing division septacompared with 66% of exponential-phase cells. At 25°C, glucose-limitedcultures contained a large proportion of "ghost" cells, indicatingcell lysis; these can be seen as debris surrounding the intactcells in Fig. 4B. Interestingly, cultures incubated at 37°C hadno ghost cells (data not shown), but the cytoplasm of most cellswas patchy, possibly indicating cell death. The cell lysis observedat 25°C could be due to the induction of an autolysin which isrepressed when the cells are incubated at 37°C.

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FIG. 4. Electron micrographs of exponential-phase S. aureus cells grown in CDM at 37°C (a), and 25-day-glucose-limited cells incubated at 25°C (b). The cells were stained with uranyl acetate and Reynolds lead citrate before being subjected to microscopy.

Rapid assessment of viable, VBNC, and total cell numbers by flow cytometry. Flow cytometry allows the analysis of single cells within a population and hence can measure the heterogeneity of a populationwith respect to a number of parameters. Staining of cells withFITC-conjugated IgG is an accurate method of directly enumeratingthe total number of intact cells of S. aureus in a culture (6).FITC-conjugated IgG binds to protein A of S. aureus, with intactcells fluorescing more strongly than lysed cells. When exponential-phaseS. aureus cells were stained with FITC-conjugated IgG and thefluorescence distribution was determined by flow cytometry, 94%of the particles detected had a fluorescence peak channel numbergreater than 50 (Fig. 5a). As a negative control, E. coli, whichdoes not bind FITC-conjugated IgG, was shown to have a fluorescencedistribution below channel 50 (data not shown). Channel 50 thereforedefined the threshold level to distinguish between stained andnon stained cells. The extent of NALS can be used to indicatethe distribution of cell sizes within a population since it isdependent on the mass or volume of the cell, although this relationshipis not always linear (5).

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FIG. 5. Flow cytometric examination of S. aureus. (a) FITC-conjugated IgG-stained exponential-phase S. aureus cell grown at 37°C; (b) FITC-conjugated IgG-stained 3-week-glucose-limited cells incubated at 25°C.

The FITC-IgG staining and NALS distribution for exponential-phase cells (Fig. 5a) and glucose-limited cells incubated for3 weeks at 25°C (Fig. 5b) were compared. Glucose-limited cellsgave slightly higher fluorescence when stained with FITC-IgG (peakchannel fluorescence of 162, with 93% of the detected particlesabove channel 50) than did exponential-phase cells (peak channelfluorescence of 137, with 94% of the detected particles abovechannel 50). The most dramatic difference was observed with thedistribution of NALS. Exponential-phase cells gave a broad distributionof NALS (peak channel 65), indicating a large variation in cellsize, whereas the glucose-limited cells had a narrow defined distributionwith a lower peak channel number (peak channel 30), supportingthe electron microscopic conclusion that starved cells becomesmaller. The broad cell size distribution of exponential-phasecells was presumably due to the presence of large cells in theprocess of dividing and also of cells which had divided but notseparated. Clumping was minimized by treatment in a sonic bath(Kerry Ultrasonics), which breaks up aggregates but does not killcells.

The lipophilic dye Rh123 was used to enumerate viable cells, since it accumulates within bacterial cells in an energy-dependentfashion, with this accumulation being reversible by treatmentof cells with compounds which uncouple the membrane potential(16). Diaper and Edwards (6) demonstrated that Rh123 is auseful indicator of cell viability for S. aureus, since cell countsof CFU on nutrient agar were not significantly different fromthose obtained by flow cytometry counting Rh123-stained cells.

Rh123 staining was used to discriminate between viable and dead cells in glucose-limited cultures incubated at 25°C for 3weeks (Fig. 6a). The flow cytometric analysis revealed a heterogeneouspopulation, with a subpopulation of cells with low fluorescence(below channel 30) and another with higher fluorescence (abovechannel 55). When the same cells were treated with the membraneuncoupler CCCP (Fig. 6b), the population of cells with fluorescencegreater than channel 55 disappeared while the population withfluorescence below channel 30 increased. This confirmed that theaccumulation of Rh123 was energy dependent and enabled the identificationof cells with an active membrane potential. By fluorescence-activatedcell sorting, the population of cells with fluorescence greaterthan channel 50 was separated from the rest of the sample andthe fraction was plated onto CDM agar. The number of cells capableof forming colonies on agar was comparable to the number of fluorescentparticles separated by fluorescence-activated cell sorting (1.3× 10⁶ and 1.9 × 10⁶ ml¹, respectively). This is in agreement with the observation thatRh123 is an accurate indicator of cell viability (6). It alsoindicates that all "viable" starved cells are capable of recoveryon CDM plates.

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FIG. 6. Flow cytometric examination of S. aureus following Rh123 staining. (a) 3-week-glucose-limited cells incubated at 25°C; (b) 3-week-glucose-limited cells incubated at 25°C and treated with CCCP before Rh123 staining.

Viable-cell numbers enumerated by Rh123 staining were compared with those determined by measurement of CFU on CDM agar atvarious periods during starvation for cultures incubated at either25 and 37°C. There was no significant difference between viable-cellnumbers enumerated by either method, proving that there is noviable but nonculturable state during the starvation of S. aureus(data not shown).

Changes in resistance properties upon entry into starvation. Exponentially growing, 6-h-post-exponential-phase and 7-day-glucose-limited cells (incubated at 37°C) were exposed to oxidativestress, high temperature, UV light, and acidic conditions to determinechanges in the resistance levels of cells as they entered starvation.Under all stress conditions, 6-h-post-exponential-phase cellswere less resistant than exponential-phase or 7-day-glucose-starvedcells (Fig. 7 and results not shown). Compared to exponential-phasecells, 7-day-glucose-limited cells exhibited approximately a 100-foldincrease in resistance to both oxidative stress (Fig. 7a) andacid stress (Fig. 7c) after a 30-min treatment. However, therewas no increased resistance to heat (Fig. 7d) or to UV exposure(data not shown). Interestingly, resistance to oxidative stresscould be increased if the cells were left in their culture supernatantwhen exposed to hydrogen peroxide (Fig. 7b). Under these conditions,starved cells were almost completely resistant to 7.5 mM hydrogenperoxide whereas exponential-phase cells exhibited only a 1-log-unitdecrease in viability after 1 h. This increased resistance isprobably due to a catalase/peroxidase secreted into the supernatant,breaking down hydrogen peroxide before it can enter and damagethe cell.

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FIG. 7. Changes in the stress resistance of cells at different growth phases. Cells were harvested from glucose-limiting cultures during the exponential phase (A₆₀₀ = 0.6) ( $bullet$ ), at 6 h-post-exponential phase ( $black-triangle$ ), and after 7 days of incubation at 37°C ( $black-square$ ). The cells were washed in PBS and then resuspended in either PBS containing 7.5 mM H₂O₂ (a), their own supernatant containing H₂O₂ (7.5 mM) (b), CDM acidified to pH 2 with HCl (c), or PBS preheated to 55°C (d). Viability was measured at various times by performing appropriate dilutions onto CDM agar.

Intriguingly, 6-h-post-exponential-phase cells exhibited biphasic death kinetics under oxidative stress conditions (Fig. 7b)and when heat treated (Fig. 7d). Within the first 15 min, about99% of cells die, and then the rate of death decreased to becomecomparable to that of exponential-phase cells. This biphasic deathprofile is similar to that observed during glucose limitation,where about 99% of cells die and 1% survive prolonged starvation.

Role of protein synthesis during starvation survival. To determine whether continued protein synthesis is required for starvation survival, cells were treated with the proteinsynthesis inhibitor chloramphenicol during starvation (Fig. 8).Starvation was induced synchronously by transferring the cellsto glucose-free CDM. When chloramphenicol was added immediatelyupon transfer to starvation conditions, all the cells lost viabilitywithin 30 days, whereas the untreated culture retained 0.4% viabilityafter 60 days under these conditions. The chloramphenicol-inducedaccelerated loss of viability was greatest when chloramphenicolwas added within the first hour of starvation and decreased whenthe chloramphenicol was added later in starvation. However, itis interesting that even when chloramphenicol was added 24 h afterthe induction of starvation, the culture exhibited an approximately300-fold-greater drop in viability than did the control after55 days. These results show that proteins synthesized within thefirst hour are crucial to survival whereas continued protein synthesisis required for the long-term survival of cells.

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FIG. 8. Effect of chloramphenicol on the survival of glucose limited cells. Exponential-phase cells (A₆₀₀ = 1.0) were transferred to glucose-free CDM to induce synchronous starvation (0 h). Chloramphenicol (100 µg ml¹) was added after 0 h ( $bullet$ ), 1 h ( $triangle$ ), 2 h ( $black-triangle$ ), and 24 h ( $black-square$ ) of incubation at 37°C. A control culture with no chloramphenicol added ( $open circle$ ) was also monitored. Changes in viability were determined at various times by measuring colony formation on CDM agar.

Analysis of protein synthesis during glucose starvation. Changes in the rate of protein synthesis during starvation induced by glucose limitation in methionine-free CDM were examinedby pulse-labelling the cells with [³⁵S]methionine. When the [³⁵S]methionine incorporation rate was calculated per cell, long-term-starvedcells (5 days at 37°C) showed comparable incorporation rates toexponentially grown cells (1 to 4 dpm min¹ CFU¹), although incorporation by the nonviable cells cannot be ruledout.

Proteins synthesized during starvation were examined by [³⁵S]methionine pulse-labelling of cells grown in methionine-free glucose-limitingCDM, SDS-PAGE, and fluorography (Fig. 9). For the post-exponential-phaseculture (Fig. 9, lane 1), the cells were pulse-labelled for 5min, whereas long-term-starved cells were labelled for 1 h, dueto the lower methionine incorporation rates (lanes 2 to 4). Evenafter 5 days of starvation, a large number of proteins were stillbeing synthesized and the pattern was changing. Between 8 h and3 days of starvation, a 19-kDa protein was transiently expressed(lane 2). Two new proteins (21 and 15.5 kDa) appeared by 3 daysinto starvation and were still abundant after 5 days (lanes 3and 4). Even after 5 days of starvation, two new proteins increasedin intensity (26 and 36 kDa [lane 4]). Changes in protein expressiondemonstrate that specific proteins are produced during developmentof the starvation survival state, and there is also a temporalorder in the expression of these proteins. Since many proteinsare still synthesized 5 days into starvation, it confirms ourprevious observations that starved cells are not metabolicallydormant. Due to the extensive labelling times required to obtainenough material for analysis and the presence of large amountsof unlabelled material, two-dimensional gels of proteins synthesizedby long-term-starved cells were impractical.

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FIG. 9. SDS-PAGE analysis of proteins synthesized during glucose limitation. The cells were pulse-labelled with [³⁵S]methionine, and 2 × 10⁴ dpm of the cell lysate was loaded into each lane. Lanes: 1, 8-h culture; 2, 1 day after onset of the stationary phase; 3, 3 days after onset; 4, 5 days after onset.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

S. aureus is an important pathogen, and starvation associated-processes may well be important not only outside the host butalso as part of its pathogenicity. Elucidation of the survivalmechanism is also of intrinsic interest, since it is an importantpart of bacterial ecology. Given the medical importance of S.aureus and its obvious long-term survival potential, such knowledgemay lead to new procedures for the eradication of surviving cellsin the clinical environment.

The development of a long-term starvation-survival state of S. aureus was shown to be induced under glucose- or multiple-nutrient-limitingconditions, whereas phosphate- or amino acid limitation led toa rapid loss of cell viability. This parallels the situation withVibrio spp., where carbon starvation and multiple-nutrient starvationwere the only limiting conditions that resulted in cells withincreased survival potential (31). In contrast, S. typhimuriumand E. coli develop long-term survival potential irrespectiveof the limiting nutrient (24, 37).

Upon entry into the long-term starvation-survival state, 99 to 99.9% of S. aureus cells lost viability within the first 2days at 37°C. The viability of the culture then remained relativelyconstant for a period of months. This is similar to the survivalprofile of S. typhimurium (44) and of E. coli grown under certainlimiting conditions (41), where 90% of cells in the culturelose viability in the first few days. Why such a large proportionof cells die while a small number of cells survive is unclear.It is possible that this phenomenon is due to cryptic growth,where most of the cells die, providing nutrients for the maintenanceof the remaining surviving cells. The fact that the survival ofcells resuspended in water was observed only at high cell densitiessupports this theory. At low cell densities, the entire populationlost viability, presumably because the dying cells did not provideenough nutrients for the survival of a small subpopulation. Thissupports the observations of Diaper and Edwards (6) that S.aureus was able to survive prolonged starvation only at high celldensities in a lake water microcosm. In contrast, Vibrio spp.(31) and E. coli under certain defined conditions (41) cansurvive starvation without any loss of viability. The stationary-phasemedium of these cultures must therefore retain sufficient nutrientsfor the long-term survival of the total population without requiringthe sacrifice of cells to supply additional nutrients.

There is considerable evidence that starved cultures are not a static population of cells. Addition of penicillin G to starvedcultures resulted in an accelerated loss of cell viability, suggestingthat peptidoglycan synthesis is occurring, although very slowly.A similar effect has been observed in V. vulnificus, where theaddition of ampicillin to starved cells resulted in a slow lossof viability (36). Electron microscopy of S. aureus cells alsorevealed that starved cells were capable of cell division, sincea small proportion of cells had evidence of division septum formation.Culture dynamism has also been shown in E. coli, where long-term-starvedcells have a competitive advantage in a mixed culture with newlystarved cells (49). These changes take place due to the presenceof mutants with a growth advantage over the rest of the population.

It has been demonstrated that some bacteria may enter a VBNC state upon starvation (48). The existence of pathogenic bacteriain a VBNC state has wide implications for sterility testing, whichstill relies on the ability to form colonies in order to detectthe presence of bacteria. If VBNC cells can persist and regaingrowth capacity and pathogenicity once inside the host, conventionalsterility testing will fail to protect against infections. Ithas been reported that some VBNC cells can be resuscitated, includinga fraction of VBNC cells in membrane chambers in situ in the environment(36) and in vivo in mice (35).

We have found no evidence of the formation of a VBNC state in S. aureus upon starvation under defined conditions. The numberof cells determined by measurement of CFU on CDM agar was notsignificantly different from viable-cell counts determined byRh123 labelling and flow cytometry during starvation. Fluorescence-activatedcell sorting also demonstrated that Rh123-labelled particles weredue to living cells with colony-forming ability.

The acquisition of heightened resistance to environmental stresses is characteristic of the starvation-survival response ofmany gram-negative bacteria. For E. coli (15) and Vibrio spp.(31), starvation induces cross-resistance to heat, hydrogenperoxide, and UV irradiation, whereas S. typhimurium developsincreased acid, UV, and hydrogen peroxide resistance (42). Surprisingly,starvation of S. aureus did not confer a broad range of cross-resistanceproperties upon the cell. Resistance to acidic conditions andto oxidative stress increased, but no significant change in UVand heat resistance was observed. Interestingly, the increasedprotection against hydrogen peroxide was conferred by culturesupernatants and an increase in individual cellular resistance.Presumably, cells can synthesize an extracellular catalase thataccumulates in the external milieu, protecting the cells fromthe damaging effects of external hydrogen peroxide. This catalaseappears to be synthesized throughout growth, since both exponential-phaseand long-term-starved culture supernatants conferred resistanceto hydrogen peroxide. Such an extracellular catalase has beenidentified in Bacillus subtilis and was found to protect cellsfrom a hydrogen peroxide challenge (28).

E. coli has two catalases, one of which is synthesized only upon entry to stationary phase under the control of $sigma$ ^S (27), demonstrating the importance of oxidative stress resistancein starvation survival. Oxidative stress resistance is also importantin pathogenesis, since superoxide plays a significant role inthe killing process of S. aureus by neutrophils (12). Recently,it has also been shown that a periplasmic superoxide dismutasein S. typhimurium contributes to the pathogenesis of salmonellosisby protecting the cells from oxygen radical-mediated host defenses(9). Superoxide free radicals are neutralized by the actionof superoxide dismutase, generating hydrogen peroxide, which inturn is broken down by catalase.

Surprisingly, post-exponential-phase S. aureus cells had an increased sensitivity to hydrogen peroxide and heat stresses comparedto that of exponential-phase cells. The death kinetics were biphasic,with about 99% of cells appearing to be more sensitive to thesestresses than the remainder of the population. It may be thatthe cells which show reduced resistance properties are the samecells which will die upon long-term starvation. This suggeststhe possibility that the cells become committed to survival ordeath early after entry into the stationary phase unless theyare rescued by the provision of nutrients.

During long-term starvation, the cells undergo morphological changes. Glucose-starved S. aureus cells exhibited a reduceddiameter, a reduced number of division septa, and a more electron-denseappearance. The reduction in cell size upon starvation has beenobserved in a number of bacteria, including E. coli, Vibrio spp.,and M. luteus (19, 23, 26) and is thought to be the resultof reductive division upon entry into stationary phase. For E.coli, changes in cell morphology upon entry to stationary phaseare regulated by BolA (1). The bolA gene is induced duringentry to stationary phase under the control of stationary-phasesigma factor, $sigma$ ^S (23) and results in the increased expression of penicillin-bindingprotein PBP6, which is involved in septum formation.

We have shown that protein synthesis is necessary for starvation survival in S. aureus and that even long-term-starved cellsare actively synthesizing proteins. Protein synthesis was alsodemonstrated to be necessary for starvation survival in E. coli,Vibrio spp., and S. typhimurium (25, 39, 45). In S. aureus,the acceleration of loss of viability was greater the earlierchloramphenicol was added to glucose-starved cells. The proteinssynthesized during the first few hours of glucose starvation aretherefore probably critical for the survival of starvation. However,even though the majority of proteins required for starvation survivalare synthesized early, continued protein synthesis is still required.The requirement for continued protein synthesis during starvationwould not contradict a cryptic growth hypothesis. In E. coli andVibrio spp., most of the survival related proteins are similarlysynthesized during the early hours of starvation and continuedprotein synthesis is still essential (25, 39). We found thatfor S. aureus new proteins were being synthesized even 5 daysinto glucose starvation, which suggests the dynamic nature ofthe population. A similar analysis of protein synthesis by glucose-starvedE. coli cells also revealed marked changes in the identities ofproteins synthesized up to 5 days into starvation (2).

Similar changes have been observed, and well characterized by one- and two-dimensional gel electrophoresis, in E. coli, S.typhimurium, and Vibrio spp. (11, 31, 45). Many proteinsinvolved in starvation have been identified. It has been shownthat a characteristic set of 40 to 80 proteins are induced specificallyin response to starvation. In E. coli, the synthesis of starvationproteins involves the expression of several temporal classes ofstarvation genes, which are coordinately expressed under the controlof three alternative sigma factors (23, 32, 43). Some ofthe proteins synthesized in response to starvation have been identifiedand shown to play diverse roles, including nutrient scavenging(46), heat shock response (14), and recovery from starvation(33). One-dimensional gel analysis of proteins synthesized by5-day-starved E. coli cells led to the identification of severalprominently labelled proteins, one of which was designated DPS(for DNA binding protein from starved cells; 2). This proteinis abundant in 3-day-starved cells and was shown to form extremelystable complexes with DNA, leading to dramatic changes in proteinexpression, while also playing a role in protecting the DNA fromoxidative damage. It is interesting to speculate that the proteinsidentified during long-term starvation in S. aureus may play similarroles.

In this study, we have characterized the starvation-survival response of S. aureus. We are currently using transposon mutagenesisto identify mutants defective in starvation survival. This willenable the identification of specific components involved in theresponse and also of the global regulators of starvation-survivalgene expression. Recently, a homolog of B. subtilis $sigma$ ^B has been identified in S. aureus (47). $sigma$ ^B is involved in the regulation of stationary-phase and stressresistance genes in B. subtilis (3, 4, 8). S. aureus $sigma$ ^B is therefore a good candidate for a starvation-survival generegulator. We are currently analyzing the role of sigB in starvationsurvival and stress resistance in S. aureus.

	ACKNOWLEDGMENTS

This work was supported by the Royal Society (S.J.F.), BBSRC (S.P.W.), and the BBSRC/Celsis Connect (M.O.C.).

We thank Ian Morton for his assistance with the flow cytometry.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Biology and Biotechnology, University of Sheffield, Firth Court,Western Bank, Sheffield S10 2TN, United Kingdom. Phone: 44 1142224411. Fax: 44 114 2728697. E-mail: s.foster{at}sheffield.ac.uk.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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1.	Aldea, M., C. Hernandezchico, A. G. Delacampa, S. R. Kushner, and M. Vicente. 1988. Identification, cloning, and expression of bolA, an ftsZ-dependent morphogene of Escherichia coli. J. Bacteriol. 170:5169-5176[Abstract/Free Full Text].
2.	Almiron, M., A. J. Link, D. Furlong, and R. Kolter. 1992. A novel DNA-binding protein with regulatory and protective roles in starved Escherichia coli. Genes Dev. 12B:2646-2654.
3.	Binnie, C., M. Lampe, and R. Losick. 1986. Gene encoding the sigma-37 species of RNA polymerase sigma factor from Bacillus subtilis. Proc. Natl. Acad. Sci. USA 83:5943-5947[Abstract/Free Full Text].
4.	Boylan, S. A., A. Rutherford, S. M. Thomas, and C. W. Price. 1992. Activation of Bacillus subtilis transcription factor $sigma$ ^B by a regulatory pathway responsive to stationary-phase signals. J. Bacteriol. 174:3695-3706[Abstract/Free Full Text].
5.	Burkill, P. H. 1987. Analytical flow cytometry and its application to marine microbial ecology, p. 139-166. In M. A. Sleigh (ed.), Microbes in the sea. Ellis Horwood, Chichester, United Kingdom.
6.	Diaper, J. P., and C. Edwards. 1994. Survival of Staphylococcus aureus in lakewater monitored by flow-cytometry. Microbiology 140:35-42[Abstract/Free Full Text].
7.	Diaper, J. P., K. Tither, and C. Edwards. 1992. Rapid assessment of bacterial viability by flow cytometry. Appl. Microbiol. Biotechnol. 38:268-272[Medline].
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