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Novel Roles of the Master Transcription Factors Spo0A and ^B for Survival and Sporulation of Bacillus subtilis at Low Growth Temperature

Department of Microbiology, Rosario University School of Biochemistry and Pharmacy, and Institute of Molecular and Cellular Biology of Rosario, IBR-CONICET, Rosario, Argentina

Received 20 June 2003/ Accepted 5 November 2003

	ABSTRACT

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Spore development and stress resistance in Bacillus subtilis are governed by the master transcription factors Spo0A and ^B, respectively. Here we show that the coding genes for both regulatory proteins are dramatically induced, during logarithmic growth, after a temperature downshift from 37 to 20°C. The loss of ^B reduces the stationary-phase viability of cold-adapted cells 10- to 50-fold. Furthermore, we show that ^B activity is required at a late stage of development for efficient sporulation at a low temperature. On the other hand, Spo0A loss dramatically reduces the stationary-phase viability of cold-adapted cells 10,000-fold. We show that the requirement of Spo0A for cellular survival during the cold is independent of the activity of the key transition state regulator AbrB and of the simple loss of sporulation ability. Furthermore, Spo0A, and not proficiency in sporulation, is required for the development of complete stress resistance of cold-adapted cells to heat shock (54°C, 1 h), since a loss of Spo0A, but not a loss of the essential sporulation transcription factor ^F, reduced the cellular survival in response to heat by more than 1,000-fold. The overall results argue for new and important roles for Spo0A in the development of full stress resistance by nonsporulating cells and for ^B in sporulation proficiency at a low temperature.

	INTRODUCTION

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The exposure of bacteria to diverse growth-limiting conditions induces the synthesis of a large set of proteins (called general stress proteins) that protect the cell against internal (metabolic) or external (environmental) stresses (22, 23, 29, 32, 33). In the gram-positive, endospore-forming bacterium Bacillus subtilis, the general stress response is controlled mainly by ^B, the alternative transcription factor of the RNA polymerase that brings about a special physiological state which significantly enhances bacterial survival (11, 20, 22, 23, 29, 32, 33, 37). It is estimated that over 200 genes (5% of the coding capacity of the genome) are directly or indirectly under ^B control, and the loss of ^B function leads to multiple-stress sensitivity, compromising the survival of the ^B null mutant strain (23, 29, 32). Besides having this very important, rapid, reversible, and plastic adaptive response (22, 29), B. subtilis is also able to differentiate into dormant spores when nutritional conditions become so extreme that the ^B-dependent response would not be adequate to guarantee the survival of the cell (19, 21, 24, 30, 31). While ^B is the key regulatory protein involved in the reversible adaptive stress response of vegetative cells, the master transcription factor Spo0A is the key regulator responsible for the decision of a vegetative cell to differentiate into a dormant and highly resistant new cell, i.e., the spore (31). It is accepted that these responses, general stress adaptation and sporulation, are important for the survival of B. subtilis in its natural environment, i.e., soil (29-33). Furthermore, high levels of expression of general stress proteins provide stressed or starved cells with multiple, nonspecific, protective functions for future or unexpected insults (37). In particular, soil is subject to important fluctuations of the environmental temperature, which can vary from mesophyllic values at midday to chilling temperatures at night (28, 41). Taking these observations into consideration, we considered it to be of interest to analyze whether ^B and/or Spo0A might play a role in the stress adaptation and survival of B. subtilis during growth and permanence at a low growth temperature.

	MATERIALS AND METHODS

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Bacterial strains, media, and growth conditions. The experiments conducted in this study were performed with wild-type reference strain JH642 and isogenic derivatives (38). Mutations and gene reporter fusions were introduced into strain JH642 by transformation of competent cells as previously described (3). The parent strain and the resulting isogenic derivatives are described in Table 1. Bacteria were routinely grown under vigorous agitation (220 rpm) in Spizizen minimal medium (MM), with 0.5% (wt/vol) glucose as the carbon and energy source and L-tryptophan (50 µg/ml) and L-phenylalanine (50 µg/ml) (14). Where indicated below, the strains were grown in Schaeffer sporulation medium or Luria-Bertani (LB) medium. For sporulation efficiency, cells were grown in MM for the times indicated in Tables 2 and 3 and the figure legends and then treated with CHCl₃ or heated at 80°C for 15 min before being plated (38). For drug resistance selection in B. subtilis, antibiotics were used at the following final concentrations: 5 µg/ml for chloramphenicol, 1 µg/ml for erythromycin, 2 µg/ml for kanamycin, and 25 µg/ml for spectinomycin.

Western blot analysis. B. subtilis cultures of the parent strain JH642 and its isogenic derivate Sik31 (spo0A::Ery^r P_spac-spo0Asad67) (Table 1) were grown in MM and LB medium, respectively. Aliquots of 20 ml of each culture were collected by centrifugation and washed three times in disruption buffer {50 mM TES [N-tris(hydroxymethyl)methyl-2-aminoethanesulfonic acid], 50 mM NaCl, 5 mM dithiothreitol, 10% glycerol, 1 mM EDTA (pH 7.5), and protease inhibitor cocktail (Complete; Boehringer)}. Cells were finally resuspended in 0.5 ml of disruption buffer and disrupted by sonication (six times, 10 s each time) using a model 200 sonifier (Branson). Cell debris was removed by centrifugation (10 min, 13,000 rpm at 4°C [Marathon 16 Km; Fisher Scientific]). Protein concentrations in crude extract were determined by using the Bradford protein assay (Bio-Rad) (8a). The samples were subjected to sodium dodecyl sulfate-12% polyacrylamide gel electrophoresis, transferred to an Immobilon membrane (Millipore, Bedford, Mass.), and revealed by using anti-Spo0A rabbit antibody and an alkaline phosphatase-conjugated anti-rabbit immunoglobulin G (IgG) (Bio-Rad). For signal quantification, films were scanned and analyzed densitometrically. The Sik31 culture was grown in LB medium at 37°C until the mid-exponential phase. At this point, IPTG (isopropyl-ß-D-thiogalactopyranoside; 1 mM) was added to half of this culture, and growth continued for another 2 h. After this induction period (production of Spo0A-Sad67), the culture was processed for protein analysis.

	RESULTS AND DISCUSSION

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Expression of sigB and spo0A at a low growth temperature. It was previously shown that the measurement of ß-galactosidase activity from transcriptional lacZ fusions constitutes a satisfactory method to analyze the response of B. subtilis genes to cold shock (1, 2). Therefore, we assayed the effect of the cold shock (from 37 to 20°C) on the expression of sigB (coding for ^B) and spo0A in isogenic B. subtilis strains harboring transcriptional lacZ fusions to the promoter regions of both regulatory genes (Table 1). Figure 1A shows a typical growth curve of a culture of B. subtilis grown in MM (Spizizen salts supplemented with 0.5% glucose, 50 µg of Trp/ml, and 50 µg of Phe/ml) with strong aeration (220 rpm) until the early exponential phase (optical density at 525 nm [OD₅₂₅], 0.25), half of which was then transferred from 37 to 20°C. The cold-shocked culture did not show a lag phase, and the generation times under these conditions of exponential growth at 37 and 20°C were 2.5 and 13.0 h, respectively (Fig. 1A). Despite the important reduction in the rate of growth, the cold-shocked culture reached the same cellular density as that of the culture that remained at 37°C (Fig. 1A) and reached similar cellular yields at both temperatures (an average of 1.0 x 10⁸ to 4.0 x 10⁸ CFU/ml [data not shown]). Under these experimental conditions, comparing cultures maintained at 37°C, we observed a reproducible 10-fold increase in sigB expression and a significant induction (four- to fivefold increase) of spo0A expression during the vegetative and stationary phases of the cultures transferred to 20°C (Fig. 1B and C). Interestingly, despite the absence of a lag phase, the cold induction of sigB and spo0A after the temperature downshift was not immediately perceptible. This delay in gene activation is intriguingly different from what occurs with the widely studied induction of sigB that follows the input of metabolic or environmental stress signals at 37°C (7, 8, 23, 29, 33) or the rapid response of the cold shock regulon of B. subtilis (6, 16-18, 39). Effectively, all these adaptive responses are fully displayed after the first 15 min following the stress (6, 29, 33). By contrast, in our study, the induction of sigB and spo0A began to be noticeable only 4 to 5 h following the temperature downshift but many hours before (40 h) the cold-shocked cultures reached the stationary phase of growth at 20°C (Fig. 1B and C). Interestingly, this apparent delay of ^B induction during adaptation to the cold had been previously reported to occur during the cold shock response of the psychrotrophic food-borne pathogen Listeria monocytogenes (5). In this bacterium, the ^B-like transcription factor was induced by the cold shock (from 37 to 8°C) only 4 h following the temperature downshift, with a substantial increase in sigB expression after 6 h of that treatment (5). Furthermore, as is the case for sigB in B. subtilis, the induction of the ^B-like transcription factor of L. monocytogenes by other stresses (i.e., osmotic stress) at 37°C occurs during the 10 min that follows the stressing signal (12). Thus, we deduced that although sigB and spo0A are not components of the rapidly induced cold shock regulon of B. subtilis (6), they may constitute a second repertoire of genes induced during the vegetative growth of the adapting cell to the low growth temperature.

View larger version (26K): [in this window] [in a new window]   FIG. 1. Growth and gene expression of B. subtilis at 37 and 20°C. (A) Growth curve of wild-type strain JH642 in MM at 37°C (filled symbols) or transferred at early exponential phase (OD525 of 0.25) to 20°C (open symbols). The growth curves are representative of several independent experiments (see the text for details). (B to E) JH642-derived B. subtilis strains harboring the lacZ fusions indicated in each panel were grown in MM at 37°C (filled symbols) until early exponential phase. Then, half of each culture was shifted (at the point indicated by the asterisk) to 20°C (open symbols). Samples were collected at different OD525s and assayed for ß-galactosidase activity expressed in Miller units. The arrows in each panel indicate the end of the exponential growth of each culture and the beginning of the stationary phase. (E) The curves with open symbols correspond to the Miller units accumulated at 20°C in cultures proficient () or deficient () in the production of the H transcription factor. In addition, the accumulation of ß-galactosidase activity of the same H-deficient culture grown at 37°C for the entire experiment () is shown (see the text for details). The strains used for the experiments were MR100 (B), JH19005 (C), MR102 (D), and JH19005 () and MR200 ( and ) (E). The ß-galactosidase experiments described above were independently repeated five times in triplicate, and a representative set of results is shown in each panel. (F) Diagram showing the appearance of Spo0A and B during the vegetative growth of a cell transferred to a low growth temperature.

It has been extensively observed that the induction of sigB and spo0A expression in cultures of B. subtilis grown at 37°C under nonstress conditions occurs only at the beginning of the stationary phase of growth (T₀). It is believed that this postexponential induction of sigB and spo0A expression at 37°C allows the growth-restricted cells to adapt (^B-dependent response) or sporulate (Spo0A-dependent response) under the unfavorable conditions prevailing during the stationary phase (23-25, 29, 33). By contrast, the present results indicate that sigB and spo0A expression is induced after a temperature downshift from 37 to 20°C and suggest that ^B and Spo0A would be overproduced in cold-shocked cells of B. subtilis many hours before the beginning of the stationary phase of growth. Moreover, the unexpected high levels of induction of sigB and spo0A expression during the logarithmic growth of B. subtilis at 20°C (Fig. 1B and C) leaves open the possibility that ^B and/or Spo0A plays a previously unrecognized role during the adaptive response of this bacterium to the cold (Fig. 1F).

Spo0A is overproduced and active during the vegetative phase of cold-shocked cells. As we have shown, the expression of the regulatory genes spo0A and spo0H was highly induced after the temperature downshift (Fig. 1C and D). Since the expression of both genes is controlled by a positive autoregulatory loop (3, 4, 24, 25, 31) that requires high levels of the active phosphorylated form of Spo0A (Spo0AP), it can be hypothesized that the observed upregulation of ß-galactosidase activity derived from the spo0H-lacZ and spo0A-lacZ fusions at the low temperature reflected an overproduction of Spo0A during the vegetative phase. Hence, it was conceivable to hypothesize that the active form of Spo0A (Spo0AP) should be present in higher levels at 20°C than at 37°C. Effectively, Western blot experiments using anti-Spo0A antibodies (4) confirmed the overproduction of Spo0A during the logarithmic growth of B. subtilis at 20°C (Fig. 2). The vegetative levels of Spo0A at 20°C were severalfold higher than the levels of the regulatory protein found in logarithmic cells of the same strain (JH642) grown at 37°C (Fig. 2). This result confirmed the overproduction of Spo0A and strongly suggested that Spo0AP was predominant during logarithmic growth at the low temperature. Effectively, this presumption was confirmed since the expression of two exclusive Spo0AP-dependent sporulation genes (spoIIA and spoIIG), which are normally activated after T₀ at 37°C, was dramatically induced many hours (40 h) before the cold-shocked culture reached the stationary phase of growth (T₀) (Fig. 3). These results confirmed the cold induction of spo0A and the overproduction of active Spo0A (Spo0AP) during the vegetative growth of B. subtilis at the low temperature (Fig. 3C).

View larger version (27K): [in this window] [in a new window]   FIG. 2. Western blot analysis of Spo0A levels in vegetative cells grown at 37 and 20°C. (A) Crude protein extracts were prepared from cultures of the wild-type strain JH642 grown in MM at 37 or 20°C until the end of the exponential phase. After separation by sodium dodecyl sulfate-polyacrylamide protein gel electrophoresis and transfer of the proteins to a nitrocellulose membrane, the proteins were reacted against anti-Spo0A antibodies. (B) Specificity and sensitivity of the antibodies used (kindly provided by F. Kawamura and M. Fujita) to put in evidence the level of induction of spo0A (see Materials and Methods for details). The 8.1 ratio in panel A indicates the increase in the level of Spo0A (determined by densitometric analysis) that occurred during growth at the low temperature relative to the level produced by the same strain grown at 37°C. ND, not determined.

View larger version (19K): [in this window] [in a new window]   FIG. 3. Active Spo0A is present during the logarithmic phase of cold-shocked cultures. (A and B) Levels of expression of the Spo0AP-dependent genes spoIIA (strain JH16302) (A) and spoIIG (strain JH16304) (B) in cultures grown in MM at 37°C (filled symbols) or transferred (at the moment indicated by the asterisk) to 20°C (open symbols) are shown. The arrows indicate the end of the exponential growth of each culture. (C) Diagram of the production of Spo0AP in a vegetative cell after its transference to a low growth temperature (see the text for details).

View larger version (27K): [in this window] [in a new window]   FIG. 4. The transcription factor Spo0A, and not the ability to sporulate, is required for the survival of B. subtilis during long permanence at a low growth temperature. (A) Survival of cold-shocked cells during permanence in the stationary phase of growth. The wild-type strain JH642 () and its isogenic derivatives; the single mutant strains JH646 (spo0A []), RG12607 (abrB::spc []), and RG19148 (sigF::kan []); and the double mutant strain MR12607 (spo0A::ery-abrB::spc []) were grown in MM at 20°C until 2 weeks into the stationary phase. Cellular survival during the stationary phase was monitored by measuring the OD525 and by plating appropriate dilutions of samples at different times (see the text for details). The data shown are the averages of results from four independent experiments. (B) Diagram showing the two roles (sporulation and stress adaptation) of Spo0A that contribute to the survival of B. subtilis at a low environmental temperature.

A loss of ^B function results in a decreased rate of survival of cells grown at a low temperature.

View larger version (17K): [in this window] [in a new window]   FIG. 5. The transcription factor B is overproduced and required for the cellular survival of B. subtilis at a low temperature. (A) Induction of the B-dependent reporter fusion ctc-lacZ (strain MR101) after a temperature downshift (indicated by the asterisk) from 37°C (filled symbols) to 20°C (open symbols). The arrows indicate the commencement of the stationary phase of growth. (B) Survival of sigB+ and sigB mutant B. subtilis cells during the stationary phase at 20°C. The wild-type strain JH642 () and its isogenic sigB mutant derivate MR644 () were grown until several days into the stationary phase in MM at 20°C. Cellular survival was determined as described in the legend to Fig. 4A. The data are the averages from four independent experiments. (C) Synthesis and requirement of the B transcription factor for B. subtilis survival after a temperature downshift during the logarithmic phase of growth.

A loss of ^B function results in a delayed and decreased sporulation proficiency for B. subtilis at a low growth temperature.

View larger version (47K): [in this window] [in a new window]   FIG. 6. The transcription factor B is required for an efficient sporulation of B. subtilis at low temperatures. (A) Sporulation phenotype of B-proficient (sigB+) and B-deficient (sigB-) cells (strains JH642 and MR644, respectively) after 1 week of incubation on solid sporulation medium (Schaeffer agar plate) at 20°C. Note that the B-deficient strain (on the right site of the plate) formed translucent and dying colonies but that the wild-type strain (sigB+) formed opaque colonies that indicate spore formation. (B) Cellular viability and efficiency of spore formation of sigB+ and sigB mutant B. subtilis cells during growth and maintenance at 20°C. The wild-type and sigB strains JH642 and MR644, respectively, were grown in MM at 20°C and assayed for cellular survival and spore formation as described in the text. Black bars, viable JH642 cells; shaded bars, viable MR644 cells; hatched bars, JH642 spores; open bars, MR644 spores). The data are the averages of results from five independent experiments.

View larger version (40K): [in this window] [in a new window]   FIG. 7. The transcription factor B is required at a late stage of spore development in cultures grown at a low temperature. (A to D) ß-Galactosidase accumulation in B-proficient (filled symbols) and B-deficient (open symbols) cultures grown after inoculation at 20°C. The strains utilized for these experiments harbored transcriptional lacZ fusions activated by Spo0AP (JH16302 and MR16302) (A), F (RG2051 and MR2051) (B), E (RG851 and MR851) (C), and G (RG348 and MR348) (D). (E) Diagram illustrating the novel requirement of B activity to complete the last developmental stages of spore development.

sigB induction is interconnected with the Spo0AP activity in B. subtilis.

View larger version (37K): [in this window] [in a new window]   FIG. 8. Spo0AP downregulates the expression of sigB at 37 and 20°C. (A) This diagram shows three possibilities for the complete adaptation of B. subtilis to the cold. (I) The temperature downshift induces the production of Spo0AP, which in turn is essential for sigB induction and cold adaptation. (II) The alternative transcription factor B is primarily induced by the cold shock, and its activity is essential for spo0A induction and cold adaptation. (III) The inductions of expression of sigB and spo0A, after the temperature downshift, are independent of one another. The independent induction of Spo0A and B provides the cold-shocked cell with different attributes (the scarf and the wool cap) to confront the low temperature. (B and C) ß-Galactosidase accumulation in JH642-derived strains proficient and deficient in B (B) or Spo0A (C) function. The strains harboring a spo0A-lacZ (B) or a sigB-lacZ (C) fusion were JH19005 (sigB+ [filled symbols]) and MR19005 (sigB mutant [open symbols]) (B) and MR100 (spo0A+ [filled symbols]) and MR110 (spo0A mutant [open symbols]) (C). The strains had been grown since inoculation in MM at 37 or 20°C and processed as indicated in the legend to Fig. 1. (D) Shown are the independence of the cold induction of sigB and spo0A from the activities of Spo0A and B, respectively (possibility III in panel A) and the negative effect, direct or indirect, of Spo0AP activity on sigB expression.

The main contribution of the present work is the evidence that the very recently characterized cold shock response (6) is not sufficient for the development of a complete adaptation to low temperatures, and hence of the survival, of B. subtilis. In fact, the present study demonstrates that the genes encoding the key transcription factors Spo0A and ^B are strongly induced after a temperature downshift from 37 to 20°C (Fig. 1). This transcriptional induction of spo0A and sigB was not immediate, as it was for the genes belonging to the cold shock regulon that were induced during the first minutes following the temperature downshift (6), but occurred during logarithmic growth and many hours (45 h) before the cold-shocked cultures reached the stationary phase of growth (Fig. 1). This delay in gene activation might explain why the cold induction of sigB and spo0A was not observed in previous proteome and transcriptome studies that analyzed the initial response of B. subtilis to cold shock (6, 16-18, 39). Our results suggest that spo0A and sigB might correspond, as would be the case for the sigB-like gene of L. monocytogenes (5), to a second class of cold-induced genes whose function is not related to an immediate adaptation of the cell to cold shock but is related to cellular viability and stress survival during long permanence at the low temperature.

It can be unquestionably asseverated that Spo0A is essential for spore formation at any temperature, but this work has clearly demonstrated that Spo0A has a novel sporulation-independent activity required for the efficient survival of nonsporulating resting cells at a low temperature (Fig. 4). Furthermore, the strong spo0A expression during the logarithmic phase at 20°C (Fig. 1C) and the overproduction of active Spo0A (Fig. 2 and 3) were not correlated with an improved ability of the cold-adapted cells to form spores at the low temperature (Table 2). Effectively, the number of spores formed at 20°C did not differ from the number of spores formed at 37°C during either the exponential phase or the early stationary phase of growth (Table 2). This result opened the possibility that the overproduction of Spo0AP during logarithmic growth at 20°C might be required for the development of full stress resistance before the cold-adapted cells abandon exponential growth. In fact, cold-adapted cells proficient in Spo0A activity at the end of exponential growth (T₀) were >2,000-fold more resistant to heat treatment (54°C, 1 h) than were the equivalent cells deficient in Spo0A production (Table 3). These properties were completely dependent on Spo0A activity and not on the sporulation ability or the activity of the transition state regulator AbrB (Fig. 4A). Therefore, these results indicated a novel and important role for Spo0A in cellular viability and stress survival at a low growth temperature (Fig. 9). This new role of Spo0A might contribute to the preparation of B. subtilis cells for future stresses during long-term survival as nongrowing vegetative cells in natural environments (Fig. 4B and 9).

View larger version (42K): [in this window] [in a new window]   FIG. 9. Workable model marking the novel participation of the transcription factors Spo0A and B in the stress adaptation and sporulation of B. subtilis at a growth-restricting temperature (20°C) in comparison to their roles at an optimal laboratory temperature (37°C) (see the text for details).

	ACKNOWLEDGMENTS

 
We are indebted to A. Grossman, W. Haldenwang, F. Kawamura, T. Leighton, R. Losick, P. Piggot, C. Price, P. Setlow, G. Shujman, W. Schumann, G. Spiegelman, and P. Zuber for providing strains and suggestions during the course of the work. We also thank F. Kawamura and M. Fujita for the anti-Spo0A antibodies.

This research was supported by grants from the following national agencies: Fundación Antorchas (RG-14022-57), FONCyT (RG-PICT-0103379), and CONICET (RG-PIP-03052).

	FOOTNOTES

 
* Corresponding author. Mailing address: Facultad de Ciencias Bioquímicas y Farmacéuticas, Departamento de Microbiología, Subsuelo de Sala 9, Suipacha 531, Rosario-2000, Argentina. Phone: (54) 341-4353377. Fax (54) 341-4804601. E-mail: rrgrau{at}infovia.com.ar.

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