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Applied and Environmental Microbiology, August 2002, p. 3873-3877, Vol. 68, No. 8
0099-2240/02/$04.00+0     DOI: 10.1128/AEM.68.8.3873-3877.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.

The pepR Gene of Lactobacillus sakei Is Positively Regulated by Anaerobiosis at the Transcriptional Level

Unité Flore Lactique et Environnement Carné, INRA, Domaine de Vilvert, 78 350 Jouy en Josas, France

Received 31 October 2001/ Accepted 19 April 2002

	ABSTRACT

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Lactobacillus sakei is a lactic acid bacterium belonging to the natural flora of meat products. It constitutes the main flora of vacuum-packed meat and is largely used in western Europe as a starter for the manufacturing of fermented sausages. This species is able to grow both under aerobiosis and anaerobiosis. In many technological processes involving it, oxygen is scarce. The aim of this study was to identify the major proteins affected by growth under anaerobiosis. Using two-dimensional electrophoresis, we showed that one spot was 10-fold overexpressed when cells were grown under anaerobiosis. By N-terminal sequencing it was identified as a peptidase (PepR), and the pepR gene was cloned. Northern analysis revealed that pepR was expressed as a single 1.27-kb transcript induced under anaerobiosis. A mutant was constructed by single crossover in the pepR gene, and its growth and survival were not affected by anaerobiosis.

	INTRODUCTION

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Lactobacillus sakei (formerly Lactobacillus sake) (32) is one of the most important lactic acid bacteria (LAB) in meat technology. It is naturally present on fresh meat and becomes the predominant flora on vacuum-packed meat. It is largely used in France and western Europe as a starter for the manufacturing of fermented sausages. This species is able to produce lactic acid and also some compounds that are inhibitory towards pathogenic or spoilage bacteria. It also might be involved in aroma production. Its development during technological processes is thus very important for organoleptic and safety reasons (for a review, see reference 5). This species is facultatively heterofermentative, and it is able to grow under both aerobiosis and anaerobiosis. Nevertheless, during the main technological process in which it is involved, it must develop under hypoxic environmental conditions.

Two-dimensional electrophoresis (2-DE) is a powerful method to investigate variation of protein expression during environmental changes. It has been used to investigate changes induced by anaerobiosis in various species. The gram-negative species Escherichia coli (2, 22, 28), Salmonella enterica serovar Typhimurium (30), and Neisseria gonorrhoeae (7) and the gram-positive species Bacillus subtilis (20) have been studied by this approach. Such studies led to the identification of proteins whose expression was significantly modified by the presence or absence of oxygen. These proteins could be assigned to respiratory or carbon flux functions, and proteins subjected to catabolite repression have been shown to be also regulated by growth under anaerobiosis. In E. coli, analysis of the glucose starvation stimulon revealed a partial similarity to the response to a shift from aerobiosis to anaerobiosis (22). Proteins induced by acids or bases during aerobic or anaerobic growth were also analyzed by 2-DE. It appeared that some inductions were pH dependent only, but complex relationships between pH and oxygen were shown (2). In N. gonorrhoeae, a shift from aerobiosis to anaerobiosis resulted in the induction of outer membrane proteins (7). In B. subtilis, such a shift resulted in the induction of various systems for the utilization of alternative carbon sources (inositol, melibiose, and 6-phospho--glucosides). Mutants affected in global regulatory proteins were also analyzed, and this allowed identification of the genes whose regulation was independent from these systems (20).

The aim of this study was to identify the major protein(s) of L. sakei affected by growth under anaerobiosis. In this paper we show that a peptidase is 10-fold overexpressed during growth under anaerobiosis. The corresponding gene, pepR, was identified, and its regulation was studied.

	MATERIALS AND METHODS

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Strains and growth conditions.
Two L. sakei strains were used. The wild-type strain 23K (1) and a pepR mutant, RV4041, were routinely grown at 30°C in MRS medium (8) or MCD medium (13) supplemented with glucose (5 g liter^-1) as the carbon source. When necessary, media were supplemented with 5 mg of erythromycin liter^-1. E. coli TG1 was used for cloning experiments. It was routinely grown at 37°C on Luria-Bertani medium supplemented with ampicillin (50 mg liter^-1) when necessary. Aerobiosis was obtained by shaking flasks at 200 rpm. Anaerobiosis was obtained either under nitrogen (12) or under carbon dioxide using the Anaerogen GasPak (Oxoid) system in BBL jars. Growth was evaluated by measuring the optical density at 600 nm (OD₆₀₀).

Growth and survival of the pepR mutant (RV4041) were tested at 30°C in MCD medium under both aerobiosis and anaerobiosis in the presence or absence of 10 µg of puromycin ml^-1 for up to 40 h. Growth and survival after addition of 20 µg of puromycin ml^-1 at the end of the exponential phase of growth were also monitored under the same conditions. The effect of temperature was tested by comparing the ability to grow on MRS agar supplemented or not with puromycin 10 µg ml^-1 and by incubating plates at either 30 or 37°C under aerobiosis or anaerobiosis.

2-DE and N-terminal sequencing.
Analyses were performed as previously described on 30-µg protein extracts (19). Gels were stained using silver nitrate (19). In some experiments Sypro Orange (Molecular Probes) was used. After the second dimension was run, gels were fixed for 30 min in 7.5% acetic acid-0.05% sodium dodecyl sulfate. Staining was performed by incubation for 1 h in 0.02% Sypro Orange-7.5% acetic acid. Reading was performed on a fluoroimager with excitation at a wavelength of 488 nm (Molecular Dynamics). Quantification was done by using ImageQuant software (Molecular Dynamics).

PCR amplification of the pepR gene and cloning of the pepR region.
Degenerate primers 5'-TTC(T)ATGCAC(T)TGC(T)TTA(G)CC-3' and 5'-(A,T,C,G)CGG(A)TTT(C)TC(A,T,C,G)GCT(C)TC-3' were used for the PCR amplification of a DNA fragment of strain 23K. PCR experiments were performed on a Perkin-Elmer 9600 apparatus using Taq DNA polymerase from Promega. Reactions were carried out in 10 µl with 1 µg of chromosomal DNA, a 0.2 mM concentration of each deoxynucleoside triphosphate, a 2.5 µM concentration of each primer, and 1.25% formamide for 30 cycles (94°C for 1 min, 55°C for 2 min, and 72°C for 3 min).

Cloning experiments were performed in pBluescript SK(+) (Stratagene) by standard methods (24) and as previously described (31). Southern hybridizations were performed with chemiluminescence using a kit, according to the instructions of the manufacturer (Amersham). DNA sequence reactions were done using dye terminator dideoxynucleotides and Taq DNA polymerase on a Perkin-Elmer 9600 apparatus, and products were separated on a Perkin-Elmer sequencing apparatus 337. DNA sequence was analyzed with the Genetics Computer Group software package from the University of Wisconsin.

Construction of a pepR mutant by single crossover.
An internal fragment of the pepR gene was amplified by PCR and cloned in the integrative vector pRV300 (14), leading to plasmid pRV415. This plasmid was used to transform L. sakei strain 23K for erythromycin resistance as previously described (1, 14). The structure of the mutated pepR gene was verified by PCR.

Analysis of the pepR transcript.
RNA preparation and Northern hybridization were performed as previously described (31) with the following modifications. Thirty micrograms of total RNAs was loaded on the gels. Labeling of the probes was performed with an enhanced chemiluminescence kit (ECL) according to the instructions of the manufacturer (Amersham).

Nucleotide sequence accession number.
The GenBank accession number is AF402317.

	RESULTS

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Growth under aerobiosis and anaerobiosis and identification of PepR.
L. sakei was grown both under aerobiosis and anaerobiosis in the chemically defined medium MCD. The growth rates observed were not significantly different as measured by the doubling times (81 ± 3 min under aerobiosis versus 79 ± 2 min under anaerobiosis). The final cell densities reached after 24 h of cultivation were also similar (0.75 to 0.8). Moreover, whatever the anaerobiosis conditions were (nitrogen or carbon dioxide), no growth difference could be observed. This is in accordance with previous data showing that anaerobiosis influenced mainly survival during stationary phase (4).

We compared protein expression under aerobiosis and anaerobiosis. Samples were prepared during exponential growth (OD₆₀₀ = 0.4) and at the beginning of the stationary phase (OD₆₀₀ = 0.7) and subjected to 2-DE. Several variations in protein pattern expression were observed. One major spot strongly affected by anaerobiosis was further studied. It had an apparent molecular weight (MW) of 34,918, and its pI was estimated to be 5.24. This spot was specifically overexpressed in cells grown under anaerobiosis and at the beginning of the stationary phase (Fig. 1). It was present but barely detectable when cells were grown under aerobiosis. In order to obtain a better quantification of these variations, gels were stained with the fluorescent dye Sypro Orange and the signal was quantified. This revealed a 10-fold overexpression in cells grown anaerobically.

View larger version (69K): [in this window] [in a new window]   FIG. 1. Portions of two-dimensional gels showing expression of PepR of L. sakei under aerobiosis (a) and under anaerobiosis (b). The arrows indicate the position of PepR. Proteins were extracted from early-stationary-phase cells.

Cloning and analysis of the pepR gene cluster.
Comparison of the L. helveticus and L. rhamnosus PepR proteins revealed conserved motifs. One of them, GGHHHM, located at positions 267 to 274, as well as the N-terminal sequence of PepR of L. sakei were used to design degenerate primers. A 829-bp fragment was PCR amplified, and the sequence revealed a protein 69 to 75% identical to other PepR proteins known so far and with lesser identities to various peptidases. The PCR fragment was used as a probe in Southern experiments on chromosomal DNA of L. sakei 23K digested with various restriction enzymes. This allowed to identify a 3.3-kb EcoRV fragment hybridizing with the pepR probe. An EcoRV genomic library was constructed in E. coli TG1 by the use of pBluescript SK(+) and screened with the pepR probe. This allowed us to obtain a fragment containing the pepR gene, leading to plasmid pRV416. The gene organization of the fragment is shown in Fig. 2. Five open reading frames (ORFs) were found in this region. PepR of L. sakei is encoded by a 903-bp ORF. The protein is 75.5% identical to PepR of L. rhamnosus. The motif GQSWGG, which corresponds to the active site of prolyl oligopeptidases (23) found in PepR of L. rhamnosus and L. helveticus and also in PepI of Lactobacillus delbrueckii and L. helveticus (6), is also present in L. sakei. The calculated MW is 34,240.28 and the estimated pI is 4.85, in agreement with the experimental values determined on 2-DE gels (see above). A putative ribosome binding site was found 10 nucleotides upstream from the start codon. The pepR gene is followed by an inverted repeat structure (G° = -24 kcal) located 45 nucleotides downstream from the stop codon and resembling a transcription terminator. A 457-bp ORF (labV) was observed starting 338 bp downstream from the stop codon of pepR. labV is 25% identical to laaB, an hypothetical transcriptional regulator of L. sakei (accession number AF115391). It also shares 25% identity with various other transcriptional regulators in different species. A 656-bp ORF (gpm) starts 262 nucleotides downstream from labV and is 30 to 40% identical to various prokaryotic and eukaryotic 2-phosphoglyceromutases (9). In its N-terminal part the encoded protein has the phosphoglycerate mutase family phosphohistidine signature. At 50 nucleotides downstream from the stop codon of gpm, a 291-bp partial ORF showing 25% identity to rbsR of L. sakei (accession number AF115391) and various other transcriptional regulators was observed.

View larger version (7K): [in this window] [in a new window]   FIG. 2. Schematic representation of the pepR encoding region. The insert of plasmid pRV415 and putative transcription terminators are shown.

Transcriptional analysis.
Total RNAs were prepared from cultures grown under aerobiosis and anaerobiosis at the beginning of the stationary phase. Expression of the pepR transcript under these two conditions was measured by Northern analysis (Fig. 3). Using a 830-bp pepR probe, we determined that the pepR gene is expressed as a single 1.27-kb transcript and is 20-fold overexpressed under anaerobiosis. This is in accordance with the estimated size of the pepR gene. From the results of DNA sequence analysis, a transcription terminator might exist 45 bp downstream from the stop codon of pepR. A promoter should thus be present 1.27 kb upstream from the terminator, i.e., in labU. However no obvious promoter sequences were observed in this region, based on the consensus hexamers TTGACA and TATAAT (17), and no TG motif could be observed (36).

View larger version (33K): [in this window] [in a new window]   FIG. 3. Transcriptional analysis of pepR of L. sakei under anaerobiosis (lane a) and under aerobiosis (lane b).

Construction of a pepR mutant and phenotypic analysis.
In order to investigate the involvement of PepR in anaerobic metabolism of L. sakei, a pepR mutant was constructed by single crossover. A 660-bp internal fragment of the pepR gene was PCR amplified and cloned in the pRV300 integrative vector developed for L. sakei, leading to pRV415. A pepR-negative strain (RV4041) was then obtained. This strain was analyzed by 2-DE. The PepR spot was no longer detected (not shown). No other change was observed in the protein pattern of this mutant strain in comparison with the wild-type strain (data non shown). The behavior of the mutant was analyzed under both aerobiosis and anaerobiosis. No difference was observed between the mutant and the wild type regarding growth rates and survival. pepR mutants of L. helveticus (29) and L. rhamnosus (34) have also been constructed. Their growth in MRS or milk were identical to those of the wild type.

We also investigated possible involvement of PepR in protein repair mechanisms by studying growth and survival in the presence of puromycin. This compound is a tRNA analog which leads to the production of misfolded puromycyl-containing peptides. In L. lactis, mutants affected in protein repair mechanisms, such as clpP mutants, are affected in their growth in the presence of 10 µg of puromycin ml^-1 (10). In L. sakei the pepR mutant did not show any clear modification of growth characteristics in the presence of puromycin at concentrations ranging from 1 to 20 µg ml^-1 (data not shown). It also did not show any difference from the wild-type strain in behavior at 37°C.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

 
In this study we identified a peptidase (PepR) of L. sakei which is 10-fold overexpressed when cells are grown under anaerobiosis. We cloned the gene and its surrounding region. We show here that the overexpression of PepR is due to a transcriptional regulation of the pepR gene. This transcriptional regulation (20-fold) is consistent with the 10-fold overexpression of the protein as measured in 2-DE gels. No obvious transcription promoter could be observed, and no classical regulatory motif was detected upstream from pepR. However, the transcriptional promoters of several LAB, including peptidase-encoding genes, showed great variability. Moreover, no information is yet available on sigma factors in L. sakei.

PepR has been identified only in species of the genus Lactobacillus. It has been purified from L. helveticus (29, 33), L. rhamnosus (34), and L. curvatus (18). The encoding genes have been cloned from L. helveticus and L. rhamnosus, but pepR is absent in the Lactococcus lactis IL-1403 genome (3). PepR seems to be highly conserved in lactobacilli (65 to 75% identity).

PepR cleaves Pro-X dipeptides. A putative role in flavor has been proposed for this enzyme, since proline-containing peptides have a bitter taste (see reference 34 and references therein). Mutants with mutations in these genes have been constructed but were not tested for such properties. These pepR mutants did not show a different growth rate in MRS medium or in milk compared to the wild type. Similarly, the L. sakei pepR mutant also did not show any difference in growth rate or survival ability, under neither aerobiosis nor anaerobiosis. The physiological role of PepR is thus still unknown. Nevertheless, to our knowledge, the pepR transcriptional regulation by anaerobiosis observed in L. sakei is the first reported for a peptidase of an LAB. Such an induction has been described only for a peptidase of S. enterica serovar Typhimurium (15). In this species the pepT gene, encoding a tripeptidase, has been shown to be 30-fold induced at the transcriptional level. This induction was mediated by cyclic AMP receptor protein-FNR. However, in the 5' region of pepR in L. sakei, we could not detect a putative Fnr binding site which could explain the transcriptional regulation by anaerobiosis.

Information on regulation of expression of LAB peptidases is scarce. A global analysis of transcriptional regulation of the proteolytic system of Lactococcus lactis was recently done by using promoter fusions with reporter genes (11). Most of the genes were shown to be regulated at the transcriptional level by nitrogen source. In L. rhamnosus, pepX, encoding an X-prolyl dipeptidyl aminopeptidase, has been shown to belong to the glnA glnR operon encoding glutamine synthetase (35). This peptidase was revealed to be regulated differently from other LAB peptidases. Under some conditions, a 7-kb transcript encompassing glnA and pepX was synthesized from the glnR promoter. This transcript was then processed by an RNase. This revealed that both proteolytic and biosynthetic enzymes could be expressed through the same mRNA (35). Recently, six L. helveticus peptidase-encoding genes, including pepR, were expressed in Lactococcus lactis under the control of their own promoters (16). pepD and pepR were the only two peptidases for which no expression in Lactococcus lactis was obtained. This expression could be obtained only under the control of the nisA promoter. It thus seems that their promoters were not recognized in Lactococcus lactis. The anaerobic regulation found for pepR of L. sakei illustrates the diversity in the regulation of peptidase expression in LAB species.

We do not yet possess knowledge on the whole proteolytic system in L. sakei. Only four peptidases have been purified and studied in this species: a general aminopeptidase with broad specificity (25), a dipeptidase with main specificity towards Ala-X peptides and neutral amino acids (21), an X-prolyl dipeptidyl aminotransferase (27), and a tripeptidase with broad specificity against di- or tripeptides (26). Nevertheless, their involvement in growth and physiology or their possible impact on meat technology is not established. Furthermore, a partial ORF encoding a putative dipeptidase has also been reported (GenBank accession number X98238).

Most studies have been focused on the role of peptidases in providing LAB with amino acids. Besides this role, it is clear that peptidases might also be involved in regulatory mechanisms and in breakdown and turnover of proteins. The transcriptional regulation of pepR by anaerobiosis is a new insight in the regulation of expression of LAB peptidases. This study also constitutes the first report of a correlation between transcriptional and proteomic studies in expression of LAB peptidases. As we could not observe any phenotype for the pepR mutant, we cannot exclude the possibility that PepR has a regulatory role in the activity or function of proteins that are not essential for growth or survival or that whatever is the role of PepR, its function is also encoded by another gene.

	ACKNOWLEDGMENTS

 
We thank C. Beauvallet for N-terminal sequencing, A. M. Dudez for DNA sequencing, and V. Davant for technical assistance.

	FOOTNOTES

 
* Corresponding author. Mailing address: Unité Flore Lactique et Environnement Carné, INRA, Domaine de Vilvert, 78 350 Jouy en Josas, France. Phone: 33 (0)1 34 65 22 92. Fax: 33 (0)1 34 65 21 05. E-mail: verges{at}jouy.inra.fr.

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