- Research article
- Open Access
Comparative proteomic analysis of Lactobacillus plantarumfor the identification of key proteins in bile tolerance
© Hamon et al; licensee BioMed Central Ltd. 2011
Received: 15 October 2010
Accepted: 29 March 2011
Published: 29 March 2011
Lactic acid bacteria are commonly marketed as probiotics based on their putative or proven health-promoting effects. These effects are known to be strain specific but the underlying molecular mechanisms remain poorly understood. Therefore, unravelling the determinants behind probiotic features is of particular interest since it would help select strains that stand the best chance of success in clinical trials. Bile tolerance is one of the most crucial properties as it determines the ability of bacteria to survive in the small intestine, and consequently their capacity to play their functional role as probiotics. In this context, the objective of this study was to investigate the natural protein diversity within the Lactobacillus plantarum species with relation to bile tolerance, using comparative proteomics.
Bile tolerance properties of nine L. plantarum strains were studied in vitro. Three of them presenting different bile tolerance levels were selected for comparative proteomic analysis: L. plantarum 299 V (resistant), L. plantarum LC 804 (intermediate) and L. plantarum LC 56 (sensitive). Qualitative and quantitative differences in proteomes were analyzed using two-dimensional electrophoresis (2-DE), tryptic digestion, liquid chromatography-mass spectrometry analysis and database search for protein identification. Among the proteins correlated with differences in the 2-DE patterns of the bacterial strains, 15 have previously been reported to be involved in bile tolerance processes. The effect of a bile exposure on these patterns was investigated, which led to the identification of six proteins that may be key in the bile salt response and adaptation in L. plantarum: two glutathione reductases involved in protection against oxidative injury caused by bile salts, a cyclopropane-fatty-acyl-phospholipid synthase implicated in maintenance of cell envelope integrity, a bile salt hydrolase, an ABC transporter and a F0F1-ATP synthase which participate in the active removal of bile-related stress factors.
These results showed that comparative proteomic analysis can help understand the differential bacterial properties of lactobacilli. In the field of probiotic studies, characteristic proteomic profiles can be identified for individual properties that may serve as bacterial biomarkers for the preliminary selection of strains with the best probiotic potential.
Research efforts are currently underway in order to better understand the host-microbe interactions that occur in the human gastrointestinal (GI) tract [1, 2]. Evidence suggests that the upset of the GI microflora balance underlies many diseases and that therapies often start with the restoration of a healthy balance . In this respect, probiotics (i.e. "live organisms that, when administered in adequate amounts, confer a health benefit on the host" ) are gaining widespread recognition as new prevention strategies or therapies for multiple GI diseases .
Lactic acid bacteria (LAB) are indigenous inhabitants of the human GI tract . They also have a long history of traditional use in many industrial and artisanal plant, meat, and dairy fermentations. Based on their putative or proven health-promoting effects, these bacteria are commonly marketed as probiotics . Some LAB strains have clearly been shown to exert beneficial health effects . However, these effects are known to be strain specific , and the underlying molecular mechanisms remain poorly understood . The level of evidence provided varies greatly depending on studies, and effects associated with most of the marketed products remain unsubstantiated. Current legislations agree to call for scientific substantiation of health claims associated with foods, mainly through well-designed human intervention clinical studies . Therefore, scientific evidence that would help understand the mechanisms behind the activities of probiotics and narrow down the expensive and time-consuming clinical trials to strains that stand the best chance of success are of great interest. Such evidence may include data from epidemiological studies, from in vivo and in vitro trials, as well as from mechanistic, genomic and proteomic studies.
Proteomics plays a pivotal role in linking the genome and the transcriptome to potential biological functions. As far as probiotics are concerned, comparative proteomics can be used in the identification of proteins and proteomic patterns that may one day serve as bacterial biomarkers for probiotic features . Comparison of differentially expressed proteins within the same strain in different conditions have been performed, shedding light on bacterial adaptation factors to GI tract conditions, such as bile [13–16], acidic pH [18, 19], and adhesion to the gut mucosa [20, 21]. On the other hand, 2-DE coupled with mass spectrometry (MS) has been used to analyze bacterial protein polymorphisms and to distinguish between closely related pathogenic organisms [22–25], but this approach has rarely been employed to compare strains based on their probiotic features. We previously reported the first study of this kind which highlighted key proteins involved in the adhesion properties of Lactobacillus plantarum to mucin . Recently, hydrophobicity and cell agglutination properties in Bifidobacterium longum were investigated through the protein patterns of four strains . Both studies focused on cell surface properties related to adhesion. To our knowledge, proteomics has not been used to compare intra-species strains as regards other GI tract adaptation factors.
Yet, the ability to survive exposure to bile is one of the commonly used criteria to select potential probiotic strains, since bile is a major challenge for bacteria entering the GI tract . In addition to affecting membrane characteristics, bile has numerous other effects on bacterial cells including detergent action, DNA damage, acid, oxidative and osmotic stresses . Thus, when it comes to the study of bile stress, the overall bile, oxidative, acid, detergent and salt (BOADS) stresses should be taken into account. Although mechanisms of survival to bile stress are not fully understood, several genes and molecules involved in this process have been indentified in lactobacilli .
The latter remain the most prominent group of probiotic bacteria, despite the increasing use of other genera such as bifidobacteria. Widely studied with regard to numerous properties, they represent a suitable bacterial model. Among the most common species, L. plantarum is part of a number of ethnic as well as commercial probiotic preparations where it has a long history of safe use . In addition, it is an important member of the GI tract microbiota and is a flexible and versatile species with one of the largest genomes known within LAB .
The present paper investigates the natural protein diversity within the L. plantarum species with relation to bile tolerance and subsequent ability to resist GI tract conditions. This investigation is based on the study of the proteomic profiles of three L. plantarum strains selected according to their in vitro bile tolerance properties.
Sources of bacterial strains
Silage of vegetable matter
Human intestinal mucosa
Bile salt tolerance
Effect of bovine bile concentration on the relative growth rates of L. plantarum strains
Relative growth rate* (% μ) with Oxgall concentrations (% [w/v])
97.1 ± 1.4a
96.3 ± 1.2a
93.5 ± 2.9a
91.2 ± 2.3a
93.9 ± 0.8a
94.2 ± 2.0a
89.6 ± 1.7a
85.5 ± 3.0b
81.7 ± 1.0b
80.3 ± 0.6b
80.5 ± 1.8b
79.1 ± 0.9c
78.5 ± 2.2b,c
78.3 ± 0.7b,c
74.5 ± 2.6c
71.6 ± 2.1d
79.1 ± 2.4b,c
76.2 ± 1.1c
72.3 ± 4.3c
66.9 ± 0.5d,e
76.2 ± 1.7c,d
76.6 ± 0.9c
72.8 ± 1.3c
68.4 ± 1.5e
74.1 ± 3.6d
67.9 ± 1.6d
66.3 ± 2.0d
66.5 ± 1.6e
69.6 ± 1.9e
68.9 ± 3.2d
68.1 ± 1.4d
66.8 ± 2.4e
58.2 ± 0.5f
45.5 ± 2.5e
39.4 ± 1.4e
19.9 ± 3.7f
Comparative proteomic analysis of L. plantarumstrains in standard growth conditions
Although the overall inherent protein patterns of the three L. plantarum strains were similar, 90 out of an average of 400 detected protein spots displayed different abundance levels in standard conditions (Additional file 1). The corresponding gel spots were excised and subjected to tryptic digestion followed by liquid chromatography-mass spectrometry (LC-MS) analysis and proteomic database search using Phenyx and OMSSA to elucidate their identity and likely function. Proteins in a total of 80 spots were identified, some of which were found in more than one spot, indicating the presence of protein isoforms. Proteins fell into 13 functional categories, covering most of the biochemical functions encountered in bacterial cells. Sequence alignment analysis focused on the three sequenced L. plantarum strains WCFS1, JDM1 and ATCC 14917 revealed a systematic occurrence of the corresponding genes with high levels of similarity (> 98%, results not shown).
Impact of a 3.6%-Oxgall exposure on specific proteomic patterns putatively related to bile tolerance
Normalized volume with 3.6% Oxgallc)
Variation factor: bile vs. standard conditionsd)
Translation, ribosomal structure and biogenesis
Ribosomal protein S30EA
0.049 ± 0.004
Posttranslational modification, protein turnover, chaperones
α-Small heat shock protein
0.952 ± 0.059
1.008 ± 0.190
0.597 ± 0.082
1.172 ± 0.159
0.744 ± 0.171
27.427 ± 1.216
14.137 ± 0.142
11.931 ± 0.715
ATP-dependent Clp protease
0.360 ± 0.072
0.282 ± 0.020
Energy production and conversion
F0F1 ATP synthase subunit delta
0.243 ± 0.051
0.110 ± 0.012
0.179 ± 0.023
0.011 ± 0.001
0.210 ± 0.008
0.314 ± 0.025
0.148 ± 0.009
Carbohydrate transport and metabolism
0.098 ± 0.005
0.116 ± 0.025
Amino-acid transport and metabolism
Glycine/betaine/carnitine/choline ABC transporter
0.034 ± 0.003
0.081 ± 0.007
Nucleotide transport and metabolism
Bifunctional GMP synthase/glutamine amidotransferase protein
0.039 ± 0.003
0.104 ± 0.009
0.209 ± 0.016
Inorganic ion transport and metabolism
Stress-induced DNA binding protein
0.278 ± 0.026
0.074 ± 0.003
1.212 ± 0.124
0.957 ± 0.077
Cell wall/membrane/envelope biogenesis
Bile salt hydrolase
0.061 ± 0.008
O, D 
0.151 ± 0.010
0.0312 ± 0.002
0.069 ± 0.007
0.046 ± 0.004
0.052 ± 0.001
Bile influence on expression levels of proteins reportedly involved in bile tolerance
Cells were cultured in stressing conditions using 3.6% Oxgall for 14 h (strain 299 V), 16 h (strain LC 804) and 20 h (strain LC 56), which allowed the harvesting of all cells at the early-stationary phase, as in non-stimulating conditions (data not shown). As protein expression is growth-phase dependent, having cells in a comparable physiological state was in fact key in this investigation. Analysis of changes in protein expression during bile salt exposure was focused on the 15 proteins previously reported to play a role in BOADS stress tolerance. Figure 1(D-F) illustrates representative 2-DE patterns for the three strains when cultured with 3.6% Oxgall. While these patterns looked similar to each other, they were quite different from those obtained in standard conditions, suggesting quantitative changes for most of the protein spots observed. Table 3 reports changes in spot intensities between standard and bile stress conditions for the 15 proteins of interest in this study. Thirteen out of the 15 proteins linked to BOADS stress tolerance in previous studies appeared to respond to the presence of bile (absolute value of fold-change factor r > 1.5, as previously described ), suggesting a direct involvement of these proteins in the bile tolerance process of the studied L. plantarum strains. These proteins could be divided into three groups. Three proteins showed higher expression levels in stressing conditions: Hsp1, spot 1 (2.1 ≤ r ≤ 34); Hsp3, spot 4 (1.7 ≤ r ≤ 2.2); and ClpP, spot 77 (1.7 ≤ r ≤ 2.0). Conversely, two other proteins were repressed when challenged with Oxgall: Bsh1, spot 11 (r = -2.6); and ribosomal protein S30EA, spot 62 (r = -3.2). The third group includes eight proteins with modifications in expression levels that depended on strains (OpuA, spot 18; GshR4, spot 19; GshR1, spot 24; GroEL, spot 76; GuaA, spot 80; and AtpH, spot 90) or resulted in a different expression of protein isoforms (Dps, spots 34 and 41; Cfa2, spots 64 and 72). The expression levels of two proteins (Gpd, spot 26; and RfbC, spot 42) however were not impacted following exposure to 3.6% Oxgall (absolute value of variation factor r ≤ 1.5), suggesting a minor role for these in the bile tolerance process of the considered L. plantarum strains.
This paper reports the application of 2-DE and MS analysis to investigate LAB proteins that are key in the bile tolerance process, a major factor when it comes to probiotics adaptation to the GI tract. Although 2-DE has known limitations and only explores part of bacterial proteomes as compared to other gel-less analyses , it is a widely used and affordable technique which proved to be valuable in discriminating strains according to their bacterial features [22–25]. With regard to probiotic research, two previous studies used a similar approach to explore adhesion properties of L. plantarum  and B. longum . However, this is the first time that an attempt is made towards getting a broad picture of bile tolerance at the species level rather than focusing on a single strain.
L. plantarum, a versatile species with marketed probiotic strains, was chosen as a model for this study. An in vitro test was used to assess bile tolerance of nine strains, including L. plantarum 299 V, a probiotic with outstanding bile resistance properties . These properties were confirmed in our study, as this strain showed the best ability to grow in bile supplemented culture broths. Considerable variations in growth rates were observed between strains, with the highest effect of bile on L. plantarum LC 56, which is in accordance with previous reports showing a strain-specific behavior of LAB with regard to bile tolerance [33, 34]. Strains LC 56 (weak bile tolerance), LC 804 (intermediate bile tolerance) and 299 V (strong bile tolerance) were selected for the proteomic investigation. For that purpose, we focused on the whole cell proteomes, since the ability of an organism to tolerate bile may require a wide array of proteins implicated in either membrane- or cytosol-based functions and mechanisms .
The differentially expressed proteins among the three selected strains cultured in standard conditions all appeared to be encoded by highly conserved genes in the L. plantarum species. These core-genome proteins are of great interest in the search for bacterial biomarkers as their relative abundance is likely to be assessed for any L. plantarum strain. In our case, 10 proteins displayed increasing levels of expression from the sensitive strain (LC 56) to the resistant one (299 V), suggesting a positive correlation of these proteins with bile resistance. Conversely, 4 proteins showed decreasing levels of expression as the considered strain was more tolerant to bile, indicating a link with bile sensitivity. Therefore, these proteins might represent potential biomarker candidates of bile tolerance in L. plantarum and should be further studied, especially the ones with unknown functions (protein of unknown function lp_2652, spot 31; putative alkaline shock proteins 1 and 2, spots 3 and 2 respectively).
Particular interest was in differentially expressed proteins with a reported putative involvement, not specifically in bile tolerance, but in the overall BOADS stress tolerance, since the deleterious effects of bile not only include a detergent action, but also low-pH, oxidative and osmotic stresses . This led to the identification of 15 proteins likely to be implicated in bile tolerance of the selected strains. Two of these proteins (GuaA and ribosomal protein S30EA) have previously been negatively correlated to constitutive acid  and bile  tolerance, respectively, suggesting they could impart bacterial sensitivity to theses stress factors. Interestingly, they were not detected (ribosomal protein S30EA) or naturally underexpressed (GuaA) in the resistant strain. On the other hand, the 13 remaining proteins have been linked to BOADS stress resistance in previous studies. Ten of them were overexpressed in the resistant or intermediate strains, while only one of them displayed higher expression levels in the bile sensitive strain. These results showed that the natural protein diversity observed among L. plantarum strains cultured in standard conditions can reflect their ability to tolerate bile. The more resistant a strain is to bile, the more it naturally expresses proteins that can help in the bile resistance process, but also the less it produces proteins that may impart sensitivity to this stress. These proteins could therefore constitute an inherent and characteristic proteomic profile that is indicative of bile tolerance.
To confirm the putative involvement of the 15 proteins of interest in the bile tolerance process and get an overview on how bile salts affect their levels of expression, proteomic analysis of strains response to bile exposure was performed. Thirteen proteins appeared to be directly implicated in bile stress adaptation, since their expression was significantly affected by exposure to bile salt (p < 0.05). Five of them (ClpP, Dps, GroEL, Hsp1, and Hsp3) are general stress-response proteins involved in repair and protection of proteins and DNA. They were up-regulated in response to bile challenge, which is in accordance with previous findings [14, 16, 36–38]. This set of proteins intervenes in numerous stress-management response systems, suggesting they have unspecific contributions to bile stress tolerance, which may result in multifaceted stress-dependent mechanisms of action, as this was recently reviewed for Dps . Two other proteins (GuaA and ribosomal protein S30EA) are part of regulatory systems modulating protein translation during environmental stresses. GuaA, involved in guanine nucleotide metabolism, indirectly governs intracellular GTP level responsible for translation efficiency , while ribosomal protein S30EA limits protein synthesis by reducing translation initiation . Both proteins were down-regulated in the sensitive strain following bile exposure, which is consistent with previous studies [14, 38]. All in all, 7 out of the 13 proteins directly involved in bile tolerance of the three-selected L. plantarum strains were not dedicated to one of the damaging effects of bile, but covered a wide range of environmental stresses instead.
In contrast, other factors contribute in a specific way to bile tolerance. This is the case of GshR1 and GshR4 which help protect the cell against oxidative injury . This coincides with the lower global levels of glutathione reductases in the sensitive strain in both standard and stimulating conditions found in our study. Another protein, the Cfa2, catalyzes the cyclopropane ring formation in phospholipid biosynthesis, which may help maintain integrity of the cell envelope. In Escherichia coli, the cytoplasmic membrane of a cfa-mutant displayed increased overall permeability to protons compared to the native strain . This could for instance explain the higher acid sensitivity of a cfa-mutant of L. acidophilus NCFM . In our study, a Cfa2 isoform was absent in the sensitive strain, while another isoform was not detected in the resistant one, suggesting different functional properties of the isoforms with regard to bile tolerance.
Another specific mechanism of bile adaptation is the active removal of bile-related stress factors. Such is the case of the F0F1-ATP synthases which facilitate the extrusion of protons from the cytoplasm by proton motive force . Previous findings reported that a bile-adapted B. animalis strain was able to tolerate bile by inducing proton pumping by a F0F1-ATP synthase, therefore tightly regulating the internal pH . In our study, a representative F0F1-ATP synthase, AtpH, was absent in the weak strain and was up-regulated in the intermediate strain, which is consistent with the up-regulation of the corresponding gene reported for L. plantarum WCFS1 when exposed to porcine bile . ABC transporters are also a major part of the efflux systems involved in the transport of harmful-compounds and cell detoxification . A representative ABC transporter, OpuA, was more abundant in the resistant strain, less abundant in the intermediate one, and not detected in the sensitive one. This protein is known to be implied in the L. plantarum response to osmotic stress, one of the numerous deleterious effects of bile . In addition, deletion of an opuA gene in Listeria monocytogenes was shown to significantly increase bacterial sensitivity to physiological concentrations of human bile . This protein is therefore likely to be a key determinant of the high bile resistance of strain 299 V.
When it comes to bile tolerance, Bsh is probably what first comes to mind, since it involves the direct hydrolysis of bile salts. Although the ecological significance of microbial Bsh activity is not yet fully understood, the suggestion was made that it may play a major detoxification role . L. plantarum strains carry four bsh genes (bsh1 to bsh4). Bsh2, bsh3 and bsh4 are highly conserved among L. plantarum species, while bsh1 is not and seems to be the major determinant of the global Bsh activity of L. plantarum strains. Besides, a bsh1-mutant of L. plantarum WCFS1 displayed a decreased tolerance to glycine-conjugated bile salts . In our study, a Bsh1 homologue could only be found in the most resistant strain in standard conditions, but its amount decreased following the strain's exposure to bile. This result contrasts with the bsh1 gene up-regulation in L. plantarum WCFS1 following bile challenge . Strains from L. acidophilus and L. salivarius on the other hand did not seem to up-regulate their Bsh1 production following bile exposure [38, 50]. Such discrepancy in regulation trends of bsh genes suggests that, depending on the considered strains and species, Bsh activity may or may not be a major determinant of bile resistance.
Finally, it appeared that the six bile tolerance factors described above may contribute in various ways to the bile tolerance of L. plantarum strains. In particular, strains appeared to regulate key proteins differently following exposure to bile, which suggests that several strategies coexist in the bile adaptation process of L. plantarum species, some strains favoring certain specific pathways, while others downplaying them.
This work used comparative and functional proteomics to analyze cell-free protein extracts from three L. plantarum strains with different bile resistance properties. This approach showed that the natural protein diversity among L. plantarum strains cultured in standard conditions can reflect their ability to tolerate bile. The results provided an overview of proteomic patterns related to bile tolerance, and showed a clear effect of bile salts on the level of expression of certain proteins within these patterns. Particularly, 13 out of the 15 proteins of interest were shown to be directly involved in the bile tolerance of L. plantarum, six of which could be part of specific bile adaptation pathways, including protection against oxidative stress (GshR1 and GshR4), maintenance of cell envelope integrity (Cfa2), and active removal of bile-related stress factors (Bsh1, OpuA, and AtpH). Also, analysis of changes in protein expression gave insight into the way the different strains use these pathways for their survival, suggesting complex, strain-specific and probably conflicting molecular mechanisms in the cell's adaptation strategy to bile.
Finally, this study showed that comparative proteomic analysis can help understand the differential bacterial properties of LAB. In the field of probiotic studies, characteristic proteomic profiles can be identified for individual properties which may serve as bacterial biomarkers for the preliminary selection of strains with the best probiotic potential. This would certainly increase the chances of success of clinical trials through a more focused approach.
Strain characterization and standard culture conditions
Lactobacillus strains used in this study were identified at the species level by recA PCR (data not shown) . All cultures were maintained as frozen stocks held at -80°C in Cryobank cryogenic beads (Bio-Rad, Hercules, CA, USA). For experimental use, strains were cultured anaerobically (Anaerocult A system, Merck, Darmstadt, Germany) at 37°C in Man-Rogosa-Sharpe broth (Biokar, Beauvais, France) supplemented with 0.05% (w/v) L-cysteine hydrochloride monohydrate (MRSC; Merck) to early stationary phase, using three successive subcultures (1% v/v inoculation; 12-15 h).
Bile salt tolerance
Tolerance to bile was assessed by investigating the ability of strains to grow in the presence of different concentrations of bovine bile (Oxgall, Sigma-Aldrich, St Louis, MO, USA), as previously described . Fresh cultures were inoculated (0.1%, v/v) into MRSC broth containing 0.5%, 1.0%, 1.8%, and 3.6% (w/v) Oxgall and incubated anaerobically at 37°C. Bacterial growth was monitored in honeycomb plates (Oy Growth Curves AB, Helsinki, Finland) by measuring the optical density at 600 nm (OD600) every 30 min for 48 h using an automated turbidimetric system (Bioscreen C MBR, Oy Growth Curves AB). Three independent experiments were carried out and each assay was performed in triplicate. Comparison of cultures was based on their growth rates in each broth, expressed as a percentage of that of the control which was assigned a value of 100% . Using Statgraphics plus 5.1 software (Manugistics, Rockville, MD, USA), data were subjected to two-way ANOVA with strain and bile concentration as variables. Multiple comparison test using least significant difference procedure was carried out to compare means for which the ANOVA test indicated significant mean differences (p < 0.05).
Whole cell protein extraction
The following experiments (including 2-DE) were performed for bacterial cells cultured in two different broths (MRSC and MRSC supplemented with 3.6% Oxgall). Early stationary phase cells from a 10-mL broth culture were harvested and washed three times with phosphate-buffered saline (PBS). Cell pellets were resuspended in 2 mL of PBS and cryobeads of these suspensions were prepared in liquid nitrogen. The bacterial beads were ground in liquid nitrogen using a cryogenic grinder (6870 Freezer/Mill, Spex CertiPrep, Stanmore, UK) with three steps of 3 min at a rate of 24 impacts/s. After sample centrifugation (5000 g for 5 min, 4°C), supernatants were filtered through a 0.45-μm pore size filter (Chromafil PET; Macherey-Nagel, Düren, Germany). Protein purification was carried out with Trizol reagent (Euromedex, Souffelweyersheim, France) as previously described . Protein concentrations were determined using Bradford protein assay (Bio-Rad) according to the manufacturer's instructions.
Protein extracts (150 μg) were loaded onto 17-cm strips with a pH range of 4 to 7 (Bio-Rad), focused for 60,000 V.h, and then separated on a 12% SDS-polyacrylamide gel as reported previously . The gels were stained with Bio-Safe Coomassie (Bio-Rad) and scanned on a GS-800 Calibrated Densitometer (Bio-Rad).
Image analysis of the 2-DE gels was performed using the PD Quest 8.0.1 software (Bio-Rad). Three gels were produced from independent cultures of each strain and only spots that were present on the three gels were selected for inter-strain comparison. Spot intensities were normalized to the sum of intensities of all valid spots in one gel. For analysis of changes in protein expression during bile salt exposure, a protein was considered to be under- or overproduced when changes in normalized spot intensities were of least 1.5-fold at a significance level of p < 0.05 (Student's t test for paired samples), as previously described . Regarding proteome comparison between strains, proteins were considered differentially produced when spot intensities passed the threshold of a twofold difference (one-way ANOVA, p-value < 0.05), as described previously .
Spots of interest were subjected to tryptic in-gel digestion and analyzed by chip-liquid chromatography-quadrupole time of flight (chip-LC-QTOF) using an Agilent G6510A QTOF mass spectrometer equipped with an Agilent 1200 Nano LC system and an Agilent HPLC Chip Cube, G4240A (Agilent Technologies, Santa Clara, CA, USA), as described previously .
Briefly, one microliter of sample was injected using an injection loop of 8 μL, a loading flow rate of 3 μL/min for 4 min and a solvent made of ultra-pure water and acetonitrile (HPLC-S gradient grade, Biosolve, Valkenswaard, The Netherlands) (97/3 v/v) with 0.1% formic acid (98-100%, Merck). For the analytical elution, a 24 min gradient from 3 to 60% of acetonitrile in ultra-pure water with 0.1% formic acid was applied at a flow rate of 300 nL/min. ESI in positive mode with 1850 capillary voltage was used. The data were collected in centroid mode using extended dynamic range at mass range of m/z 200-2000 both in MS1 and MS/MS and using two method with different scanning speed: one slow with a scan rate of 1 spectra/s for both MS1 and MS/MS, and one fast scan rate of 0.25 spectra/s for both MS1 and MS/MS. For data acquisition and data export, MassHunter version B.02.0.197.0 (Agilent Technologies) was used.
After data acquisition, files were uploaded to the in-house installed version of Phenyx (Geneva Bioinformatics, Geneva, Switzerland) for searching the NCBInr (r. 20090608) database with the following criteria: taxonomy: bacteria; scoring model: ESI-QTOF; parent charge: +2, +3 (trust = medium); single round; methionine oxidation, cysteine carboxyamidomethylation (cysteine treated with iodoacetamide), and phosphorylation as partial modifications; trypsin as digestion enzyme; allowance of two missed cleavages; cleavage mode: normal; parent ion tolerance: 0.6 Da; peptide thresholds: length ≥6, score threshold ≥5.0, identification significance p-value ≤ 1.0E-4, accession number score threshold 6.0, coverage threshold ≥0.2, identified ion series: b; b++;y; y++; allowance of conflict resolution. A publicly available MS/MS search algorithm (Open Mass Spectrometry Search Algorithm, OMSSA, ) was used with the same search criteria as described above to confirm protein identities and limit the risk of false positives. On the basis of consensus scoring, only proteins recognized by both database search algorithms at a false positive rate of 5% were considered to be correctly identified .
This work was supported by the ''Ministère de l'Enseignement Supérieur et de la Recherche'', and by the ''Ministère de l'Agriculture et de la Pêche'' through the ''Unité Mixte Technologique 06.03: Méthodes analytiques et nutrimarqueurs''.
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