Lactic Acid Bacteria Isolation from Spontaneous Sourdough and Their Characterization Including Antimicrobial and Antifungal Properties Evaluation

This research effort aimed at isolating and phenotypically characterizing lactic acid bacteria (LAB) isolates from a spontaneous rye sourdough manufactured following traditional protocols, as well as at evaluating their antimicrobial and antifungal properties as key features for future industrial applications. Thirteen LAB strains of potential industrial interest were isolated and identified to species-level via PCR. Most of the sourdough isolates showed versatile carbohydrate metabolisms. The Leuconostoc mesenteroides No. 242 and Lactobacillus brevis No. 173 demonstrated to be gas producers; thus, revealing their heterofermenter or facultative homofermenter features. Viable counts higher than 7.0 log10 (CFU/mL) were observed for Lactobacillus paracasei No. 244, Lactobacillus casei No. 210, L. brevis No. 173, Lactobacillus farraginis No. 206, Pediococcus pentosaceus No. 183, Lactobacillus uvarum No. 245 and Lactobacillus plantarum No. 135 strains, after exposure at pH 2.5 for 2 h. Moreover, L. plantarum No. 122, L. casei No. 210, Lactobacillus curvatus No. 51, L. paracasei No. 244, and L. coryniformins No. 71 showed growth inhibition properties against all the tested fifteen pathogenic strains. Finally, all LAB isolates showed antifungal activities against Aspergillus nidulans, Penicillium funiculosum, and Fusarium poae. These results unveiled the exceptionality of spontaneous sourdough as a source of LAB with effective potential to be considered in the design of novel commercial microbial single/mixed starter cultures, intended for application in a wide range of agri-food industries, where the antimicrobial and antifungal properties are often sought and necessary. In addition, metabolites therefrom may also be considered as important functional and bioactive compounds with high potential to be employed in food and feed, as well as cosmetic and pharmaceutical applications.


Spontaneous Rye Sourdough Preparation and Sampling
Spontaneous rye sourdough was prepared by using the following procedure. Rye flour (100 g) was mixed with 150 mL of tap water (at room temperature), 1 mL acetic acid (1%, v/v), and NaCl (1%, v/v) was added till pH 4.0, and kneaded by hand during 5 min-thus giving rise to a dough yield (DY) of 250, i.e., the dough to flour weight ratio × 100 (which correlates with water activity. Resulting dough was allowed to stand for fermentation during 48 h at 30 • C in a thermostat (Memmert GmbH, Schwabach, Germany) followed by the addition of 50 g rye flour and 50 mL tap water (DY = 233.3). Finally, the fermentation was continued for an additional of 24 h at 30 • C. Aliquots of the resulting sourdough were used for in the microbiological analysis towards LAB isolation.

Culture Media and Microbiological Growth and Enumeration
For the enumeration and isolation of LAB de Man, Rogosa and Sharp agar (MRS) was purchased from Biolife (Milan, Italy). The culture medium was supplemented with cycloheximide (Sigma-Aldrich (Taufkirchen, Germany) to prevent growth of yeasts and molds. The pH of the culture media was adjusted to the desired value of 6.4 ± 0.2 at 25 • C. The culture media was further autoclaved after previous dissolution, under stirring, to boiling point 121 • C. The media was cooled to 50 • C and the non-thermostable cycloheximide was aseptically added to the culture media through a 0.22-µm membrane filter (Whatman, Maidstone, UK) and stirred. Duplicates of 10 g-samples of sourdough were suspended in 90 mL of sterile 2% (w/v) NaCl solution (Sigma-Aldrich (Taufkirchen, Germany), aseptically homogenized in a homogenizer (Bosch GmbH, Stuttgart, Germany) till pure consistency. The results were expressed as log of colony-forming units (CFU) per gram of sample. The logarithmic transformation was necessary for stabilization of variance and normalization of residuals. Analysis was performed according to method described by Bartkiene et al. [25].

Isolation, Atype Identification of Sourdough Lactic Acid Bacteria Strains
The 16S rDNA sequencing was conducted by applying the primer set [Bak4 (5'-AGG AGG TGA TCC ARC CGC A-3'); Bak11 (5'-AGT ATTG ATC MTG GCT CAG-3')] and the PCR protocol as described by Di Cello et al. [28]. The RAPD PCR products were separated with agarose (2%, w/v) electrophoresis. The molecular fingerprinting of the all final strains was also done by rep-typing with the primer (GTG) 5 (5 -GTG GTG GTG GTG GTG-3 ). The PCR products were purified applying the peqGold Cycle-Pure Kit (Peqlab Biotechnology GmbH, Erlangen, Germany) and sequenced (Eurofins MWG Operon, Ebersberg, Germany). The received sequences were analyzed with the BLASTn tool (http://blast.ncbi.nlm.nih.gov), and a minimum sequence identity of 98% was chosen as the criterion for species identification. The PCR-based identification of the genus and species was performed according to the references given in Table 1. Table 1. Primer details of PCR-based identification of LAB at genus and species level.

Genus and Species
References Primers Used (Fw = Forward; Re = Reverse) Size (pb)

Phenotype Characterization of the Isolated Sourdough Lactic Acid Bacteria Strains
The metabolism of several carbohydrates by sourdough LAB strains was determined by using API 50 CHL galleries (BioMérieux, Marcy-l'Etoile, France) according to the manufacturer instructions. Gas production was detected by Durham tube method [37] in MRS broth (Biolife, Milan, Italy) for 24 h at 30 • C. The growth performance of strains was monitored at 10, 30, 37 and 45 • C for 24 h in an MRS broth using a Thermo Bioscreen C automatic turbidometer (Labsystems, Helsinki, Finland). The viability of the isolated strains to grow in acidic environments was evaluated in MRS broth acidified to a final pH of 2.5 with HCl (Biolife, Milan, Italy) in tubes, according to Lee et al. [38]. Total viable counts were determined by using standard plate count techniques [39]. The results were expressed as log of colony-forming units (CFU) per milliliter. All phenotype analyses were carried out in triplicate.  [40,41].

Antimicrobial Activity
The tested LAB strains were inoculated in MRS broth (Biolife, Milan, Italy) and incubated at 30 • C for 24 h. After incubation, 2 mL of the MRS broth (v/v), in which the LAB strains were multiplied, were inoculated into fresh MRS broth (Biolife, Milan, Italy) and propagated at 30 • C for 18 h. Afterwards, the multiplied LAB were used for the determination of their antimicrobial activities against the pathogenic and opportunistic bacterial strains listed above.
The agar well diffusion assay was used for the antimicrobial activity testing of the LAB supernatants (supernatant sample was adjusted to pH 6.5 with 1 M NaOH to eliminate the organic acid). Analysis was performed according to method described by Bartkiene et al. [16]. In addition, ability of LAB to inhibit pathogens in liquid medium was evaluated. With this aim, 0.1 mL of pathogens (previously suspended in physiological solution up to 0.5 McFarland Units) were transferred in tubes with 4.4 mL Mueller Hinton Broth (Oxoid, Basingstoke, UK) and afterwards 0.5 mL of LAB suspension (8.56 log 10 CFU/mL) was added. The same procedure was performed using 1.0 mL of LAB with the aim to test two different LAB concentrations. Tubes were incubated for 48 h at +35 • C. The results were evaluated according to the presence/absence of visible growth. Experiments were performed in triplicate.

Evaluation of Antifungal Activity of the Isolated Sourdough Lactic Acid Bacteria
The antifungal activities of the LAB were determined against seven different species, viz. Aspergillus fischeri, Aspergillus nidulans, Penicillium oxalicum, Penicillium funiculosum, Fusarium poae, Alternaria alternata and Fusarium graminearum. These molds were previously isolated from grain-based food and were provided by the collection of the Lithuanian University of Health Sciences (Kaunas, Lithuania). All these microorganisms were cultivated on yeast extract, peptone and dextrose (YEPD) agar medium at 25 • C, in the thermostat for 5 days. The antifungal activity of LAB strains was tested by the agar well diffusion assay [41].

Statistical Analysis
The results were expressed as the mean (n = 3) ± standard deviation. Non-parametric Kruskal Wallis test followed by Dunn's post hoc tests were used for data analysis. p ≤ 0.05 was considered statistically significant. Statistics were performed with SPSS for Windows XP V15.0 (SPSS, Inc., Chicago, IL, USA, 2007).
Metabolic activity and microbial stability are key factors to ensure reproducibility between batches; therefore, to ensure the quality of sourdough bread and/or any other fermentation process that resorts to mother-dough (or sour ferment) or to microorganisms isolated therefrom as microbial starter culture. However, the microbial profile and microbial dynamic found in the sourdough depends largely on the ecological/environment conditions prevailing throughout time, from the preparation of the baking dough until the end of the fermentation process. Spontaneous sourdough fermentation and the employed environmental conditions plays a major effect upon the various microbial groups and species prevailing at the end of such a fermentative process. In a developed sourdough, only some species well-adapted to the rigid environmental conditions, prevailing during fermentation (i.e., low temperatures, high relative humidity, high total titratable acidity; presence of different antimicrobial and antioxidant metabolites, etc), became dominant. In fact, the competitive and synergetic consortia of acid tolerant yeasts and LAB usually reach rapidly viable counts above those of the adventitious microbiota initially present in the flour or flours. Nevertheless, other ubiquitous microorganisms present in the flours are likely to stay viable in some sourdoughs [1][2][3][4]10]. Previous researchers have shown that microbial diversity in sourdoughs can varied according to different geographic location [43]. It was published that Weissella cibaria and Lactobacillus sanfranciscensis were predominant in the microbiota of jiaozi and type I sourdoughs, respectively [44]. In Japan different species of LAB such as Lactobacillus brevis, Lactobacillus alimentarius, Lactobacillus pentosus, Lactobacillus vaccinostercus, Lactobacillus sanfranciscensis, and Lactobacillus sakei were detected, as well as the yeasts primarily included Saccharomyces cerevisiae, with Candida humilis in some samples [45]. Also, Chinese traditional sourdoughs from different regions were studied, and the results showed that the West group was significantly different from the North and South groups in the dominant genera (mainly Lactobacillus, Pediococcus, and Leuconostoc) [46]. About the LAB diversity of wheat sourdoughs collected in Ya'an city was published, from which two hundred nineteen LAB strains were isolated, and genotypic characterization indicated that the isolated LAB strains included Lactobacillus plantarum, L. pantheris, Leuconostoc citreum, Weissella viridescens, Leu. pseudomesenteroides, Lactococcus lactis, L. raffinolactis, and Leu. mesenteroides [47]. Study about the microbial diversity of the traditional Chinese sourdough showed that the predominant microbes in sourdough were Lactobacillus, Pediococcus, and Wickerhamomyces [48]. In spontaneous fermented chia sourdough, besides among identified LAB by culture-dependent approach, species from genus Enterococcus were the most abundant, as well as Lactococcus (Lc. lactis), Lactobacillus (L. rhamnosus), and Weissella (W. cibaria) species were also isolated [49]. In sourdough, as well as maize and rye flours from several geographic locations in Portugal predominant yeasts were Saccharomyces cerevisiae and Candida pelliculosa, as well as the most frequently isolated LAB were (heterofermentative) Leuconostoc spp. and (homofermentative) Lactobacillus spp.; L. brevis, L. curvatus, and L. lactis ssp. lactis for the Lactobacillus genera; Lactococcus lactis ssp. lactis for lactococci; Enterococcus casseliflavus, E. durans, and E. faecium for enterococci; and Streptococcus constellantus and S. equinus for streptococci [10]. Finally, sourdough has a complex microbiota that is affected by multiple factors including factors related to cereal plants, grains, and sourdough processing techniques [9].
Furthermore, during prolonged fermentation processes the variety of LAB (and other) strains tends to the greatly reduced: from several LAB species initially contained in a dough, only a few become dominant and viable at the end. Furthermore, LAB species, which do not remain viable in sourdough during the high temperatures employed during the baking processes, exhibit unique desirable technological, antimicrobial, antifungal, probiotic, biodegradation, absorption and adsorption properties, among others. Based on the above description, the isolation of the sourdough LAB in the first stages of fermentation (where higher microbial diversity is found) can prove to be very promising for the industries with special needs for microorganism with such antimicrobial, antifungal and other abilities. For this reason, all the isolated thirteen LAB strains were used for the further analysis, so as a maximum diversity of strains could be guaranteed.

Carbohydrate Metabolism, Gas Production, and Viability and Growth Performance at Different Temperatures and Low pH Values of Sourdough Isolates
The carbohydrate metabolism, gas production, tolerance to temperature and low pH conditions of the LAB isolated from sourdough are shown in Table 3. The carbohydrate metabolism was studied for 47 different carbon sources ( Table 3) Conversion of carbohydrates into lactic and acetic acids by LAB is one of the most important fermentation processes employed in cereal-based products technologies. With the advent of pure (commercial) starter cultures for fermentation processes, it became possible to control more effectively the microbial metabolic activities and the fermentation process as a whole and, consequently, to improve food quality and safety, as well as to enhance the extending of its use to novel and a large number of biotechnological processes. The experimental information on LAB carbohydrate metabolism, as depicted in Table 3, is of utmost importance to accurately evaluate and modelling the dynamics of single/co-culture fermentations and to optimize their environmental and growth conditions to improve technological, nutritional and health attributes [16,50].                Table 3. Carbohydrate metabolism, gas production, tolerance to temperature (10, 30, 37 and 45 • C) and low pH conditions (pH 2.5 for 2 h) of the isolated sourdough lactic acid bacteria (LAB) strains.  According to the carbohydrate metabolic pathways, LAB can be classified into homofermentative, facultative homofermentative or obligate heterofermentative. Depending on the type of species and strains belonging to the LAB group, they can metabolize carbohydrates into different metabolites, chiefly: Pediococcus and Lactobacillus (homofermentative) to DL or L(+) lactic acid (depending on the species, Lactobacillus can be homofermenters or facultative or obligate heterofermenters), Leuconostoc (obligate heterofermentative) to CO 2 , acetate, and D(−) lactic acid. However, it should be emphasized that the metabolic pathways for carbohydrates can be changed by the same microbial strain throughout time, depending on the environment and growth conditions, for instance during the depletion of certain substrates and the production of metabolites that became substrates to the others throughout a batch or fed-batch fermentation-thus making difficult the full elucidation and control of metabolic pathways. As examples, the metabolic pathways will depend in the complexity of the growth medium, temperature, time, water activity, and acidity, interactions between microorganisms in co-culture starters or natural sourdough systems, among many other variables [1][2][3][4]10]. Yet and particularly, when complex substrates (containing other substrates rather than the fermentable hexoses) are present in a growth medium, its fermentation may yield organic acids, acetate and CO 2 at distinct ratios-which is very often to occur in industrial processes. Finally, most of the sourdough LAB strains in the present investigation exhibited versatile carbohydrate metabolisms-thus envisaging high potential attributes for their application in industry, for example in many fermentation processes or to be employed in recovery technologies intended for the valorization of by-products, residues and agri-food wastes resulting from the agriculture or industry.
According to the results (Table 3), from the 13 isolated sourdough LAB strains, gas production was detected in only two, viz. Leu. mesenteroides No. 242 and L. brevis (Group III lactobacilli). Such findings are in agreement with the expected results since both species are known to be obligate heterofermenters.
Analysis of the growth performance of the isolated sourdough LAB at different temperatures (Table 3) revealed that only the L. casei No. 210 strain was able to display weak growth (+) at the lowest temperature (10 • C). The activity at low temperatures is an important characteristic, since the microbial growth may be desirable or, inversely, undesirable depending on the application on demand. As example, during the storage of semi-fluid (type I and II sourdoughs) or other non-freeze-dried starter cultures, low or absence of growth activities are desirable. Conversely, it becomes undesirable when the intent is the bioconversion of materials or compounds in processes undertaken in low temperature regimes.
With respect to the ability of selected sourdough LAB to grow under acidic environments, the highest concentration of viable cells after 2 h incubation at pH 2.5 was found to L. paracasei No. 244 (9.29 ± 0.1 log 10 CFU/mL). Good microbial viability at low pH was observed for L. casei No. 210, L. brevis No. 173, and L. farraginis No. 206 strains-for which the concentration was higher than 8.0 log 10 (CFU/mL), whereas viable counts higher than 7.0 log 10 (CFU/mL) was found for P. pentosaceus No. 183, L. uvarum No. 245, and L. plantarum No. 135 strains after 2 h incubation at pH 2.5. Other isolated LAB strains showed significantly lower tolerance to the same acidic conditions, with values lower than 6.0 log 10 (CFU/mL), or even absence of growth in the case of L. coryniformins No. 71. It is generally accepted that an isolate with full tolerance to pH 3.0 for 3 h can be considered as high-acid-resistant strain with promising probiotic properties [51,52].
In the event of microorganisms belonging to the LAB group, acid stress is a self-imposed condition, once lactic acid is the major end-product of carbohydrate metabolism and plays a major role in their competitiveness as antimicrobial agents against other microorganisms [36].
Low pH values damage both the cell wall and cell membrane; thus, influencing the membrane potential, which leads to undesirable metabolic processes, energy depletion and, eventually, to cell death [4]. Adaptation of the LAB to low pH conditions depends on their phenotype characteristics and the environmental conditions, in which cells are transiently exposed to mild nonlethal stress conditions, which, in turn, drive to an increased survival ability after a subsequent lethal challenge to the same stress [53]. The molecular mechanisms underlying transient adaptation and habituation to a specific stress may overlap to a certain degree, but they are not completely identical [53][54][55]. This may explain a number of contradictory results reported for some LAB species [56,57].

Antimicrobial Activity of the Isolated Lactic Acid Bacteria Strains
Diameter inhibition zones (DIZ) of the sourdough LAB strains against pathogenic and opportunistic microorganisms are shown in Figure 1a-c. We observed inhibition properties against all the tested fifteen pathogenic and opportunistic bacterial strains by L.    No. 242 and L. curvatus No. 51 inhibited 13 of the 15 analyzed pathogenic strains, whereas the lowest antimicrobial activity was observed for L. brevis No. 173-which inhibited 7 of the 15 analyzed pathogenic bacterial strains. When increasing the level of sourdough LAB inoculum (i.e., 1.0 mL sourdough LAB + 0.1 mL pathogen), most of the strains unfolded the capacity to inhibit a broader spectrum of pathogens ( Figure 2). However, increased concentration of P. pentosaceus No. 183 proved to be still not effective enough to inhibit MRSA.    The selection of appropriate LAB strains intended for in situ production of antimicrobial compounds by fermentation and the application of the purified states of such metabolites as biological food preservatives in sectors as large as food and feeds, nutraceuticals (dietary supplements and food additives), cosmetics and pharmaceuticals, is very promising.
The preservative effect of fermented products is mainly due to the acidic conditions, which are formed during LAB conversion of carbohydrates into organic acids; chiefly, lactic and acetic acids. The acidification is not exclusive to LAB, but other microorganisms may also be mostly involved in the acidification of fermentation food products, such as the group of acetic acid bacteria producers (from the Acetobacter species). Yet, the inhibitory action of LAB is not limited to lactic and acetic acids and a wide range of other metabolites excreted to the growth medium may possess antagonistic properties against several prokaryotic bacteria and/or eukaryotic yeasts and molds. As already cited, among those metabolites are formic acid, free fatty acids, ammonia, ethanol, hydrogen peroxide, diacetyl, acetoin, 2,3-butanediol, acetaldehyde, benzoate, bacteriolytic enzymes, bacteriocins and BLIS, as well as several other less known inhibitory substances [1,3,4,10,41,[58][59][60][61][62][63][64]. Furthermore, the antimicrobial effect of LAB can also be significantly influenced by numerous physical, chemical and nutritional environmental factors [65,66].
Under this context, sourdough LAB isolated in this research work could be used to design specific starter cultures or to produce antimicrobial metabolites (among many other commercially high-added value compounds). Actually, the applications of LAB individually or as co-cultures in the prevention of bacterial and mold food spoilage represent major challenges to the industry. As a matter of fact, the production of industrial single/mixed starter cultures still needs further and deep investigations to address the incipient existing knowledge concerning the metabolic activity and microbial dynamic in such complex biological systems, but also to find innovative solutions to the actual technological demands. Further and deeper research is also needed to produce starters with novel properties and solve limitations such as metabolic activity and microbial stability, susceptibility to bacteriophage infections, spontaneous mutations or loss of key-physiological properties and sensorial acceptance by consumers. Particularly, the development of sourdough starter cultures for bread making is very topical due to the need to avoid deviations in bread quality between batches as frequently observed when the laborious and time-consuming artisanal procedures based on spontaneous sourdough fermentation are employed. In these artisanal processes, a piece of the spontaneously fermented dough, called mother-dough or sponge-dough, is kept aside and added to dough in next fermentation batch, thus serving as a natural ferment or microbial starter culture. In addition to the previous benefits, the use of starter cultures in bread making and other fermented food may be of interest to attain several other advantages, such as the reduction of production costs, fermentation times and risk of spoilage, to increase shelf-life, to predict microbial metabolic activities and to improve the control of the biotechnological processes, and to improve sensory quality and food safety, among others. Moreover, regarding the use of sourdough biotechnology, behind the technological advantages, it also holds a high potential to improve nutritional value and health-promoting effects of the final food products, including reduction of the glycemic response, increase of minerals bioavailability and promoting the formation of bioactive compounds (e.g., prebiotic oligosaccharides) [1,2,67].
Similarly, a considerable number of health benefits have been postulated as a result of the intake of viable LAB strains (probiotics) and which were correlated with their antimicrobial properties, including desirable modification of microbiota, prevention of pathogens, stimulation of immune system, immune modulation of the human host [68,69]. However, each property is strain-specific, as well as culture medium and/or environmental-dependent. The current study also showed that different experimental conditions (specifically, the antimicrobial evaluation of LAB by using the agar well diffusion method and liquid medium) can lead to different behaviors. However, it must be mentioned that trends on LAB inhibition properties remained similar in the both experimental conditions. Finally, it is apparent from this study that the isolation and characterization of LAB from different matrices and geographical locations are very likely to contribute to the discovery of a greater diversity of LAB with distinct phenotypic features.

Antifungal Activity of the Isolated Sourdough Lactic Acid Bacteria Strains
The antifungal activity of sourdough LAB against the species of Aspergillus fischeri, Aspergillus nidulans, Penicillium oxalicum, Penicillium funiculosum, Fusarium poae, Alternaria alternate, and Fusarium graminearum are displayed in Table 4. Delay of Aspergillus fischeri spore formation was observed by using the sourdough LAB isolates L. Fungal spoilage of food and feed represents a major concern, as well as for human and animal health. Significant progress has been reported on the isolation and characterization of antifungal compounds (different organic acids, peptides, fatty acids, etc.), as well as various food-based applications of antifungal LAB have been described in the literature [21,23,26,27,70]. Rouse et al. [52] reported four cultures with antifungal activity originally isolated from cereals, chiefly strains of L. plantarum (CM8) and P. pentosaceus (R47) [71]. Other strains belonging to L. plantarum and P. pentosaceus species have previously been found to have antifungal activity [72]. Antifungal activity of the above-mentioned studies [71] was explained by different amounts of organic acids yielded by LAB strains and detected in the supernatants. Also, Magnusson et al. [72] unveiled the existence of cyclic dipeptides metabolized by LAB and with antifungal activity. According to Rouse et al. [71], by varying the growth conditions and chemical composition of fermentable media, the LAB antifungal activity is fairly consistent and stable [23]. The anti-fungal activity of these microorganisms is, obviously, modulated by such growth parameters as temperature, pH and incubation time. From above it is intuitive that LAB, which possess antifungal activity and are generally regarded as safe microbial starters, may represent an important tool to control or retard mold growth in a wide range of applications [1][2][3][4]10].  The production of organic acids during sourdough fermentation constitutes, indeed, a major safeguard against pathogens and spoilage microorganisms, since their undissociated forms exhibit strong microbial antagonistic effects, as verified in the present research effort. The organic acid production increases the mold-free shelf-life of sourdough breads. In LAB, the anti-microbial activities of lactic and acetic acids, at a given molar concentration, are not the same; the latter is more inhibitory than lactic acid, and can inhibit yeasts, molds and bacteria. Still, propionic acid inhibits preferentially fungi and bacteria, thus the co-fermentation of propionic acid bacteria, LAB and yeasts seems to be a promising natural sourdough-based biotechnological method to retard mold growth (although some technical limitations may occur) [1][2][3][4]10].
Compounds with anti-fungal properties are typically low-molecular-weight molecules, as is the case of organic acids, reuterin (β-hydroxypropionaldehyde), hydrogen peroxide, as well as proteinaceous compounds, hydroxyl fatty acids and phenolic compounds. Since fungistatic effects are mainly due to acetic rather than lactic acid production (acetic acid has a higher dissociation constant than lactic acid), heterofermentative LAB display the widest spectrum of anti-fungal activity, which is in agreement with the current experimental data [23,27]. Furthermore, the main LAB metabolites bearing anti-fungal attributes are, besides lactic and acetic acids, carbon dioxide, diacetyl, hydrogen peroxide, caproic acid, 3-hydroxy fatty acids, phenyllactic and 4-hydroxy-phenyllactic acids, cyclic dipeptides, fungicins (i.e., compounds of proteinaceous nature) and reuterin [1][2][3][4]10].
In Western Europe, economic losses related to contamination by molds in bread are estimated to exceed the 200 M€ a year. Mold growth may produce many kinds of food spoilage, viz. off-flavors, toxins, discoloration, rotting and triggering of pathogenic or allergenic effects. Though, production of mycotoxins is the most important issue of mold spoilage of foods. The experimental data in this work showed that sourdough biotechnology and sourdough LAB may play important roles on this purpose, and were the main LAB possessing ability to prevent (or limit) mycotoxinogenic mold growth belong to the genera of Lactobacillus, Lactococcus, Pediococcus, and Leuconostoc [4].

Conclusions
Spontaneous sourdough is an excellent source of lactic acid bacteria (LAB), as demonstrated in the present study, with high potential to answer to several needs and overcome technical limitations faced in the industry. The antimicrobial and antifungal properties as well as the metabolic capacity to ferment a large number of carbohydrate sources are only some good examples of the high techno-economic industrial potential of sourdough LAB or sourdough starter cultures based on single cultures or in distinct consortium designs.
In the present research work, 13 LAB strains with potential industrial application were isolated from spontaneous fermented rye sourdough. Most of the isolated sourdough strains showed versatile carbohydrate metabolisms. Leu. mesenteroides No. 242 and L. brevis No. 173 demonstrated ability for gas production. The seven out of 13 isolated strains exhibited growth yieldshigher than 7.0 log cycle after being submitted for 2 h to a culture medium with a pH value of 2.5. Furthemore, L. plantarum No. 122, L. casei No. 210, Lactobacillus curvatus No. 51, L. paracasei No. 244 and L. coryniformins No. 71 revealed inhibition properties against all the tested 15 pathogenic and opportunistic bacterial strains. Also, most of the isolated sourdough LAB displayed antifungal activities against seven selected mold strains. These results unveiled that LAB isolated from spontaneous sourdough are promising antimicrobial and antifungal ingredients.
This work highlighted the potential of sourdough biotechnology and, particularly, the LAB isolated from spontaneous sourdough to be applied in a wide range of agri-food industries, such as baking (sourdough bread and other sourdough-based baking goods, e.g., biscuits, cookies, crackers, pastry, pizza and pasta), feed and pet food, dairy (yoghurts, cheeses, smoothies, etc), meat (dried sausages, etc), alcoholic beverages (e.g., beer, cider and wine) and non-alcoholic beverages (juices, refrigerants, non-fermented and fermented cereal drinks), and nutraceuticals (dietary supplements and food additives), and also in other industrial sectors such as cosmetics and pharmaceuticals.