1. Introduction
The snail is part of the general situation of agricultural activity, which is defined as “full cycle raising edible terrestrial snails.” This is a word composed of “Helici”, Helix derived from the name given to a genus of its shell snails which have a helix, and “culture” derived from Latin that means growing Cultivare.
The snails have been part of the diet of mankind for thousands of years. Fossil remains of prehistoric shellfish found in caves prove it. Until recently activity was limited to simple search of snails, both for their own consumption or to be sold on the market. From the last century, the gastronomic qualities of the snail began to be so appreciated that it went on to become a highly sought-after food. In recent decades snail consumption has been increasing throughout Europe, particularly in Mediterranean countries, while there has been a gradual disappearance of these delicious shellfish in areas where they live in a free state, which contributes to predation of the species and the introduction of pathogens that harm the productivity of it [1] [2] .
Helix aspersa Müller is also called common snail or Bovë, depending on the area of Europe. This variety is used on farms dedicated to raising snails for being the most popular in European countries where it is consumed by the snail, especially in France and Spain. Also this species is usually most familiar to consumers, speaking of a species native to these ecosystems and on the other hand this variety is best suited to rearing in captivity, thanks to its high prolificacy and high resistance. However, the development of this industry is limited by the presentation of bacterial gastrointestinal origin [3] . Wild snails with food and commercial interest, generate a whole agri-food production sector called “helicícola industry”, which is linked to the rural implications that are majorly environmental, economic and cultural, including industries and downstream activities, such as preparation, processing, marketing and consumption of the product [4] -[8] .
2. Materials and Methods
In order to assess the health status of snails have been sampled snail farms located in the province of Barcelona and parallel free-living snail, collected around the farm in order to compare the microbiota present in the thereof.
2.1. Processing the Samples
Samples from the farm were transferred to the laboratory under conditions of refrigeration, in order to carry out microbiological analysis.
For these analyzes were applied protocols established by the working group of the Laboratory of Applied Microbiology and Environ-mental Health Department and Anatomy, Faculty of Veterinary Medicine, Universidad Autonoma de Barcelona.
The samples were obtained from feces of healthy snails and snails that had a compromised health status, manifested by enteric problems. Additionally samples were obtained free-living snails.
These samples were stored in sterile containers and maintaining the cold chain is transferred to the laboratory for processing. Feces were weighed and resuspended in sterile 1/4 Ringer solution. Then, we proceeded to make a bank of decimal dilutions were plated on various culture media for microbiological assessment and establish broad microbiota in the faeces of the animals sampled.
The culture media used were Tryptic soy agar (TSA), general culture medium permits the growth of microorganisms demanding agar Man Rogosa Sharpe (MRS) to establish the lactic acid bacteria in general, and in particular for species of the genera Lactobacillus, Leuconostoc and Pediococcus, Mac Conkey agar (MK) in order to differentiate fermenting Gram-negative enteric bacilli and no lactose fermenters, agar Sabouraud (SAB) with antibiotic (Ab) allows the selective growth of filamentous fungi and yeast , Baird Parker agar (BP), which allows the development and differentiation of Staphylococcus.
2.2. Isolation and Identification
After incubation the stool samples was carried out snail isolation of the colonies grown on each of the culture media fields. Subsequently raised the strain identification, according to the methodologies established in our laboratory.
Once isolated colonies proceeded to differentiate according to their morphological characteristics such as shape, size, surface, edge lifting, internal structure, opacity, consistency.
By Gram staining microscopic characteristics were determined for strains such as: cocci, bacilli, coco-bacilli, etc., as well as the arrangement of bacterial cells (isolated, in chains, in clusters, tetrads, etc.) and classify in Gram-positive or Gram-negative according to the characteristics of the cell wall. Furthermore spore stains were performed that allowed us to demonstrate forms of resistance. Catalase test to check the presence or absence of catalase enzyme found in most aerobic and facultative anaerobic bacteria. Hemolytic activity tests revealed possible pathogenicity.
2.3. Identification to Species Level by Biochemical Tests
The identification of these strains was carried out using biochemical tests which are used for miniaturized systems that contain different substrates which facilitate the specific identification of each microorganism.
For identification of Lactobacillus and Bacillus used API 50 CH®, for identification of yeasts API20 C AUX® and identification of bacteria belonging to the family Enterobacteriaceae and other non-fastidious Gram-negative bacilli was used API 20 E®.
2.4. Conservation of Isolates
In order to proceed to the preservation of the strains, we proceeded to the lyophilization thereof.
3. Results and Discussion
From MRS agar isolation were obtained 17 strains that showed morphologies and characteristics of lactic acid bacteria, of which 11 strains belong to the genera Pediococcus, Lactococcus and Lactobacillus (See Table 1).
The genera Pediococcus and Lacobacillus were isolate in a 27.27% corresponding to the specie Pediococcus pentosaceus, Lactoccocus lactis and Lactobacillus was isolate in a 45.45% corresponding to a species: Lactobacillus plantarum, Lactobacillus brevis and Lactobacillus acidophilus. Of these eleven strains, nine were isolated from farm and were identified as Pediococcus pentosaceus, Lactoccocus lactis, Lactobacillus plantarum, Lactobacillus brevis and Lactobacillus acidophilus. Free-living isolated two strains identified as: Lactoccocus lactis
Table 1 . Strains isolated on MRS. Samples: Feces obtained from free-living snails and farm.
(Ca9) and Lactobacillus plantarum (Ca7).
Strains of Lactobacillus plantarum and Lactococcus lactis were isolated from stool specimens from snails, both as free life farms, which may show that these strains are typical species of snails, because it is part of the normal microbiota free-living snails.
In the bibliography, it is described that the genus Lactococcus is one of the genres that is part of normal microbiota snails [9] , claim that matches our research, since both snails living in captivity and free life strains were isolated from Lactococcus lactis.
The other authors do not mention the presence of species of the genus Lactobacillus, however in our study we have isolated three species belonging to this genre, matching the species Lactobacillus plantarum isolates from feces of snails farmed and free living.
In Table 2 are provided the strains isolated on Agar Sabouraud chloramphemicol and incubated under aerobic conditions at 28˚C for 24 to 48 hours.
In this medium were isolated five strains presenting yeast morphology, being identified as: Candida norvegensis, Candida guilliermondii and Cryptococcus humicola. In thebibliography, no information is provided in the presence of yeast, as constituents of the normal microbiota snails.
Table 3 shows the results obtained from the Isolation on MacConkey Agar, incubated under aerobic conditions at 37˚C for 24 to 48 hours, snails stool had a deteriorated state of health enteric derivative processes.
Among the microorganisms which are part of the normal microbiota Helix aspersa species described in the literature, four groups of Gram-negative anaerobic bacteria, belonging to the families Enterobacteriaceae and Pseudomonadaceae [9] -[11] . In our study we isolated bacteria belonging to the family Enterobacteriaceae coinciding with the species described in literature.
Throughout our research, we isolated and identified two species belonging to the genus Klebsiella: Klebsiella oxytoca and Klebsiella terrigena, a strain of the genus Pantoea Pantoea sp., Two strains belonging to the genus Citrobacter, identified as Citrobacter koseri/farmeri and two strains belonging Enterobacter: Enterobacter cloacae and Enterobacter amnigenus.
Helix aspersa is a prolific and phytophagous species that is limited by the manifestation of bacterial gastrointestinal origin [9] and by certain bacteria that can behave as opportunistic pathogens [10] . Such is the case of bacteria isolated from apparently healthy animals as Salmonella enterica [12] , Aeromonas sp. [11] and Enterobacter sp. [13] .
Table 2. Strains isolated in Agar Sabouraud + chloramphenicol isolated from feces of snails.
Table 3. Strains isolated from feces of snails with health troubles on Agar MacConkey.
4. Conclusion
The results obtained in our study can contribute to the normal microbiota of the species Helix aspersa Müller, which is constituted mainly by species of the genera Lactobacillus, Lactococcus and Pediococcus and yeasts identified as Candida norvegensis, Candida guilliermondii and Cryptococcus humicola. In the case of snails with enteropathogenic symptoms, the presence of Lactobacillus and Lactococcus are reduced and in this case we found high prevalence of species of Klebsiella, Pantoea, Citrobacter and Enterobacter.
NOTES
*Corresponding author.