Effect of the substrate and the cell treatment conditions on the ethanolic fermentation contaminated with Saccharomyces cerevisiae wild yeasts and Lactobacillus fermentum

A little is known about the effect of the substrate and the interaction among wild yeast strains and bacteria Lactobacillus in the alcoholic fermentation, because the studies have been concentrated in the evaluation of the contamination effects by one or another contaminant, separately. This work aimed to evaluate the effect of the substrate and the cell treatment conditions over the batch fermentations contaminated with both microorganisms, yeast wild strains of S. cerevisiae (three strains displaying rough colonies and pseudohyphal cell growth) and Lactobacillus fermentum, being the S. cerevisiae strain PE-2 as the starter yeast. Fermentations using sugarcane juice and molasses, without and with cell recycle, utilizing both the pure culture of PE-2 as the mixed cultures with rough yeast strains and or L. fermentum were carried out. Modifications in the acid cell treatment by the addition of ethanol to the acid solution and the lowering of pH of the acid solution or a treatment with potassium metabisulphite were evaluated, aiming the growth control of the contaminants without affecting the starter yeast. An acid treatment with the addition of 13% ethanol was applied in fermentation with cell recycle, both in sugarcane juice and molasses, utilizing PE-2, one of the rough yeast strains and L. fermentum. The extracellular invertase activity was also evaluated in both substrates for the microorganisms studied, in growing conditions. The type of substrate, sugarcane juice or molasses, influenced the performance of the PE-2 strain as well as affected the development of the contaminations with rough S. cerevisiae yeast strains with or without L. fermentum, in fermentations without cell recycle. The effect of the contamination was more remarkable when sugarcane juice was utilized, in fermentations contaminated with rough yeast strains, but the inverse was observed when L. fermentum was the contaminant. The contamination effect was more harmful with the rough yeast strain than with the bacteria, and the double contamination (with both rough yeast strain and bacteria) did not have a higher effect over the fermentative efficiency than the single contamination, by one or another microorganism in isolation, especially in the batch fermentation with cell recycle, regardless the substrate. In cell-recycled fermentations the effect of the substrate was less evident. The growth control of the rough yeast strains may be done by modifying the acid cell treatment carried out in the industry, both by the addition of ethanol to the acid solution or by the pH lowering, depending on the rough yeast strain. , The combined treatment (pH 2.0 + 13% ethanol) affected PE-2 physiology, bringing about loss in the cell-recycled fermentation, with low growth control of the rough yeast strain but causing cell death of L. fermentum. The difference in the invertase activity between the rough yeast strains and the starter yeast PE-2 may be responsible for the low fermentation rate displayed by the rough yeast strains, but a non significant effect of the substrate on the enzyme activity was observed. (AU)