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首页> 外文期刊>Journal of Advances in Biology & Biotechnology >Influence of Agitation on the Propagation of Saccharomyces cerevisiae in the Process of Manufacturing Artisan Beers
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Influence of Agitation on the Propagation of Saccharomyces cerevisiae in the Process of Manufacturing Artisan Beers

机译:搅拌对手工啤酒酿造过程中酿酒酵母繁殖的影响

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Aims: In view of the growth of the production of artisan beers and the influence of aeration on microbial growth, this work aimed to show the importance of approaching the transfer of oxygen in aerobic fermentation processes. Study Design: In this study the agitation in the propagation of yeast Saccharomyces cerevisiae in the artisan brewing process was carried out, as it is of fundamental importance to consider the function of oxygen in the control of the metabolism and growth of the yeast. Place and Duration of Study: Laboratory of Food Microbiology, University of Uberaba, between June 2016 and July 2016. Methodology: The research was carried out at the Laboratory of Microbiology of Food and for the propagation, a dry malt extract (DME) was used, which is basically obtained by the hydrolysis of the raw and malted barley, and then subjected to concentration, vacuum dehydration and milling. For the fermentation process, the lyophilized yeast of Saccharomyces cerevisiae , Fermentis? brand, safarine strain US-05?, with the initial concentration of 19 x 109 cells per gram, was used in 11.5 g sachets, as indicated by provider. The strain was obtained from a specialist trade and is a neutral American yeast with no ester and high tolerance to alcohol. The wort, with an initial density of 1.035 g.cm-3, was prepared by dissolving 45 g of DME in 450 mL of boiling water and after 15 minutes of boiling it was cooled to 25°C. This procedure was repeated twice by obtaining propagation means 1 and 2. The yeast 11.5 g volume was divided into two portions and each portion was hydrated in 50 mL of distilled water at room temperature and inoculated into the propagation media 1 and 2. Sample 1 was shaken on a Nova Ethics? Kline shaker with rotation set at 120 RPMs for 10 hours. Sample 2 was rested and homogenized for collection every 1 hour for 10 hours. The determination of the cellular concentration (cel/mL) was performed in Neubauer chamber (1/400 mm2 x 1/10 mm) and for the determination of viable and non-viable cells, the International Coloring Method was used, using methylene blue as described in the methodology proposed by ASBC (1996). Viability is given by the ratio of viable cells to total cells. Results: The system that remained with constant agitation has a growth approximately 15% greater than the system without agitation. Conclusion: From the results obtained, it can be concluded that the propagation of yeast cells plays a fundamental role in the production of beers, whether homemade or industrial, because it increases the amount of viable cells, making the fermentation more intense. Agitation accelerates the consumption of substrate and, consequently, cell multiplication, besides increasing cell viability, which is fundamental for fermentation.
机译:目的:鉴于工匠啤酒产量的增长以及通气对微生物生长的影响,这项工作旨在表明在需氧发酵过程中处理氧气转移的重要性。研究设计:在这项研究中,在工匠酿造过程中进行了酿酒酵母发酵的搅拌,因为考虑氧气在控制酵母的代谢和生长中的作用至关重要。研究的地点和持续时间:乌贝拉巴大学食品微生物学实验室,2016年6月至2016年7月。方法:研究在食品微生物学实验室进行,为了繁殖,使用了干麦芽提取物(DME)。基本上是通过将生大麦和大麦大麦水解,然后进行浓缩,真空脱水和研磨而获得的。在发酵过程中,使用酿酒酵母Fermentis?的冻干酵母。如提供者所述,在最初的浓度为11.5 g的小袋中使用了最初浓度为每克19 x 109个细胞的Safarine菌株US-05?。该菌株是从专业商店获得的,是一种中性的美国酵母,没有酯,对酒精的耐受性很高。麦芽汁的初始密度为1.035 g.cm-3,是将45 g DME溶解在450 mL沸水中制备的,煮沸15分钟后将其冷却至25°C。通过获得繁殖工具1和2,将该过程重复两次。将酵母11.5 g的体积分成两部分,每部分在室温下在50 mL蒸馏水中水合,然后接种到繁殖介质1和2中。动摇了新星道德? Kline摇床,旋转速度设置为120 RPM,持续10小时。静置样品2,并每1小时匀浆收集10小时。细胞浓度(cel / mL)的测定在Neubauer室(1/400 mm2 x 1/10 mm)中进行,对于活细胞和非活细胞的测定,使用国际着色法,以亚甲基蓝作为在ASBC(1996)提出的方法学中有描述。存活力由存活细胞与总细胞之比得出。结果:持续搅拌的系统比没有搅拌的系统增长约15%。结论:从获得的结果可以得出结论,无论是自制啤酒还是工业啤酒,酵母细胞的繁殖在啤酒生产中都起着根本性的作用,因为它增加了活细胞的数量,使发酵更加激烈。搅动除了增加细胞活力(这对于发酵至关重要)之外,还加快了底物的消耗,进而加速了细胞增殖。

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