Impact of Storage Temperature on Microbial Diversity and Probiotic Effect of Liquid Brewers’ Yeast

Using probiotics as animal feed additives instead of antibiotics is gaining momentum to avert adverse negative effects on human health. Liquid brewers yeast (LBY) is an industrial by-product containing probiotic microorganisms and is also used as a protein supplement for dairy animals. Nevertheless, value chain actors lack of appropriate handling practices compromises the by-products quality and safety. This study aimed to determine the effect of variation in temperature on microbial diversity and probiotic effects during the storage time of LBY sampled from distributors and farmers from Githunguri sub-county of Kenya. The samples were stored at 20C, 25C and 30C, then tested on 0, 5, 10, 15 and 20 days. The studys parameters involved determining the pH levels, lactic acid bacteria (LAB), total coliform count (TCC), mould, and yeast in LBY. The rate (k) of the reaction kinetics model was used to extrapolate the expected probiotic shelf life. The LAB and yeast populations were reduced in a first-order reaction at all storage temperatures. The rate of reduction in the numbers of LAB reduced with an increase in temperature (k = 0.019 and 0.023) at 20C and 30C, respectively. Yeasts highest rate of growth reduction was 25C (k = 0.009) and least at 30C (k = 0.043). The minimum effective concentration for probiotics of 106 CFU/mL needed to observe the beneficial physiological impact on farm animals was achieved between 34.9 and 35.5 days at the tested storage temperatures. The study provides insight into the unexploited low-cost probiotic potential of LBY in dairy production. Conversely, handling practices and environmental microbial contamination along the value chain can compromise product quality and safety. There is a need to advocate its use in dairy for improved productivity and sensitize farmers to appropriate hygienic measures along the LBY value chain.

Dairy Farming Conditions and Utilization Levels of Liquid Brewers’ Yeast in Kenya

Dairy production plays an integral part in supporting smallholder farmers’ livelihoods. The desire to increase the number of dairy cattle is not feasible due to the reduced output of feed resources occasioned by climate change. Consequently, the need to increase productivity per cow is inevitable. Conventional protein supplements are costly;hence, the need to explore affordable nutrientdense alternative feed resources. Liquid brewers’ yeast (LBY), a by-product of the brewing industry, is a rich protein supplement in dairy production. This study aimed to assess the dairy farming conditions and utilization levels of LBY as a feed supplement in Githunguri Sub-county, Kiambu. Semi-structured questionnaires were administered to 457 dairy farmers in a cross-sectional survey. The findings revealed that most farmers (94.2%) fed their cattle on established forage/fodder and crop residues with supplementation. Even though 53.1% of the respondents were aware of the use of LBY, only 30.6% utilized it to supplement dairy cows, most of whom (96.0%) used it fresh without preservation. Membership in farmers’ organizations increased awareness of LBY (r = 0.732). Principal component analysis indicated that the benefits of using LBY outweigh the challenges involved with a loading matrix of 0.891 - 0.954 and 0.681 - 0.807, respectively. The low adoption and use levels of LBY as a source of protein supplements were due to low awareness. There is a need for concerted efforts by stakeholders in the industry to increase farmers’ knowledge base on the utilization and effectiveness of LBY in dairy production.

Recovery of Residual Brewer’s Yeast by Electroactivation

Yeasts resulting from the brewing process (RBY) are a valuable by-product, with an important content of minerals, vitamins and, especially, proteins. The purpose of the research was the electroactivation of RBY and the simultaneous obtaining of two products—protein concentrates and hydrolyzed protein from residual brewer’s yeast. Electroactivation is a non-residual process, without the use of chemical reagents and relatively inexpensive. The variation of the electroactivation conditions allowed the separation of 90% - 94% of the proteins in the form of protein concentrates. During the process, it is attested to increase the pH value and decrease the redox potential, which characterizes the multiple redox processes that take place in the cathode cell, including sedimentation at the isoelectric point. The presence of albumin in the protein fractions of RBY allows the formation of protein complexes with calcium, attributing a higher biological value to the obtained products.

荧光微孔板法检测啤酒酵母胞内脯氨酸含量

高浓酿造是啤酒生产中一种常用的高效经济技术,而在高浓酿造过程中啤酒酵母在各个时期存在不同的环境压力。脯氨酸被认为是啤酒酵母中的一种应激保护剂,赋予了酵母细胞更高的胁迫耐受性。酵母胞内脯氨酸含量可以作为筛选环境耐受能力强菌株的参考,因此有必要建立一种能够快速检测啤酒酵母胞内脯氨酸含量的方法。该研究基于次氯酸钠氧化和邻苯二甲醛/N-乙酰半胱胺酸荧光检测脯氨酸的通用方法,结合细胞破碎的优化,成功建立了一种可以准确测定啤酒酵母胞内脯氨酸含量的荧光微孔板法,其线性范围和回收率分别为5~40μmol/L(0.58~4.6 mg/L)和73.33%~105.5%。通过比较该检测方法与氨基酸专用高效液相色谱法,发现两者测定胞内脯氨酸含量绝对值相比无显著性差异,但是荧光微孔板法操作简便快捷。因此,该研究建立的荧光微孔板法为测定酵母胞内脯氨酸提供了一种新思路,同时为适应高浓酿造胁迫的啤酒酵母筛选提供了一种新策略。

啤酒废酵母提取物皮肤美白功效研究

为探究啤酒废酵母(BSY)提取物作为护肤化妆品美白功能因子的可行性。该试验采用乙醇溶液提取得到啤酒废酵母浸膏,并以提取率为评价指标,采用单因素试验和响应面试验优化提取条件。啤酒废酵母浸膏分别用乙醇、石油醚、乙酸乙酯、正丁醇提取得到4种不同极性的提取物,以抗紫外线、抗氧化及酪氨酸酶抑制活性为评价指标,考察4种不同极性提取物对美白效果的影响。结果表明,啤酒废酵母在料液比1∶28(g∶m L)、乙醇体积分数79%、提取温度57℃、提取时间1.5 h的条件下,实际提取率最高为38.1%。不同极性溶剂提取物对紫外线均有吸收效果,石油醚提取物紫外吸收率最高(>87%);乙醇提取物对2,2'-联氮双(3-乙基苯并噻唑啉-6-磺酸)二铵盐(ABTS)自由基清除率最高,为96.49%;乙酸乙酯提取物对1,1-二苯基-2-三硝基苯肼(DPPH)自由基清除率最高,为93.49%;不同极性溶剂提取物均表现出酪氨酸酶抑制作用,其中石油醚提取物最高,达到33.29%。该研究结果可为啤酒废酵母提取物在护肤化妆品中的应用提供指导,可用于美白护肤产品的研发。

富铬酵母中铬的化学种态及结合形态研究

对富铬酵母中铬的化学种态进行了分析和初步探讨.在铬的化学种态测定中,使用离子交换和火焰原子吸收法测定了富铬酵母中的Cr(Ⅲ)和Cr(Ⅵ),方法快速简便,定量回收.结果表明,总铬含量为1582μg/g的富铬酵母中,无机态铬占16%,其中Cr(Ⅲ)为232μg/g、Cr(Ⅵ)为24.5μg/g.酵母细胞富铬过程中,84%以上的无机铬化合物转化成有机铬.说明铬参与了酵母细胞的生物合成,促进生物转化,对提高富铬酵母的生物效应极为有益.

啤酒废酵母对铜离子的吸附研究

以啤酒酿造厂的啤酒废酵母为生物吸附剂,研究啤酒废酵母对Cu2+的生物吸附行为.利用原子吸收光谱法测定Cu2+含量.结果表明,啤酒废酵母吸附Cu2+受吸附时间、吸附温度、溶液pH值、酵母添加量和Cu2+起始浓度等因素影响.实验确定了啤酒废酵母对Cu2+的最佳吸附条件.即:pH为4.0,Cu2+浓度为100 mg.L-1,酵母添加量1.0 g.L-1,吸附温度25℃,吸附时间2.5 h.此时啤酒废酵母对Cu2+的吸附量可达91.82±0.54 mg.g-1干酵母.对未吸附Cu2+的空白酵母和吸附Cu2+的酵母进行红外光谱分析,结果显示啤酒废酵母吸附Cu2+后羟基和羧基吸收峰发生明显变化,因此认为羟基和羧基在生物吸附中起着重要作用.

富铬酵母的理化性质和氨基酸分析

用２００～３００ｎｍ的波长范围对富铬酵母及普通酵母的溶液进行紫外扫描，发现在λ_(２６０ｎｍ)处有一特征紫外吸收峰，富铬酵母细胞的铬含量与其吸收峰的光密度呈线性关系；在不同的温度和ｐＨ值条件下，通过紫外吸收峰的测定，富铬酵母溶液在酸性条件下稳定，在碱性条件下不稳定。溶液的λ_(２６０ｎｍ)紫外吸收峰随着温度的上升而升高。从氨基酸含量分析结果看，富铬酵母的谷氨酸、甘氨酸、组氨酸、丙氨酸和赖氨酸含量高于普通酵母，但其他氨基酸含量比普通酵母低。

啤酒酵母自溶液中的物质变化及酵母自溶评价指标探索

以4株不同的啤酒酵母菌株为研究对象,比较其在模拟自溶条件下电镜细胞形态及溶液物质变化,寻找能够判定酵母自溶性能的较优评价指标。结果表明,α-氨基氮、甲醛氮、各种分子质量蛋白质和游离长链脂肪酸等指标虽然都随酵母自溶有一定的变化,但规律性不强,单一因素不适合作为判定酵母自溶的直接指标。随着酵母自溶性能和自溶程度的变化,(A260/A280)/死亡率呈现明显且一致的变化趋势,酵母自溶程度越大,该比值越小。该指标综合性好、灵敏度高、耗时少、操作简单,能够及时反映不同菌株自溶性能的差异,以及同一株菌在不同阶段的自溶情况,是较好的酵母自溶评价指标。

固定化啤酒废酵母对Cr^(6+)吸附行为的研究

用啤酒废酵母作吸附剂,以海藻酸钠作包埋剂将酵母固定化制作成小球,分别从吸附时间、温度、Cr6+溶液质量浓度、pH等因素,研究啤酒废酵母菌体对Cr6+的吸附特性。确定固定化啤酒废酵母对Cr6+吸附的最佳条件为:吸附时间2 h、温度25℃、Cr6+溶液质量浓度60 mg/L、pH为2。在该条件下,对Cr6+最大吸附率为94.71%。其中,Ca2+、Na+、Mg2+、Cu2+不会干扰啤酒废酵母对Cr6+的吸附,以1 mol/L盐酸的解吸效果最佳,解吸率达94.1%。

富铬酵母降低糖尿病大鼠血糖的生物效应评价

目的 : 研究富铬酵母对四氧嘧啶致实验性糖尿病大鼠的降血糖作用。方法 : 对糖尿病大鼠连续口服富铬酵母〔 Cr 2 0 0μg/ (kg bw· d)〕和〔 Cr 2 0μg/ (kg bw· d)〕以及普通酵母〔 Cr 1μg/ (kg bw· d)〕4w,观察记录每天的饮水和进食情况。每周末采集尾静脉血 ,测定血糖、总胆固醇 (TC)、甘油三酯 (TG)、低密度脂蛋白 (LDL)、高密度脂蛋白 (HDL )、胰岛素、C肽的含量。结果 : 各治疗组大鼠的体重明显高于糖尿病组 ,各治疗组大鼠的血糖水平、TG、TC、LDL、胰岛素及 C肽显著降低 ,而 HDL升高。高剂量富铬酵母的降血糖作用明显高于其他各组。结论 : 富铬酵母在体内可以改善糖和脂代谢 ,可用来预防和治疗糖尿病。

化学诱变选育低双乙酰啤酒酵母菌株的研究

通过EMS诱变,从啤酒酿造生产菌株啤酒酵母(Saccharomyces carlsbergensis)FB中筛选分离得到一株发酵液中双乙酰含量优于亲株的新菌株FB-E1。以120Bx麦芽汁为培养基,用内装300ml麦芽汁的500ml三角瓶于12℃下发酵,发酵8d后发酵液中双乙酰含量比亲株降低了42.7%。该菌株的其它发酵性能的测定结果表明其保持了亲株的优良性状,且遗传性状稳定。

高浓度双乙酰定向驯化获得优良啤酒酵母菌株的研究

在双乙酰浓度为1mg/mL的12°Bx麦芽汁中进行高浓度定向驯化,经涂布抗双乙酰固体选择培养基,从啤酒酿造生产菌株啤酒酵母(Saccharomycessp.)A中富集筛选分离得到一株双乙酰还原速度优于亲株A的新菌株TA4。以12°Bx麦芽汁为培养基用内装300mL麦芽汁的500mL三角瓶10℃下发酵,发酵8d后发酵液双乙酰含量比亲株降低了36.31%,发酵度提高4.5%,且该菌株的絮凝性、发酵速率等特性仍保持了亲株A的优良性状。

利用啤酒废酵母间歇发酵合成谷胱甘肽的研究

研究利用啤酒废酵母生产谷胱甘肽的目的是降低谷胱甘肽生产成本、提高啤酒废酵母附加值.研究考察了在2升通气搅拌罐中通气量、搅拌速度、初始葡萄糖浓度以及废酵母加入量对谷胱甘肽合成的影响.实验表明,好氧活化可以显著提高酵母细胞内的谷胱甘肽含量.由于啤酒废酵母的添加量较大,使得反应液中菌体浓度较高,发酵过程中保持较大的通气量和搅拌速率有利于提高细胞活性和促进谷胱甘肽的积累.通过实验确定了2L发酵罐中较佳的操作参数为搅拌速度500r@min-1,通气量6 L@L-1@min-1.过高的初始葡萄糖浓度对谷胱甘肽的合成有一定的抑制作用,比较合适的初始葡萄糖用量为加入的废酵母湿重的10%.废酵母加入量增大会导致胞内谷胱甘肽含量下降,但由于细胞干重的大幅度增加,在实验范围内,最终单位反应器体积的谷胱甘肽产量则随废酵母加入量增大而增大.实验表明,废酵母加入量在湿酵母为100～300g@L-1之间是合适的.

固定化啤酒废酵母对Pb^(2+)的吸附

用2%海藻酸钠与1%明胶混合为包埋剂固定啤酒酵母废菌体,研究固定化啤酒废酵母对Pb2+的吸附行为。利用原子吸收光谱法测定Pb2+含量。结果表明,固定化啤酒废酵母吸附Pb2+受吸附时间、吸附温度、溶液pH值、酵母添加量和Pb2+起始浓度等因素影响。实验确定了固定化啤酒废酵母对Pb2+的最佳吸附条件。即:pH为3.0～5.0,Pb2+浓度为100mg.L-1,酵母添加量1.2g.L-1,吸附温度25℃,吸附时间120min。在一定的浓度范围内啤酒废酵母对Pb2+的吸附符合Langmuir吸附模型和Freundlich吸附模型,但符合Freundlich吸附模型的程度更优。

酶法制备啤酒废酵母生物活性肽的工艺条件研究

以啤酒废酵母为原料,经木瓜蛋白酶酶解、分离、纯化、干燥等工序制得啤酒废酵母活性肽。试验通过单因素及响应面分析方法确定了木瓜蛋白酶对废酵母的最佳酶解条件为:酶解温度57.78℃,pH 7.05,酶用量3.03%.酶解后多肽得率可达到52.13%。

啤酒废酵母菌体吸附Ni^(2+)的特性研究

啤酒废酵母菌体是一种新型的生物吸附剂,可用于处理重金属离子。本实验研究不同吸附温度、吸附时间、pH值,以及镍离子浓度和啤酒废酵母菌体浓度条件下,啤酒废酵母菌体对Ni2+的吸附能力。初步确定啤酒废酵母菌体对Ni2+吸附的最佳组合,即吸附温度为40℃、吸附时间为60min、起始pH值为5、啤酒废酵母菌体的质量浓度为0.9g/L、Ni2+质量浓度为230mg/L,在此条件下啤酒废酵母菌体对Ni2+吸附率可达57%左右。

低双乙酰啤酒酵母工程菌的构建

利用PCR技术以啤酒酵母QY的染色体为模板扩增出含有乙酰羟酸合成酶 (AHAS)基因ILV2的片段 ,将ILV2基因的内部EcoRI片段连接到整合载体YIp5上 ,并在该载体的BamHI -SalI位点插入铜抗性基因CUP1-MT1,构建了YIpCE质粒 ,将其转化啤酒酵母QY ,所得到的转化子AHAS酶的活力比受体菌QY降低75 %左右 ,在发酵测试中 ,转化了产生双乙酰的量比原始菌株降低 30 %。

富铬酵母中14种元素的ICP-AES测定

本文用ＩＣＰ－ＡＥＳ法同时测定富铬酵母中Ｋ、Ｆｅ、Ｐ、Ｚｎ、Ｃｒ、Ｃｕ、Ｍｎ、Ｃｏ、Ｂａ、Ｓｒ、Ｖ、Ｎａ、Ｍｇ、Ｃａ１４种元素的含量。结果表明，富铬酵母中的铬对其他元素的浓度有一定影响，并且，Ｋ、Ｍｎ、Ｐ、Ｖ、Ｍｇ、Ｃａ的浓度明显低于普通酵母。

利用啤酒废酵母制备富锌酵母

以啤酒废酵母为原料制备富锌酵母。对制备的工艺条件进行了优化。确定最佳的工艺条件条件为:Zn2+的浓度为500μg/mL;培养pH值为4.5;振荡培养时间为10h;啤酒酵母投加量为50g/50mL培养基。通过红外分析对空白废酵母和富锌废酵母进行比较,分析了酵母富集锌前后吸收峰的变化。