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作 者:沈海萍[1] 吴晓刚[1] 王晓丹[1] 赵长新[1]
机构地区:[1]大连工业大学生物工程学院,辽宁大连116034
出 处:《中国酿造》2011年第1期55-58,共4页China Brewing
基 金:国家"十一五"国家科技支撑计划重点项目(2007BAK36B01)
摘 要:麦芽的皮层和胚乳糊粉层中都残存有内源酶无法完全降解的β-葡聚糖,进而影响浸出率和麦汁粘度、过滤难度和啤酒胶体稳定性。在啤酒生产中,添加外源β-葡聚糖酶可以有效解决这些问题。采用刚果红营养平板法(GCN平板法)从衡水老白干和老龙口酒曲中筛选了3株β-葡聚糖酶活力较高且生产周期短的菌株(分别标记为4#、8#、12#),通过液态发酵,测得酶活分别为0.362U/mL、0.542U/mL、0.511U/mL。并对发酵培养基进行了优化,得到8#初始菌株最佳酶活为0.556U/mL。对该菌株进行紫外诱变,得到突变株酶活为:0.879U/mL。In the husk and aleurone layer of malt, there is some β-glucan which could not be degraded completely by endogenous enzymes. The existence of β-glucan affects extraction efficiency, wort viscosity, filtration and beer colloid stability. The problem could be solved effectively by the addition of exogenous β-glucanase during beer production. In this study, 3 microbial strains, which had relatively high β-glucanase activities, were isolated from Hengshui Laobaigan and Laolongkou Daqu by GCN plate method and were coded as 4#, 8# and 12# respectively. Their β-glucanase activities were detected to be 0.362U/ml, 0.542U/ml and 0.511U/ml respectively. By the optimization of fermentation medium, the β-glucanase activity of 8# strain was improved as 0.55U/ml. Furthermore, a mutant of 8# strain was achieved by UV treatment, whose β-glucanase activity reached 0.879U/ml.
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