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Enzymatic Removal of Diacetyl from Beer II. Further Studies on the Use of Diacetyl Reductase

机译:从啤酒II中酶法去除二乙酰基。使用二乙酰还原酶的进一步研究

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Diacetyl removal from beer was studied with whole cells and crude enzyme extracts of yeasts and bacteria. Cells of Streptococcus diacetilactis 18-16 destroyed diacetyl in solutions at a rate almost equal to that achieved by the addition of whole yeast cells. Yeast cells impregnated in a diatomaceous earth filter bed removed all diacetyl from solutions percolated through the bed. Undialyzed crude enzyme extracts from yeast cells removed diacetyl very slowly from beer at its normal pH (4.1); at a pH of 5.0 or higher, rapid diacetyl removal was achieved. Dialyzed crude enzyme extracts from yeast cells were found to destroy diacetyl in a manner quite similar to that of diacetyl reductase from Aerobacter aerogenes, and both the bacterial and the yeast extracts were stimulated significantly by the addition of reduced nicotinamide adenine dinucleotide (NADH). Diacetyl reductase activity of four strains of A. aerogenes was compared; three of the strains produced enzyme with approximately twice the specific activity of the other strain (8724). Gel electrophoresis results indicated that at least three different NADH-oxidizing enzymes were present in crude extracts of diacetyl reductase. Sephadex-gel chromotography separated NADH oxidase from diacetyl reductase. It was also noted that ethyl alcohol concentrations approximately equivalent to those found in beer were quite inhibitory to diacetyl reductase.
机译:用全细胞以及酵母和细菌的粗酶提取物研究了从啤酒中去除二乙酰的方法。双乙酰链球菌18-16细胞破坏溶液中的二乙酰,其速率几乎等于添加完整酵母细胞所达到的速率。浸渍在硅藻土滤床中的酵母细胞从渗透通过该床的溶液中除去了所有二乙酰基。酵母细胞中未透析的粗酶提取物在其正常pH值下非常缓慢地从啤酒中去除了二乙酰(4.1);在5.0或更高的pH值下,可快速去除二乙酰基。发现来自酵母细胞的经透析的粗酶提取物以与来自产气杆菌的二乙酰还原酶完全相似的方式破坏二乙酰,并且通过添加还原的烟酰胺腺嘌呤二核苷酸(NADH)显着刺激细菌和酵母提取物。比较了四种产气曲霉菌株的二乙酰还原酶活性。其中三个菌株产生的酶的比活性约为另一个菌株(8724)的两倍。凝胶电泳结果表明,在二乙酰还原酶的粗提物中至少存在三种不同的NADH氧化酶。 Sephadex凝胶色谱分离了NADH氧化酶和二乙酰还原酶。还应注意,乙醇浓度约等于啤酒中的乙醇浓度,对二乙酰基还原酶具有相当的抑制作用。

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