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Enzymatic Hydrolysis of Yeast Cell Walls I. Isolation of Wall-Decomposing Organisms and Separation and Purification of Lytic Enzymes

机译:酵母细胞壁的酶水解I.壁分解生物的分离以及溶菌酶的分离和纯化

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摘要

Tanaka, Hirosato (University of California, Davis), and Herman J. Phaff. Enzymatic hydrolysis of yeast cell walls. I. Isolation of wall-decomposing organisms and separation and purification of lytic enzymes. J. Bacteriol. >89:1570–1580. 1965.—A number of microorganisms, able to decompose and grow on yeast cell walls, were isolated from soil. These isolates demonstrated various types of attack on yeast walls. A bacterium, identified as Bacillus circulans, and a species of Streptomyces produced clear, lysed zones when grown on an agar medium containing baker's yeast cell walls. The streptomycete formed glucanase, mannanase, and protease, but B. circulans produced only glucanases. Purified mannan could be prepared from the culture fluid of B. circulans grown on baker's yeast cell walls. In a liquid, mineral medium, extracellular lytic enzyme production by B. circulans was optimal after 3 days of aerobic growth at 30 C with 0.5% baker's yeast cell walls as the carbon source. Twelve other carbon sources were ineffective as inducers. Among a number of polysaccharides tested, the crude enzymes of B. circulans hydrolyzed only β-1→3 glucan (laminarin) and β-1→6 glucan (pustulan), both by a random mechanism, to a mixture of dimer and glucose. The β-1→3 and β-1→6 glucanases were separated from each other by diethylaminoethyl cellulose column chromatography. Water-soluble oat glucan, which contains in the linear chain both β-1→3 and β-1→4 bonds, was also hydrolyzed by the bacterial β-1→3 glucanase. The products of this reaction indicated that this enzyme hydrolyzes β-1→3 or β-1→4 glucosidic linkages, provided the β-glucopyranosyl units composing these bonds are substituted in the 3 position by another glucose unit.
机译:田中弘弘(加州大学戴维斯分校)和赫尔曼·法夫。酵母细胞壁的酶促水解。 I.分离可分解壁的生物以及分离和纯化裂解酶。 J.细菌。 > 89: 1570–1580。 1965年。从土壤中分离出许多能够分解并在酵母细胞壁上生长的微生物。这些分离株表现出对酵母壁的各种类型的攻击。当细菌在含有面包酵母细胞壁的琼脂培养基上生长时,一种细菌被称为圆形芽孢杆菌(Bacillus circulans)和一种链霉菌产生了清晰的裂解区。链霉菌形成了葡聚糖酶,甘露聚糖酶和蛋白酶,但环孢芽孢杆菌仅产生葡聚糖酶。纯化的甘露聚糖可以从在面包酵母细胞壁上生长的圆环芽孢杆菌的培养液中制备。在液态的矿物质培养基中,在0.5%贝克酵母细胞壁作为碳源的情况下,在30°C下需氧生长3天后,由B. circulans产生的胞外裂解酶最为理想。其他十二种碳源无效。在许多测试的多糖中,圆环芽孢杆菌的粗酶仅通过随机机制将β-1→3葡聚糖(laminarin)和β-1→6葡聚糖(pustulan)水解为二聚体和葡萄糖的混合物。通过二乙氨基乙基纤维素柱色谱法将β-1→3和β-1→6葡聚糖酶彼此分离。在细菌的β-1→3葡聚糖酶中也水解了在直链中同时含有β-1→3和β-1→4键的水溶性燕麦葡聚糖。该反应的产物表明该酶水解β-1→3或β-1→4糖苷键,只要构成这些键的β-吡喃葡萄糖基单元在3位被另一个葡萄糖单元取代。

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