Nobutake Hamada scite author profile

An ejc0-/M,3-glucanase was purified from the commercial enzyme preparation "Kitalase" which is a yeast cell wall lytic enzyme preparation. The purification procedures consisted of following steps: ammoniumsulfate fraction, SP-Sephadex C-50 and CM-Cellulose C-32 column chromatography, and Sephadex G-100 gel filtration. The optimum pH value was 5.8, and the optimum temperature was 55°C. The enzymewas stable in the pHrange of 5.1 to 9.8 and at temperatures below 53°C. The isoelectric point and the molecular weight were estimated to be pH 9.3 and 73000, respectively. The enzyme was shown to bypass /M,6-linkaged branches to cleave /?-1,3-linkages when scleroglucan was used as substrate. The Kmvalues for laminarin, laminaripentaose, laminaritetraose and laminaritriose were 0.16, 2.01, 2.24 and 1.34him, respectively.

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Nobutake Hamada

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Purification and some properties of an exo-.BETA.-1,3-glucanase from basidiomycete species.

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