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琼脂的酶促水解:来自大西洋假单胞菌的β-新琼脂四糖水解酶的纯化与表征

Enzymatic hydrolysis of agar: purification and characterization of beta-neoagarotetraose hydrolase from Pseudomonas atlantica.

作者信息

Groleau D, Yaphe W

出版信息

Can J Microbiol. 1977 Jun;23(6):672-9. doi: 10.1139/m77-100.

Abstract

Agarose is degraded by a beta-agarase from Pseudomonas atlantica to neoagarooligosaccharides of degree of polymerization (DP), 4, 6, 8, and 10. A beta-neoagarotetraose hydrolase cleaves the central beta-linkage in neoagarotetraose and the beta-linkage near the nonreducing end in neoagarohexaose and -octaose to yield neoagarobiose. The beta-neoagarotetraose hydrolase was localized on or outside the cytoplasmic membrane, in the cell wall region. The enzyme was activated by NaCl, KCl, CaCl2, MnCl2, and MgSO4, has a Km of 3.4 X 10(-3) M for neoagarotetraose, was free from beta-agarase and alpha-neoagarobiose hydrolase activity, and showed no transglycosidic activity.

摘要

来自大西洋假单胞菌的β-琼脂酶可将琼脂糖降解为聚合度(DP)为4、6、8和10的新琼脂寡糖。β-新琼脂四糖水解酶可切割新琼脂四糖中的中心β-键以及新琼脂六糖和新琼脂八糖中非还原端附近的β-键,生成新琼脂二糖。β-新琼脂四糖水解酶定位于细胞质膜上或膜外,细胞壁区域。该酶被NaCl、KCl、CaCl2、MnCl2和MgSO4激活,对新琼脂四糖的Km值为3.4×10(-3)M,无β-琼脂酶和α-新琼脂二糖水解酶活性,且无转糖苷活性。

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