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通过内切-β-N-乙酰氨基葡萄糖苷酶H优化N-连接的高甘露糖寡糖的水解作用。

Optimizing hydrolysis of N-linked high-mannose oligosaccharides by endo-beta-N-acetylglucosaminidase H.

作者信息

Trimble R B, Maley F

出版信息

Anal Biochem. 1984 Sep;141(2):515-22. doi: 10.1016/0003-2697(84)90080-0.

DOI:10.1016/0003-2697(84)90080-0
PMID:6437277
Abstract

The ability of endo-beta-acetylglucosaminidase H (Endo H) from Streptomyces plicatus to hydrolyze high-mannose oligosaccharides from glycoproteins is influenced by numerous factors, including the tertiary structure of the substrate glycoproteins, the amount of Endo H used, the time of incubation, and the presence or absence of reagents that affect protein configuration. Endo H levels below 10 to 20 milliunits/ml may incompletely hydrolyze oligosaccharides, regardless of the incubation time, because even though the enzyme remains active, it becomes trapped or sequestered and is unavailable. Endo H activity can be potentiated by first denaturing substrate glycoproteins in a 1.2-fold weight excess of sodium dodecyl sulfate prior to hydrolysis. However, low levels of Endo H are sensitive to inactivation by sodium dodecyl sulfate, with considerable activity being lost over 4 h when the unbound detergent concentration exceeds protein by 0.02% (0.2 mg/ml). Other denaturants such as the Tritons, the zwittergents, the Brij series, or octylglucoside do not enhance or inhibit Endo H removal of oligosaccharides, but the chaotropic salt sodium thiocyanate at 0.5 M enhances Endo H action on some glycoproteins, particularly bovine thyroglobulin. Under denaturing conditions, proteolytic contaminants are a potential problem. Addition of 1 mM phenylmethylsulfonyl fluoride to Endo H incubations completely inhibits the residual Endo H-associated protease(s). Furthermore, Endo H is unaffected by a wide range of proteolytic inhibitors that may be used to protect substrate glycoproteins.

摘要

来自褶皱链霉菌的内切β-乙酰氨基葡糖苷酶H(Endo H)水解糖蛋白中高甘露糖型寡糖的能力受到多种因素的影响,包括底物糖蛋白的三级结构、所用Endo H的量、孵育时间以及影响蛋白质构型的试剂的存在与否。Endo H水平低于10至20毫单位/毫升时,无论孵育时间多长,都可能无法完全水解寡糖,因为即使该酶仍保持活性,但它会被困住或被隔离而无法发挥作用。在水解之前,先在1.2倍重量过量的十二烷基硫酸钠中使底物糖蛋白变性,可以增强Endo H的活性。然而,低水平的Endo H对十二烷基硫酸钠的失活很敏感,当未结合的去污剂浓度超过蛋白质0.02%(0.2毫克/毫升)时,4小时内会有相当多的活性丧失。其他变性剂,如Triton类、两性离子去污剂、Brij系列或辛基葡糖苷,不会增强或抑制Endo H去除寡糖的作用,但0.5 M的离液盐硫氰酸钠会增强Endo H对某些糖蛋白的作用,特别是牛甲状腺球蛋白。在变性条件下,蛋白水解污染物是一个潜在问题。在Endo H孵育体系中加入1 mM苯甲基磺酰氟可完全抑制与Endo H相关的残留蛋白酶。此外,Endo H不受多种可用于保护底物糖蛋白的蛋白水解抑制剂的影响。

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