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Denaturation Kinetics of N-Acetyl-β-D-glucosaminidase from Scylla serrata in Urea Solution

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摘要 N-Acetyl-β-D-glucosaminidase(NAGase, EC 3.2.1.52), which catalyzes the cleavage of N-acetylgluco- samine polymers, plays important roles in the molting, digestion of chitinous foods in green crab. In the study, the efforts of urea on the activity of NAGase purified from the viscera of green crab(Scylla serrata) have been studied. The results show that appropriate concentrations of urea can lead to reversible inactivation of the enzyme, and the value of the inhibitor concentration leading to 50% of enzyme activity lost(IC50) is estimated to be 0.63 mol/L. The inactivation kinetics has been studied via the kinetic method of the substrate reaction. The rate constants of inactivation have been determined. The value of k+0 is larger than that of k′+0, indicating the free enzyme molecule is more fragile than the enzyme-substrate complex in urea solution. It is suggested that the presence of the substrate offers the marked protection of this enzyme against inactivation by urea. N-Acetyl-β-D-glucosaminidase(NAGase, EC 3.2.1.52), which catalyzes the cleavage of N-acetylgluco- samine polymers, plays important roles in the molting, digestion of chitinous foods in green crab. In the study, the efforts of urea on the activity of NAGase purified from the viscera of green crab(Scylla serrata) have been studied. The results show that appropriate concentrations of urea can lead to reversible inactivation of the enzyme, and the value of the inhibitor concentration leading to 50% of enzyme activity lost(IC50) is estimated to be 0.63 mol/L. The inactivation kinetics has been studied via the kinetic method of the substrate reaction. The rate constants of inactivation have been determined. The value of k+0 is larger than that of k′+0, indicating the free enzyme molecule is more fragile than the enzyme-substrate complex in urea solution. It is suggested that the presence of the substrate offers the marked protection of this enzyme against inactivation by urea.
作者 LIN Jian-cheng LI Hua-liang CHEN Liang-hua YANG Xue-min WANG qin CHEN Qing-xi
机构地区 Key Laboratory of Coastal and Wetland Ecosystems Department of Blood Transfusion Department of Food and Biological Engineering
出处 《Chemical Research in Chinese Universities》 SCIE CAS CSCD 2011年第6期996-999,共4页 高等学校化学研究(英文版)
基金 Supported by the National Natural Science Foundation of China(No.40576066) the Science and Technology Foundation of Xiamen,China(No.3502Z20081143)
关键词 Green crab(Scylla serrata) N-ACETYL-Β-D-GLUCOSAMINIDASE UREA Reversible inactivation kinetics
分类号 TS252.1 [轻工技术与工程—农产品加工及贮藏工程] TQ925.9 [轻工技术与工程—食品科学与工程]
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  • 1Zen K.C.,Choi H.K.,Krishnamachary N.,Muthukrishnan S.,Kramer K.J.,Insect Biochem.Mol.Biol.,1996,26,435. 被引量:1
  • 2Ken A.B.,William D.S.,Barbara I.,Goddard W.A.,J Mol.Biol.,1998,280,913. 被引量:1
  • 3Banat B.M.A.,Kameyama Y.,Yoshioka T,Koga D.,Insect Biochem.Mol.Biol.,1999,29,537. 被引量:1
  • 4Peters G.,Saborowski R.,Buchholz E,Mentlein R.,Mar Biol.,1999,134,697. 被引量:1
  • 5Zou E.,Fingerman M.,Mol.Biol.,1999,133,97. 被引量:1
  • 6Xie X.L.,Chen Q.X.,Lin J.C.,Wang Y,Mar.Biol.,2004,146,143. 被引量:1
  • 7Zhang J.P.,Chen Q.X.,Wang Q.,Xie J.J.,Biochem.(Moscow),2006,71(Suppl.),55. 被引量:1
  • 8Jin Z.X.,Zhang J.P.,Yan Y.W.,Wang Q.,Appl.Biochem.Biotechnol.,2008,149,119. 被引量:1
  • 9Xie J.J.,Chen Q.X.,Zhang J.P,Wang Q.,Yang X.M.,Int.J.Biol.,Macromol.,2006,39,159. 被引量:1
  • 10Xie X.L.,Gong M.,Chen Q.X.,J.Enzym.Inhib.Meal Chem.,2006,21,55. 被引量:1
Chemical Research in Chinese Universities
2011年 第6期

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