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产黄青霉内切鼠李糖半乳糖醛酸酶的生化特性及过表达

Biochemical Characterization and Overexpression of an Endo-rhamnogalacturonan Lyase from Penicillium chrysogenum.

作者信息

Iwai Marin, Yamada Hiroyuki, Ikemoto Takeshi, Matsumoto Shotaro, Fujiwara Daisuke, Takenaka Shigeo, Sakamoto Tatsuji

机构信息

Division of Applied Life Sciences, Graduate School of Life and Environmental Sciences, Osaka Prefecture University, Sakai, Osaka, 599-8531, Japan.

出版信息

Mol Biotechnol. 2015 Jun;57(6):539-48. doi: 10.1007/s12033-015-9847-4.

Abstract

Rhamnogalacturonan lyase (PcRGL4A) was purified from the culture supernatant of Penicillium chrysogenum 31B. PcRGL4A optimal activity occurred between pH 7-8 and at 40 °C. Conserved Domain Search analysis identified PcRGL4A as a member of Polysaccharide Lyase family 4. PcRGL4A contains two conserved catalytic and four conserved substrate-binding residues as determined by X-ray crystallography of the Aspergillus aculeatus RG lyase. Recombinant PcRGL4A (rPcRGL4A) expressed in Escherichia coli demonstrated specific activity against rhamnogalacturonan (RG) but not homogalacturonan. Analysis of the RG reaction products by high-performance anion-exchange chromatography revealed that rPcRGL4A cleaved the substrate in an endo-manner and that the major final product was an RG tetrasaccharide with 4-deoxy-4,5-unsaturated galacturonic acid at the nonreducing end. Based on these results, PcRGL4A was classified as an endo-acting RG lyase (EC 4.2.2.23). Divalent cations were not essential for the enzymatic activity of rPcRGL4A, but addition of calcium ions to the reaction mixture increased enzymatic activity. rPcRGL4A demonstrated a preference for RG lacking galactose decoration.

摘要

鼠李半乳糖醛酸裂解酶(PcRGL4A)是从产黄青霉31B的培养上清液中纯化得到的。PcRGL4A的最佳活性出现在pH 7 - 8和40℃条件下。保守结构域搜索分析确定PcRGL4A为多糖裂解酶家族4的成员。通过棘孢曲霉RG裂解酶的X射线晶体学分析确定,PcRGL4A含有两个保守的催化残基和四个保守的底物结合残基。在大肠杆菌中表达的重组PcRGL4A(rPcRGL4A)对鼠李半乳糖醛酸聚糖(RG)具有特异性活性,但对同型半乳糖醛酸聚糖无活性。通过高效阴离子交换色谱对RG反应产物进行分析,结果显示rPcRGL4A以内切方式切割底物,主要终产物是一种在非还原端带有4 - 脱氧 - 4,5 - 不饱和半乳糖醛酸的RG四糖。基于这些结果,PcRGL4A被归类为一种内切型RG裂解酶(EC 4.2.2.23)。二价阳离子对rPcRGL4A的酶活性不是必需的,但向反应混合物中添加钙离子可提高酶活性。rPcRGL4A表现出对缺乏半乳糖修饰的RG的偏好。

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