生物技术通报 ›› 2016, Vol. 32 ›› Issue (7): 170-177.doi: 10.13560/j.cnki.biotech.bull.1985.2016.07.025

• 研究报告 • 上一篇    下一篇

漆酶Lac1338的酶学特性测定及定向突变对其酶解染料影响

张雪玲,陈小利,李荷   

  1. 广东药学院基础学院生物化学与分子生物学系,广州 510006
  • 收稿日期:2015-09-24 出版日期:2016-07-25 发布日期:2016-07-25
  • 作者简介:张雪玲,女,硕士研究生,研究方向:利用宏基因组学的方法筛选新型纤维素酶;E-mail:1095199175@qq.com
  • 基金资助:
    广东省科技厅项目(2012B010300021,2013B010404044),广东省教育厅项目(2013KJCX0107)

Determination of Enzymatic Properties of a Laccase Lac1338,and Effects of Directed Mutants on the Degradations of Different Dyes

ZHANG Xue-ling CHEN Xiao-li LI He   

  1. Department of Biochemistry & Molecular Biology,School of Basic Courses,Guangdong Pharmaceutial University,Guangzhou 510006
  • Received:2015-09-24 Published:2016-07-25 Online:2016-07-25

摘要: 为了获得表达量高、热稳定性好的漆酶,通过密码子优化合成漆酶基因lac1338、连接到pET-32a(+)载体上并在Escherichia coli BL21(DE3)中表达,获得HIS-Lac1338蛋白。酶学性质测定结果显示,以ABTS为底物时,HIS-Lac1338的比活力高达22.8 U/mg,Km 和Vmax 分别为567 μmol/L 和2.8 mmol/ (L·min·g);HIS-Lac1338的最适反应温度为55℃,最适pH为6.0;在55℃以下保温2 h能保留50%的酶活性,在pH 4-8范围内孵育4 h仍保留50%以上的活性;HIS-Lac1338对Cu2+抗性强,Ca2+、Na+、K+对HIS-Lac1338有促进作用,而Co2+、Fe2+、Hg2+、Ag+等重金属离子对HIS-Lac1338有抑制作用。易错PCR方法得到的Lac1338的突变酶Lac16与HIS-Lac1338相比,对酸性紫7、溴酚蓝、考马斯亮蓝的降解率分别由10.9%、20%和25%提高到90.5%、67.8%和85%。结果表明,HIS-Lac1338具有较好的温度及pH稳定性,而通过易错PCR技术定向突变获得的突变酶Lac16的染料降解率大大提高。

关键词: 漆酶, 克隆表达, 酶学性质, 定向进化, 染料降解

Abstract: In order to obtain the laccase with high expression and high thermal stability,a laccase gene lac1338 synthesized was cloned by codon optimization,ligated to the vector pET-32a(+),then expressed in Escherichia coli BL21(DE3),and the recombinant protein HIS-Lac1338 was obtained. Its enzymatic properties showed that while using ABTS as a substrate,the specific activity of HIS-Lac1338 was up to 22.8 U/mg,Km and Vmax of HIS-Lac1338 was 567 μmol/L and 2.8 mmol/(min·g protein),respectively. The optimal temperature and pH of HIS-Lac1338 were 55℃ and 6.0 respectively. Its activity remained 50% at 55℃ for 2 h and in the pH range of 4-8. HIS-Lac1338 was strongly resistant to Cu2+,while its activity was promoted by Ca2+,Na+,K+ and inhibited by heavy metal ions such as Co2+,Fe2+,Hg2+,Ag+,etc. Comparing with HIS-Lac1338,mutant enzyme Lac16 of Lac1338 by sequential error-prone PCR improved the degradation rates of Acidviolet 7,Bromophenol blue,and Coomssie brilliant blue from 10.9%,20%,and 25% to 90.5%,67.8%,and 85%,respectively. Above results reveal that HIS-Lac1338 is stable to temperature and pH,the degradation rate of dye increases greatly with the mutant enzyme Lac16 via directed evolution of sequential error-prone PCR.

Key words: laccase, cloning and expression, enzymatic properties, directed evolution, degradation to dyes