籽粒苋C<sub>4</sub>关键酶丙酮酸磷酸双激酶基因的原核表达及酶活性测定

doi:10.7668/hbnxb.2017.02.010

华北农学报 ›› 2017, Vol. 32 ›› Issue (2): 61-65. doi: 10.7668/hbnxb.2017.02.010

所属专题： 生物技术；

籽粒苋C₄关键酶丙酮酸磷酸双激酶基因的原核表达及酶活性测定

贺飞燕¹, 闫建俊², 白云凤², 冯瑞云², 张维锋²

1. 山西大学生物工程学院, 山西太原 030006;
2. 山西省农业科学院作物科学研究所, 作物遗传与分子改良山西省重点实验室, 农业部黄土高原作物基因资源与种质创制重点实验室, 山西太原 030031

收稿日期:2017-02-03 出版日期:2017-04-28
通讯作者: 白云凤(1957-),女,山西吕梁人,研究员,博士,硕士生导师,主要从事植物分子遗传和改良研究。
作者简介:贺飞燕(1991-),女,山西临汾人,在读硕士,主要从事植物分子育种研究。
基金资助:
国家自然科学基金项目（30971838）；山西省自然科学基金项目（201601D011075）

Prokaryotic Expression and Enzyme Activity Determination of C₄ Key Enzyme Pyruvate Phosphate Dikinase Gene in Amaranth hypochondriacus

HE Feiyan¹, YAN Jianjun², BAI Yunfeng², FENG Ruiyun², ZHANG Weifeng²

1. College of Bioengineering, Shanxi University, Taiyuan 030006, China;
2. Institute of Crop Science, Shanxi Academy of Agricultural Sciences, Shanxi Province Key Laboratory of Crop Genetics and Molecular Improvement, Key Laboratory of Loess Plateau Crop Gene Resources and Germplasm Creation, Ministry of Agriculture, Taiyuan 030031, China

Received:2017-02-03 Published:2017-04-28

摘要/Abstract

摘要： 为了进一步探究籽粒苋丙酮酸磷酸双激酶（AhPPDK）蛋白的作用机制，构建了AhPPDK基因的原核表达载体，通过碱裂解提取质粒，经限制性内切酶酶切，采用1.0%琼脂糖凝胶电泳检测酶切产物，选择正确表达的阳性重组子，将测序正确的重组质粒pEASY-E1-AhPPDK转化菌株Transetta（DE3）；利用IPTG诱导蛋白表达。SDS-PAGE凝胶电泳分析表明，重组AhPPDK能在大肠杆菌Transset（DE3）中高效表达，表达的重组蛋白质分子量约为108 kDa，与预期分子量相符，且为可溶性蛋白。利用紫外分光光度法测量结果表明，原核表达的AhPPDK具有酶活性，且上清粗酶液活性高于沉淀粗酶液。研究结果可为进一步探明AhPPDK蛋白的作用机制和转基因利用奠定基础。

关键词: 籽粒苋, AhPPDK, 原核表达, 酶活测定

Abstract: To further explore the mechanism of action of AhPPDK protein,the prokaryotic expression vector of AhPPDK gene was constructed.The plasmid was extracted by alkaline lysis,digested with restriction endonuclease,detected with 1.0% Agarose gel.The correct recombinant plasmid pEASY-E1-AhPPDK was transformed into E. coli Transset (DE3),and the recombinant protein was induced by IPTG.SDS-PAGE analysis showed that recombinant AhPPDK could be highly expressed in E. coli Transset (DE3).The expressed recombinant protein had a molecular weight of 108 kDa,which was consistent with the expected molecular weight and was soluble protein.Pyruvate formed by pyruvate phosphodiesterase (PPDK)catalyzes the formation of lactate by excess lactate dehydrogenase and oxidizes reduced coenzyme I (NADH).Using ultraviolet spectrophotometry,the amount of NADH could be calculated according to the change of OD value at 340 nm,and then the activity of PPDK could be deduced.Spectrophotometric method showed that the prokaryotic expression of AhPPDK had the activity of enzyme.These results provide a basis for the further study on the mechanism of action of AhPPDK and the use of transgenes.

Key words: Amaranth hypochondriacus, AhPPDK, Prokaryotic expression, Enzyme activity determination

中图分类号:

S330
Q78

贺飞燕, 闫建俊, 白云凤, 冯瑞云, 张维锋. 籽粒苋C₄关键酶丙酮酸磷酸双激酶基因的原核表达及酶活性测定[J]. 华北农学报, 2017, 32(2): 61-65. doi: 10.7668/hbnxb.2017.02.010.

HE Feiyan, YAN Jianjun, BAI Yunfeng, FENG Ruiyun, ZHANG Weifeng. Prokaryotic Expression and Enzyme Activity Determination of C₄ Key Enzyme Pyruvate Phosphate Dikinase Gene in Amaranth hypochondriacus[J]. ACTA AGRICULTURAE BOREALI-SINICA, 2017, 32(2): 61-65. doi: 10.7668/hbnxb.2017.02.010.

http://www.hbnxb.net/CN/Y2017/V32/I2/61

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籽粒苋C4关键酶丙酮酸磷酸双激酶基因的原核表达及酶活性测定

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籽粒苋C₄关键酶丙酮酸磷酸双激酶基因的原核表达及酶活性测定

Prokaryotic Expression and Enzyme Activity Determination of C₄ Key Enzyme Pyruvate Phosphate Dikinase Gene in Amaranth hypochondriacus