| 一种改进的快速PCR定点突变技术 |
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| 引用本文: | 高川,韩维涛,宋云扬,张靖,王惠芳. 一种改进的快速PCR定点突变技术[J]. 生物技术通报, 2006, 0(3): 99-103 |
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| 作者姓名: | 高川 韩维涛 宋云扬 张靖 王惠芳 |
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| 作者单位: | 北京防化研究院第四研究室,北京,102205 |
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| 摘 要: | 在基因工程与蛋白质工程研究中常常用到基因突变技术制备突变体,用于研究基因调控、蛋白质的结构与功能。本项研究在快速PCR定点突变技术的基础上,改进实验方法,简化实验步骤,以适用蛋白质结构改造研究的需要。建立的突变技术仅需一次PCR反应即可完成基因的定点突变,突变效率为79.6%左右。该法对1~3个连续碱基的突变和对间隔4个甚至多达15个碱基的数个密码子突变效果都很好。
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| 关 键 词: | PCR反应 突变引物 基因 定点突变 |
| 收稿时间: | 2006-02-14 |
| 修稿时间: | 2006-02-14 |
A Technique of Improved Rapid Site-directed Mutagenesis |
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| Gao Chuan,Han Weitao,Song Yunyang,Zhang Jiang,Wang Huifang. A Technique of Improved Rapid Site-directed Mutagenesis[J]. Biotechnology Bulletin, 2006, 0(3): 99-103 |
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| Authors: | Gao Chuan Han Weitao Song Yunyang Zhang Jiang Wang Huifang |
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| Affiliation: | The fourth department of research institute of defence chemistry, Beijing 102205 |
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| Abstract: | Mutants prepared by mutagenesis methods are usually used to study gene regulations,gene expressions and the structure-function relationships of proteins in gene engineering and protein engineering.In this study,we focus on establishing a new gene mutation technique,improving the experimental conditions and expanding the practical extents for meeting the demands of engineered protein structures.The target genes were inserted into the cloning vectors-plasmids.The mutation was completed only by one step PCR reaction using a double-stranded DNA template and double-mutation primers catalyzed by Taq plus DNA polymerase.After the DNA template was digested by a restriction endonuclease,the vectors were introduced into host cells and the target genes with mutations were expressed by using host cells' transcription and translation mechanism.The mutation rate was 79.6%.This method was effective for the mutation of 1~3 continuous bases and of a few codons spaced by several bases. |
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| Keywords: | PCR reaction Mutation primer Gene Site-directed mutagenesis |
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