生物技术通报 ›› 2022, Vol. 38 ›› Issue (5): 183-190.doi: 10.13560/j.cnki.biotech.bull.1985.2021-1210

• 研究报告 • 上一篇    下一篇

Kod DNA聚合酶的制备及纯化研究

易芳(), 来鹏程, 郑希鳌, 胡帅, 高燕丽()   

  1. 浙江农林大学,杭州 311300
  • 收稿日期:2021-09-19 出版日期:2022-05-26 发布日期:2022-06-10
  • 作者简介:易芳,女,硕士研究生,研究方向:植物分子生物学;E-mail: 309382275@qq.com
  • 基金资助:
    浙江农林大学校科研发展基金项目(203402018701)

Research on the Preparation and Purification of Kod DNA Polymerase

YI Fang(), LAI Peng-cheng, ZHENG Xi-ao, HU Shuai, GAO Yan-li()   

  1. Zhejiang Agriculture and Forestry University,Hangzhou 311300
  • Received:2021-09-19 Published:2022-05-26 Online:2022-06-10

摘要:

Kod DNA聚合酶作为常见的高保真DNA聚合酶,具有较强的DNA延伸能力以及3'-5'外切核酸酶校正活性。本研究通过对重组Kod DNA聚合酶分离纯化条件的优化,以期提高其表达和纯化效率以及片段扩增能力。利用异丙基硫代-β-D-半乳糖苷(isopropyl β-D-thiogalactoside,IPTG)对pET-30a-Kod进行诱导表达后,利用酶溶法和超声波破碎法对细胞破碎并提取粗酶液,然后利用Ni-NTA柱洗脱纯化获得较纯Kod DNA酶,再经透析得到高纯度Kod DNA酶,利用PCR反应和Sanger测序手段来检测自提纯化的Kod DNA聚合酶活性及保真性。同时,本研究对IPTG浓度和洗脱液中咪唑浓度等重要参数进行优化。结果表明,在28℃条件下0.1 mmol/L IPTG诱导16-18 h后,Kod DNA聚合酶高效表达;当咪唑浓度为200 mmol/L时蛋白洗脱效果最佳。PCR反应体系中Mg2+浓度为1.5 mmol/L,Kod DNA聚合酶浓度为0.061 25 μg/µL时,Kod DNA聚合酶效率较高,能有效地扩增3 194 bp的目的条带;通过序列比对,PCR产物序列中未引入任何突变。经优化制备后的Kod DNA聚合酶在酶活性和扩增保真性上均能达到商用高保真DNA聚合酶水平。本研究为节省实验室PCR成本,进一步开发和利用Kod DNA聚合酶奠定一定的基础。

关键词: DNA聚合酶, 聚合酶链式反应(PCR), Kod DNA聚合酶, 蛋白质纯化

Abstract:

Kod DNA polymerase,as a common high-fidelity DNA polymerase,has strong DNA extension ability and 3'-5' exonuclease activities. This study is aimed to improve the expression efficiency and extension ability as well as fragment amplification ability by optimizing the isolation and purification conditions of recombinant Kod DNA polymerase. First,isopropyl β-D-thiogalactoside(IPTG)was used to induce pET-30a-Kod for expression,and enzymatic dissolution and ultrasonic fragmentation were to grind the cells and extract the crude enzyme solution,then Ni-NTA column was to elute and purify the Kod DNA polymerase. Finally,the high-purity Kod DNA polymerase was obtained by dialysis. PCR and Sanger sequencing were used to detect the activity and fidelity of self-purified Kod DNA polymerase. Meanwhile the key parameters such as IPTG and imidazole concentrations were optimized. The results showed that Kod DNA polymerase was highly expressed after induced by 0.1 mmol/L IPTG at 28℃ for 16-18 h,and the eluted effect was optimal while imidazole concentration was 200 mmol/L. The efficiency of the Kod DNA polymerase was the highest while Mg2+ was 1.5 mmol/L and Kod DNA polymerase was 0.061 25 μg/µL in the PCR reaction system,under which 3 194 bp target band was efficiently amplified;and there was no introduced mutation in the PCR product after sequence alignment. The enzymatic activity and fidelity of self-extracted Kod DNA polymerase after optimized preparation reached the same level of commercial high-fidelity DNA polymerase. Thus,this study lays a foundation for saving the cost of laboratory PCR and further developing and utilizing Kod DNA polymerase.

Key words: DNA polymerase, polymerase chain reaction(PCR), Kod DNA polymerase, protein purification