生物技术通报 ›› 2015, Vol. 31 ›› Issue (12): 75-80.doi: 10.13560/j.cnki.biotech.bull.1985.2015.12.011

• 技术与方法 • 上一篇    下一篇

两步串联层析法纯化抗TNF-α 单克隆抗体

杨辉,杨彬,马旭通,孙文正,林小鹊,谭世杰   

  1. 广东东阳光药业有限公司,东莞 523000
  • 收稿日期:2015-03-29 出版日期:2015-12-19 发布日期:2015-12-19
  • 作者简介:杨辉,男,硕士,研究方向:生物技术药物;E-mail:highman52@163.com;杨彬同为本文第一作者
  • 基金资助:
    广东省引进创新科研团队计划(201101Y0104990178)

A Two-step Series Chromatography for the Purification of Anti-TNF-α Monoclonal Antibody

Yang Hui, Yang Bin, Ma Xutong, Sun Wenzheng, Lin Xiaoque, Tan Shijie   

  1. Sunshine Lake Pharma Co.,Ltd,Dongguan 523000
  • Received:2015-03-29 Published:2015-12-19 Online:2015-12-19

摘要: 旨在建立从重组CHO细胞发酵培养液中纯化抗TNF-α单克隆抗体的两步串联层析法。将含有抗TNF-α单克隆抗体的料液经两次离心、一步过滤的预处理后,用protein A填料捕获,阳离子填料Sourec30精细纯化。精细纯化过程中利用DoE的方法,采用CCF(Central composite face)设计,探讨了洗脱pH值及盐浓度对纯化的影响。纯化后的抗TNF-α单克隆抗体经HPLC以及毛细管电泳,检测其浓度、纯度以及多聚体含量。结果显示,亲和层析的最佳洗脱条件为pH4.0。通过DOE优化,为达到质量目标(回收率90%以上,纯度97%以上,多聚体0.3%),筛选出最佳洗脱范围为0.05-0.13 mol/L NaCl以及pH5.7-6.0,选定pH6.0与0.10 mol/L NaCl作为Source洗脱条件,此时回收率94.3%,纯度97.3%,多聚体0.3%,其质量与参比制剂接近。

关键词: 两步抗体纯化平台, 抗TNF-α单克隆抗体, 亲和层析, 阳离子交换层析

Abstract: The objective of this work is to establish a two-step series chromatography method for purification of anti-TNF-α monoclonal antibodies(mAbs)from recombinant CHO cell culture medium. Anti-TNF-α mAbs from harvested cell culture fluid(HCCF)after 2 times centrifugation and 1 filtration were captured using filler of protein A, from which the eluant was then further finely purified using the positive ion filler Source30 resin. During fine purification, the effects of pH and salt concentration of the Source30 on the purification was investigated using the DoE method and CCF(Central Composite Face)to achieve the optimal mAbs recovery and purity as well as the lowest aggregate content. The concentration and aggregation ratio of the purified mAbs were determined by HPLC and the purity by CE-SDS. Results were as the followings. The optimal elution pH for protein A affinity chromatography was 4.0. After DoE optimization, in order to reach the quality target(> 90% recovery, > 97% purity, and < 0.3% aggregate), the optimal elution range was 0.05-0.13 mol/L NaCl at pH 5.7-6.0. The elution buffer containing 0.10 mol/L NaCl at pH 6.0 was chosen as the optimal condition of Source elution with 94.3% product recovery, 97.3% purity, and 0.3% aggregate, i. e. , very close to those in the reference standard. In conclusion, we have successfully developed and optimized a two-step series chromatography method at the laboratory scale for the purification of anti-TNF-α mAbs with high recovery, high purity, and low aggregate content.

Key words: two-step chromatography antibody purification platform, anti-TNF-α monoclonal antibody, affinity chromatography, cation exchange chromatography