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Mechanistic model of minute virus of mice elution behavior in anion exchange chromatography purification

洗脱 小鼠微小病毒 化学 色谱法 离子色谱法 亲水作用色谱法 大小排阻色谱法 高效液相色谱法 病毒 生物化学 生物 病毒学 细小病毒科 病毒性疾病
作者
Ryunosuke Kitamura,Lena Enghauser,Riku Miyamoto,Takahiro Ichikawa,Takaki Aiso,Yumiko Masuda,Daisuke Kajihara,Hirofumi Kakihara,Koichi Nonaka
出处
期刊:Biotechnology Progress [American Chemical Society]
标识
DOI:10.1002/btpr.3516
摘要

Abstract This study aimed to propose a methodology for developing a mechanistic model for viral clearance of the minute virus of mice (MVM) on flow‐through anion exchange (AEX) chromatography. Protein surface analysis was applied to investigate the possibility of molecular interaction between the recombinant biotherapeutic and MVM. The protein product‐free Tris buffers were spiked with MVM, and the MVM elution profile from AEX chromatography was quantitatively analyzed using quantitative polymerase chain reaction (qPCR) for pooled fractions. GoSilico™ Chromatography Modeling Software was applied to develop the mechanistic models for MVM species. For evaluating the visual fit of the developed model, the R 2 of intact MVM virions and uncoated capsids between the simulated and measured amount in each fraction are 0.880 and 0.948, respectively. Response surface plots of logarithmic reduction values (LRV) against pH and conductivity in loaded sample were generated to show the range for suitable loaded sample conditions for achieving a good LRV. To evaluate the applicability of the developed MVM elution model to a recombinant biotherapeutic, two demonstrations of AEX chromatography purification were performed with a loaded sample of a model monoclonal antibody. The peaks of the MVM species in the elution step of both runs were accurately simulated by the developed model. In addition, to assess the possibility of molecular interaction between the virus and the target protein significantly affecting the MVM elution behavior, the antibody's surface was evaluated in terms of hydrophobicity/hydrophilicity using surface analysis.

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