On-column disulfide bond formation of monoclonal antibodies during Protein A chromatography eliminates low molecular weight species and rescues reduced antibodies

Disulfide bond reduction, which commonly occurs during monoclonal antibody (mAb) manufacturing processes, can result in a drug substance with high levels of low molecular weight (LMW) species that may fail release specifications because the drug’s safety and the efficiency may be affected by the pre...

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Autores principales: Tan, Zhijun, Ehamparanathan, Vivekh, Ren, Tingwei, Tang, Peifeng, Hoffman, Laurel, Kuang, June, Liu, Peiran, Huang, Chao, Du, Cheng, Tao, Li, Chemmalil, Letha, Lewandowski, Angela, Ghose, Sanchayita, Li, Zheng Jian, Liu, Shijie
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Taylor & Francis 2020
Materias:
Report
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7577237/
https://www.ncbi.nlm.nih.gov/pubmed/33016217
http://dx.doi.org/10.1080/19420862.2020.1829333
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author Tan, Zhijun
Ehamparanathan, Vivekh
Ren, Tingwei
Tang, Peifeng
Hoffman, Laurel
Kuang, June
Liu, Peiran
Huang, Chao
Du, Cheng
Tao, Li
Chemmalil, Letha
Lewandowski, Angela
Ghose, Sanchayita
Li, Zheng Jian
Liu, Shijie
author_facet Tan, Zhijun
Ehamparanathan, Vivekh
Ren, Tingwei
Tang, Peifeng
Hoffman, Laurel
Kuang, June
Liu, Peiran
Huang, Chao
Du, Cheng
Tao, Li
Chemmalil, Letha
Lewandowski, Angela
Ghose, Sanchayita
Li, Zheng Jian
Liu, Shijie
author_sort Tan, Zhijun
collection PubMed
description Disulfide bond reduction, which commonly occurs during monoclonal antibody (mAb) manufacturing processes, can result in a drug substance with high levels of low molecular weight (LMW) species that may fail release specifications because the drug’s safety and the efficiency may be affected by the presence of this material. We previously studied disulfide reoxidation of mAbs and demonstrated that disulfide bonds could be reformed from the reduced antibody via redox reactions under an optimal redox condition on Protein A resin. The study here implements a redox system in a manufacturing setting to rescue the reduced mAb product and to further eliminate LMW issues in downstream processing. As such, we incorporate the optimized redox system as one of the wash buffers in Protein A chromatography to enable an on-column disulfide reoxidation to form intact antibody in vitro. Studies at laboratory scale (1 cm (ID) x 20 cm (Height), MabSelect SuRe LX) and pilot scale (30 cm (ID) x 20 cm (Height), MabSelect SuRe LX) were performed to demonstrate the effectiveness and robustness of disulfide formation with multiple mAbs using redox wash on Protein A columns. By applying this rescue strategy using ≤50 g/L-resin loading, the intact mAb purity was improved from <5% in the Protein A column load to >90% in the Protein A column elution with a product yield of >90%. Studies were also done to confirm that adding the redox wash has no negative impact on process yield or impurity removal or product quality. The rescued mAbs were confirmed to form complete interchain disulfide bonds, exhibiting comparable biophysical properties to the reference material. Furthermore, since the redox wash is followed by a bridging buffer wash before the final elution, no additional burden is involved in removing the redox components during the downstream steps. Due to its ease of implementation, significant product purity improvement, and minimal impact on other product quality attributes, we demonstrate that the on-column reoxidation using a redox system is a powerful, simple, and safe tool to recover reduced mAb during manufacturing. Moreover, the apparent benefits of using a high-pH redox wash may further drive the evolution of Protein A platform processes.
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spelling pubmed-75772372020-10-28 On-column disulfide bond formation of monoclonal antibodies during Protein A chromatography eliminates low molecular weight species and rescues reduced antibodies Tan, Zhijun Ehamparanathan, Vivekh Ren, Tingwei Tang, Peifeng Hoffman, Laurel Kuang, June Liu, Peiran Huang, Chao Du, Cheng Tao, Li Chemmalil, Letha Lewandowski, Angela Ghose, Sanchayita Li, Zheng Jian Liu, Shijie MAbs Report Disulfide bond reduction, which commonly occurs during monoclonal antibody (mAb) manufacturing processes, can result in a drug substance with high levels of low molecular weight (LMW) species that may fail release specifications because the drug’s safety and the efficiency may be affected by the presence of this material. We previously studied disulfide reoxidation of mAbs and demonstrated that disulfide bonds could be reformed from the reduced antibody via redox reactions under an optimal redox condition on Protein A resin. The study here implements a redox system in a manufacturing setting to rescue the reduced mAb product and to further eliminate LMW issues in downstream processing. As such, we incorporate the optimized redox system as one of the wash buffers in Protein A chromatography to enable an on-column disulfide reoxidation to form intact antibody in vitro. Studies at laboratory scale (1 cm (ID) x 20 cm (Height), MabSelect SuRe LX) and pilot scale (30 cm (ID) x 20 cm (Height), MabSelect SuRe LX) were performed to demonstrate the effectiveness and robustness of disulfide formation with multiple mAbs using redox wash on Protein A columns. By applying this rescue strategy using ≤50 g/L-resin loading, the intact mAb purity was improved from <5% in the Protein A column load to >90% in the Protein A column elution with a product yield of >90%. Studies were also done to confirm that adding the redox wash has no negative impact on process yield or impurity removal or product quality. The rescued mAbs were confirmed to form complete interchain disulfide bonds, exhibiting comparable biophysical properties to the reference material. Furthermore, since the redox wash is followed by a bridging buffer wash before the final elution, no additional burden is involved in removing the redox components during the downstream steps. Due to its ease of implementation, significant product purity improvement, and minimal impact on other product quality attributes, we demonstrate that the on-column reoxidation using a redox system is a powerful, simple, and safe tool to recover reduced mAb during manufacturing. Moreover, the apparent benefits of using a high-pH redox wash may further drive the evolution of Protein A platform processes. Taylor & Francis 2020-10-04 /pmc/articles/PMC7577237/ /pubmed/33016217 http://dx.doi.org/10.1080/19420862.2020.1829333 Text en © 2020 The Author(s). Published with license by Taylor & Francis Group, LLC. https://creativecommons.org/licenses/by-nc/4.0/This is an Open Access article distributed under the terms of the Creative Commons Attribution-NonCommercial License (http://creativecommons.org/licenses/by-nc/4.0/ (https://creativecommons.org/licenses/by-nc/4.0/) ), which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Report
Tan, Zhijun
Ehamparanathan, Vivekh
Ren, Tingwei
Tang, Peifeng
Hoffman, Laurel
Kuang, June
Liu, Peiran
Huang, Chao
Du, Cheng
Tao, Li
Chemmalil, Letha
Lewandowski, Angela
Ghose, Sanchayita
Li, Zheng Jian
Liu, Shijie
On-column disulfide bond formation of monoclonal antibodies during Protein A chromatography eliminates low molecular weight species and rescues reduced antibodies
title On-column disulfide bond formation of monoclonal antibodies during Protein A chromatography eliminates low molecular weight species and rescues reduced antibodies
title_full On-column disulfide bond formation of monoclonal antibodies during Protein A chromatography eliminates low molecular weight species and rescues reduced antibodies
title_fullStr On-column disulfide bond formation of monoclonal antibodies during Protein A chromatography eliminates low molecular weight species and rescues reduced antibodies
title_full_unstemmed On-column disulfide bond formation of monoclonal antibodies during Protein A chromatography eliminates low molecular weight species and rescues reduced antibodies
title_short On-column disulfide bond formation of monoclonal antibodies during Protein A chromatography eliminates low molecular weight species and rescues reduced antibodies
title_sort on-column disulfide bond formation of monoclonal antibodies during protein a chromatography eliminates low molecular weight species and rescues reduced antibodies
topic Report
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7577237/
https://www.ncbi.nlm.nih.gov/pubmed/33016217
http://dx.doi.org/10.1080/19420862.2020.1829333
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