A Novel, Q‐PCR Based Approach to Measuring Endogenous Retroviral Clearance by Capture Protein A Chromatography

Zhang, Min; Lute, Scott; Norling, Lenore A.; Hong, Connie; Safta, Aurelia; O’Connor, Deborah L.; Bernstein, L.; Wang, Hua; Blank, G.; Brorson, Kurt; Chen, Qi

doi:10.1002/bit.22172

Cited by 19 publications

(17 citation statements)

References 19 publications

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“…(Zhang et al, 2009;2014 through but decreased during washes. The studies performed here do not directly demonstrate such direct association but it is the simplest mechanism consistent with the data.…”

Section: Discussionmentioning

confidence: 93%

“…These methods have been used widely to study the separation of the product-and processrelated impurities Kelley et al, 2008;Sisodiya, Lequieu, Rodriguez, McDonald, & Lazzareschi, 2012;Wensel, Kelley, & Coffman, 2008). The limited application of HTS for virus clearance studies is likely due to the cost, complexity, and need for specialized labs, all of which can be overcome in scale-down protein A models using quantitative methods to measure CHO endogenous, noninfectious RVLP (M. Zhang et al, 2009Zhang et al, , 2014 | 847 hydrogen-bond, or combinations of these functional groups that reverse the effect. The limited application of HTS for virus clearance studies is likely due to the cost, complexity, and need for specialized labs, all of which can be overcome in scale-down protein A models using quantitative methods to measure CHO endogenous, noninfectious RVLP (M. Zhang et al, 2009Zhang et al, , 2014 | 847 hydrogen-bond, or combinations of these functional groups that reverse the effect.…”

Section: Introductionmentioning

confidence: 99%

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Characterizing and enhancing virus removal by protein A chromatography

Pan¹,

Becerra-Arteaga

Tran³

et al. 2019

Biotech & Bioengineering

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Protein A chromatography is an effective capture step to separate Fc-containing biopharmaceuticals from cell culture impurities but is generally not effective for virus removal, which tends to vary among different products. Previous findings have pointed to the differences in feedstocks to protein A, composed of the products and other cell culture-related impurities. To separate the effect of the feedstock components on virus removal, and understand why certain monoclonal antibody (mAb) products have low virus log reduction values (LRVs) across protein A chromatography, we investigated the partitioning of three types of viruses on Eshmuno® A columns. Using pure mAbs, we found that low LRVs were correlated with the presence of the particular mAb product itself, causing altered partitioning patterns. Three virus types were tested, and the trend in partitioning was the same for retrovirus-like particles (RVLPs) expressed in the cell substrate, and its model virus xenotropic murine leukemia virus (XMuLV), whereas slightly different for murine minute virus. These results were extended from previous observation described by Bach and Connell-Crowley (2015) studying XMuLV partitioning on MabSelect SuRe columns, providing further evidence using additional types of viruses and resin. Other product-specific cell culture impurities in harvested cell culture fluid played a lesser role in causing low LRVs. In addition, using high throughput screening (HTS) methods and Eshmuno® A resin plates, we identified excipients with ionic and hydrophobic properties that could potentially alleviate the mAb-induced LRV reduction, indicating that both ionic and hydrophobic interactions were involved. More excipients of such nature or combinations, once optimized, can potentially be used as load and/or wash additives to improve virus removal by protein A. We have demonstrated that HTS is a valuable tool for this type of screening, whether to gain deeper understanding of a mechanism, or to provide guidance during the optimization of protein A process with improved virus removal. K E Y W O R D S Chinese Hamster Ovary cells, Eshmuno ® A, high throughput screening (HTS), protein A chromatography, virus removal Biotechnology and Bioengineering. 2019;116:846-856. wileyonlinelibrary.com/journal/bit 846 | Abbreviations: CHO, Chinese Hamster Ovary; RVLP, retrovirus-like particles; HTS, high throughput screening; XMuLV, xenotropic murine leukemia virus; MMV, murine minute virus;RT-QPCR, real-time quantitative PCR; LRV, log reduction value. *Pan and Becerra-Arteaga have contributed equally to this study.

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Section: Discussionmentioning

confidence: 93%

Section: Introductionmentioning

confidence: 99%

Characterizing and enhancing virus removal by protein A chromatography

Pan¹,

Becerra-Arteaga

Tran³

et al. 2019

Biotech & Bioengineering

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“…For RVLP, the viral RNA was extracted using Qiagen EZ1 virus mini kit v2.0 with the EZ1/EZ1 advanced robotic system, according to vendor instructions. Free viral nucleic acids not associated with intact virus particles were removed based on the digestion procedures described earlier (Lute et al, ; Zhang et al, ) with slight modifications (10 μL DNase I, 40 μL of DNase I buffer, and 350 μL sample volume).…”

Section: Methodsmentioning

confidence: 99%

“…Such traditional full studies can be extremely expensive and time‐consuming to perform if using virus‐spiking to determine viral clearance capacity. Previous publications report comparable clearance when using QPCR assays that quantify either CHO endogenous retrovirus‐like particles (RVLP) or spiked X‐MuLV, and that retrovirus removal by Protein A could be evaluated by RVLP removal using samples from a Protein A process characterization studies (Zhang et al, ). In this report, we propose an experimentally determined QbD‐based approach for assessing viral clearance by Protein A chromatography.…”

Section: Introductionmentioning

confidence: 99%

Quality by design approach for viral clearance by protein a chromatography

Zhang¹,

Miesegaes²,

Lee³

et al. 2013

Biotech & Bioengineering

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Protein A chromatography is widely used as a capture step in monoclonal antibody (mAb) purification processes. Antibodies and Fc fusion proteins can be efficiently purified from the majority of other complex components in harvested cell culture fluid (HCCF). Protein A chromatography is also capable of removing modest levels of viruses and is often validated for viral clearance. Historical data mining of Genentech and FDA/CDER databases systematically evaluated the removal of model viruses by Protein A chromatography. First, we found that for each model virus, removal by Protein A chromatography varies significantly across mAbs, while remains consistent within a specific mAb product, even across the acceptable ranges of the process parameters. In addition, our analysis revealed a correlation between retrovirus and parvovirus removal, with retrovirus data generally possessing a greater clearance factor. Finally, we describe a multivariate approach used to evaluate process parameter impacts on viral clearance, based on the levels of retrovirus-like particles (RVLP) present among process characterization study samples. It was shown that RVLP removal by Protein A is robust, that is, parameter effects were not observed across the ranges tested. Robustness of RVLP removal by Protein A also correlates with that for other model viruses such as X-MuLV, MMV, and SV40. The data supports that evaluating RVLP removal using process characterization study samples can establish multivariate acceptable ranges for virus removal by the protein A step for QbD. By measuring RVLP instead of a model retrovirus, it may alleviate some of the technical and economic challenges associated with performing large, design-of-experiment (DoE)—type virus spiking studies. This approach could also serve to provide useful insight when designing strategies to ensure viral safety in the manufacturing of a biopharmaceutical product.

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“…This was first reported in 2009 by M. Zhang of Genentech Inc. (6) and expanded upon at the 2011 Symposium by M. Zhang (Session IV). It was reported that RVLP removal by protein A chromatography is comparable to that measured from spiked MuLV, and that RVLP removal determination can use full-scale samples.…”

Section: Cho Rvlp Assay Implementationmentioning

confidence: 79%