Chromatographic removal combined with heat, acid and chaotropic inactivation of four model viruses

Valdés, Rodolfo; Ibarra, Neysi; Ruibal, Ignacio; Beldarraín, Alejandro; Noa, Enrique; Herrera, Nancy D.; Alemán, Rosario; Padilla, Sigifredo; García, J.; Perez, Marisol; Morales, Raul Junta; Chong, Eric Tzyy Jiann; Reyes, Biunayki; Quiñones, Y.; Agraz, Alberto; Herrera, Luís

doi:10.1016/s0168-1656(02)00047-0

Cited by 18 publications

(13 citation statements)

References 7 publications

(6 reference statements)

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“…The clearance results obtained using both assays, in both the process characterization and resin reuse studies were similar. Overall, the combined data provide confirmation that protein A is a robust virus removal step (Brorson et al, 2003a;Valdes et al, 2002).…”

Section: Discussionmentioning

confidence: 56%

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

Zhang

Lute

Norling

et al. 2008

Biotech & Bioengineering

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Quantification of virus removal by the purification process during production is required for clinical use of biopharmaceuticals. The current validation approach for virus removal by chromatography steps typically involves time-consuming spiking experiments with expensive model viruses at bench scale. Here we propose a novel, alternative approach that can be applied in at least one instance: evaluating retroviral clearance by protein A chromatography. Our strategy uses a quantitative PCR (Q-PCR) assay that quantifies the endogenous type C retrovirus-like particle genomes directly in production Chinese Hamster Ovary (CHO) cell culture harvests and protein A pools. This eliminates the need to perform spiking with model viruses, and measures the real virus from the process. Using this new approach, clearance values were obtained that was comparable to those from the old model-virus spike/removal approach. We tested the concept of design space for CHO retrovirus removal using samples from a protein A characterization study, where a wide range of chromatographic operating conditions were challenged, including load density, flow rate, wash, pooling, temperature, and resin life cycles. Little impact of these variables on CHO retrovirus clearance was found, arguing for implementation of the design space approach for viral clearance to support operational ranges and manufacturing excursions. The viral clearance results from Q-PCR were confirmed by an orthogonal quantitative product-enhanced reverse transcriptase (Q-PERT) assay that quantifies CHO retrovirus by their reverse transcriptase (RT) enzyme activity. Overall, our results demonstrate that protein A chromatography is a robust retrovirus removal step and CHO retrovirus removal can be directly measured at large scale using Q-PCR assays.

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Section: Discussionmentioning

confidence: 56%

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

Zhang

Lute

Norling

et al. 2008

Biotech & Bioengineering

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“…For example, the ability of the S-Q-HIC, S-Q-ABx, and S-ABx-Q processes to remove host cell DNA, small molecules, and antibody variants must be evaluated, and process robustness and process economics must be investigated. Many of these chromatography steps may not provide as much virus clearance as protein A but several alternative methods, such as filtration or chemical inactivation, may be employed [18,19,31,32]. Although most of the resins are stable to sodium hydroxide, resin cleanability must be investigated.…”

Section: Resultsmentioning

confidence: 99%

“…Affinity chromatography also provides significant virus clearance [18,19]. Because it binds a variety of mammalian IgG molecules [20], protein A affinity chromatography also allows process harmonization for multi-product manufacturing.…”

Section: Introductionmentioning

confidence: 99%

Factorial screening of antibody purification processes using three chromatography steps without protein A

Follman¹,

Fahrner²

2004

Journal of Chromatography A

199

121

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“…After this chromatography, incubation in 0.1 molar (M) citric acid pH 3.0 for an hour at 4°C was carried out. The ultra filtration and sterile filtration steps complete the basic diagram of the purification process [4].…”

Section: Inoculum Preparationmentioning

confidence: 99%

“Quality Tools for Improving a System of documentation as the basis for Good Manufacturing Practices”. Practical Case

Díaz¹,

Dominguez²,

Díaz³

et al. 2011

Pharm Anal Acta

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The documentation system is one of the mandatory elements reviewed during inspections of any regulatory agency. Generally, 20 to 30 percent of the deviations detected in a pharmaceutical inspection, are directly related to the documentation of quality system in each of the components or systems inspected. Given that no regulation on GMP will tell us in detail how the documentation system should be, we aimed to show in this work an approach used to implement some of the quality tools for establishment and maintenance of GMP and inherent Documentation in order to comply with the normative, national and international regulations typical of a productive process monoclonal antibody (MAb) which is secreted by the hybridoma 48/1/5/4, specific for the "a" determinant of the Hepatitis B surface antigen (HBsAg). This MAb is routinely used as reagents for the purification of vaccines.

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Chromatographic removal combined with heat, acid and chaotropic inactivation of four model viruses

Cited by 18 publications

References 7 publications

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

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

Factorial screening of antibody purification processes using three chromatography steps without protein A

“Quality Tools for Improving a System of documentation as the basis for Good Manufacturing Practices”. Practical Case

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