Real Time Quantitative PCR as a Method to Evaluate Simian Virus 40 Removal During Pharmaceutical Protein Purification

Real Time Quantitative PCR as a Method to Evaluate Simian Virus 40 Removal During Pharmaceutical Protein Purification

Continuous cell lines used for pharmaceutical protein manufacturing have the potential to be contaminated by viruses. To ensure the safety of pharmaceutical proteins derived from continuous cell lines, validation of the ability of the manufacturing process to clear potential contaminating viruses is...

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Veröffentlicht in:Biologicals 1999-09, Vol.27 (3), p.253-262
Hauptverfasser: Shi, Liming, Norling, Lenore A., Lau, Allen S.L., Krejci, Sherrie, Laney, Alison J., Xu, Yuan
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Sprache:eng
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Antibodies, Monoclonal - isolation & purification
Chromatography - methods
Drug Contamination
Drug Industry - methods
Polymerase Chain Reaction - methods
Recombinant Proteins - isolation & purification
Simian virus 40
Simian virus 40 - isolation & purification
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container_end_page 262
container_issue 3
container_start_page 253
container_title Biologicals
container_volume 27
creator Shi, Liming
Norling, Lenore A.
Lau, Allen S.L.
Krejci, Sherrie
Laney, Alison J.
Xu, Yuan
description Continuous cell lines used for pharmaceutical protein manufacturing have the potential to be contaminated by viruses. To ensure the safety of pharmaceutical proteins derived from continuous cell lines, validation of the ability of the manufacturing process to clear potential contaminating viruses is required for product registration. In this paper, a real time quantitative PCR method has been applied to the evaluation of simian virus 40 (SV40) removal during chromatography and filtration procedures. This method takes advantage of the 5′-3′ exonuclease activity of Taq DNA polymerase and utilizes the PRISMTM7700 sequence detection system of PE Applied Biosystems for automated SV40 DNA quantification through a dual-labeled fluorogenic probe. This method provides accurate and reproducible quantification of SV40 DNA. The SV40 clearance during chromatography and filtration procedures determined by this method is highly comparable with that determined by the cell-based infectivity assay. This method offers significant advantages over cell-based infectivity assays, such as higher sensitivity, greater reliability, higher sample throughput and lower cost. This method can be potentially used to evaluate the clearance of all model viruses during chromatography and filtration procedures. This method can be used to substitute cell-based infectivity assays for process validation of viral removal procedures and the availability of this method should greatly facilitate and reduce the cost of viral clearance evaluations required for new biologic product development.
doi_str_mv 10.1006/biol.1999.0213
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subjects Antibodies, Monoclonal - isolation & purification
Chromatography - methods
Drug Contamination
Drug Industry - methods
Polymerase Chain Reaction - methods
Recombinant Proteins - isolation & purification
Simian virus 40
Simian virus 40 - isolation & purification
title Real Time Quantitative PCR as a Method to Evaluate Simian Virus 40 Removal During Pharmaceutical Protein Purification
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