A 2D LC-MS/MS Strategy for Reliable Detection of 10-ppm Level Residual Host Cell Proteins in Therapeutic Antibodies

Methodologies employing LC-MS/MS have been increasingly used for characterization and identification of residual host cell proteins (HCPs) in biopharmaceutical products to ensure their consistent product quality and safety for patients. To improve the sensitivity and reliability for HCP detection, w...

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Veröffentlicht in:	Analytical chemistry (Washington) 2018-11, Vol.90 (22), p.13365-13372
Hauptverfasser:	Yang, Feng, Walker, Donald E, Schoenfelder, Jeannine, Carver, Joseph, Zhang, Alice, Li, Delia, Harris, Reed, Stults, John T, Yu, X. Christopher, Michels, David A
Format:	Artikel
Sprache:	eng
Schlagworte:	Analytical chemistry Animals Antibodies Antibodies, Monoclonal - analysis Cattle Chemistry Chromatography, Reverse-Phase - methods Computer simulation Cricetulus Drug Contamination Escherichia coli - chemistry Fractions Humans pH effects Pharmaceuticals Product quality Product safety Proteins Reliability Sensitivity Sensitivity analysis Sensitivity and Specificity Studies Tandem Mass Spectrometry - methods
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container_title	Analytical chemistry (Washington)
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creator	Yang, Feng Walker, Donald E Schoenfelder, Jeannine Carver, Joseph Zhang, Alice Li, Delia Harris, Reed Stults, John T Yu, X. Christopher Michels, David A
description	Methodologies employing LC-MS/MS have been increasingly used for characterization and identification of residual host cell proteins (HCPs) in biopharmaceutical products to ensure their consistent product quality and safety for patients. To improve the sensitivity and reliability for HCP detection, we developed a high pH-low pH two-dimensional reversed phase LC-MS/MS approach in conjunction with offline fraction concatenation. Proof-of -concept was established using a model in which seven proteins spanning a size range of 29–78 kDa are spiked into a purified antibody product to simulate the presence of low-level HCPs. By incorporating a tandem column configuration and a shallow gradient through the second-dimension, all seven proteins were consistently identified at 10 ppm with 100% success rate following LC-MS/MS analysis of six concatenated fractions across multiple analysts, column lots and injection loads. Using the more complex Universal Proteomic Standard 1 (UPS-1) as an HCP model, positive identification was consistently achieved for 19 of the 22 proteins in 8–12 ppm range (10 ppm ±20%). For the first time, we demonstrate an effective LC-MS/MS strategy that not only has high sensitivity but also high reliability for HCP detection. The method performance has high impact on pharmaceutical company practices in using advanced LC-MS/MS technology to ensure product quality and patient safety.
doi_str_mv	10.1021/acs.analchem.8b03044
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By incorporating a tandem column configuration and a shallow gradient through the second-dimension, all seven proteins were consistently identified at 10 ppm with 100% success rate following LC-MS/MS analysis of six concatenated fractions across multiple analysts, column lots and injection loads. Using the more complex Universal Proteomic Standard 1 (UPS-1) as an HCP model, positive identification was consistently achieved for 19 of the 22 proteins in 8–12 ppm range (10 ppm ±20%). For the first time, we demonstrate an effective LC-MS/MS strategy that not only has high sensitivity but also high reliability for HCP detection. 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Christopher</creatorcontrib><creatorcontrib>Michels, David A</creatorcontrib><title>A 2D LC-MS/MS Strategy for Reliable Detection of 10-ppm Level Residual Host Cell Proteins in Therapeutic Antibodies</title><title>Analytical chemistry (Washington)</title><addtitle>Anal. Chem</addtitle><description>Methodologies employing LC-MS/MS have been increasingly used for characterization and identification of residual host cell proteins (HCPs) in biopharmaceutical products to ensure their consistent product quality and safety for patients. To improve the sensitivity and reliability for HCP detection, we developed a high pH-low pH two-dimensional reversed phase LC-MS/MS approach in conjunction with offline fraction concatenation. Proof-of -concept was established using a model in which seven proteins spanning a size range of 29–78 kDa are spiked into a purified antibody product to simulate the presence of low-level HCPs. By incorporating a tandem column configuration and a shallow gradient through the second-dimension, all seven proteins were consistently identified at 10 ppm with 100% success rate following LC-MS/MS analysis of six concatenated fractions across multiple analysts, column lots and injection loads. Using the more complex Universal Proteomic Standard 1 (UPS-1) as an HCP model, positive identification was consistently achieved for 19 of the 22 proteins in 8–12 ppm range (10 ppm ±20%). For the first time, we demonstrate an effective LC-MS/MS strategy that not only has high sensitivity but also high reliability for HCP detection. 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Christopher</au><au>Michels, David A</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>A 2D LC-MS/MS Strategy for Reliable Detection of 10-ppm Level Residual Host Cell Proteins in Therapeutic Antibodies</atitle><jtitle>Analytical chemistry (Washington)</jtitle><addtitle>Anal. Chem</addtitle><date>2018-11-20</date><risdate>2018</risdate><volume>90</volume><issue>22</issue><spage>13365</spage><epage>13372</epage><pages>13365-13372</pages><issn>0003-2700</issn><eissn>1520-6882</eissn><abstract>Methodologies employing LC-MS/MS have been increasingly used for characterization and identification of residual host cell proteins (HCPs) in biopharmaceutical products to ensure their consistent product quality and safety for patients. To improve the sensitivity and reliability for HCP detection, we developed a high pH-low pH two-dimensional reversed phase LC-MS/MS approach in conjunction with offline fraction concatenation. 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subjects	Analytical chemistry Animals Antibodies Antibodies, Monoclonal - analysis Cattle Chemistry Chromatography, Reverse-Phase - methods Computer simulation Cricetulus Drug Contamination Escherichia coli - chemistry Fractions Humans pH effects Pharmaceuticals Product quality Product safety Proteins Reliability Sensitivity Sensitivity analysis Sensitivity and Specificity Studies Tandem Mass Spectrometry - methods
title	A 2D LC-MS/MS Strategy for Reliable Detection of 10-ppm Level Residual Host Cell Proteins in Therapeutic Antibodies
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