Improved analytical methods for the detection and quantification of neutralizing antibodies to biopharmaceuticals

Author:

Tovey Michael G1,Lallemand Christophe2

Affiliation:

1. Laboratory of Biotechnology & Applied Pharmacology, CNRS UMR 8113, ENS-Cachan, 61 Avenue President Wilson, 94235 Cachan, France.

2. Laboratory of Biotechnology & Applied Pharmacology, CNRS UMR 8113, ENS-Cachan, 61 Avenue President Wilson, 94235 Cachan, France

Abstract

Biopharmaceuticals are used extensively for the treatment of a number of chronic debilitating and fatal diseases such as cancer and inflammatory or autoimmune diseases. Although biopharmaceuticals are in general well tolerated, the development of anti-drug antibodies can impair their safety and efficacy. Assessment of immunogenicity is essential for a more effective and rational use of biopharmaceuticals, and is dependent upon the establishment of efficient standardized assays that allow direct comparison of immunogenicity data with clinical outcome. Although regulatory authorities recommend the use of cell-based assays that reflect the mechanism of action of the drug for the detection of neutralizing anti-drug antibodies, conventional cell-based assays are difficult to standardize and often give variable results. A number of strategies have been adopted to improve the performance of cell-based assays, including quantification of drug-induced proteins using either real-time RT-PCR or branched DNA to detect mRNA, or ELISAs to detect protein, bridging assays using immobilized cells and the use of reporter gene assays. The relative merits and limitations of each of these methods is reviewed herein.

Publisher

Future Science Ltd

Subject

Medical Laboratory Technology,Clinical Biochemistry,General Pharmacology, Toxicology and Pharmaceutics,General Medicine,Analytical Chemistry

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