Application of Tryptophan Fluorescence Bandwidth-Maximum Plot in Analysis of Monoclonal Antibody Structure.

AAPS PharmSciTech

BioAnalytical Sciences, Eli Lilly and Company, 22 ImClone Drive, Branchburg, NJ, 08876, USA.

Published: April 2017

AI Article Synopsis

  • * Tryptophan fluorescence can effectively monitor the tertiary structure of proteins, using log-normal distribution curves for analysis.
  • * This method distinguishes between monoclonal antibodies and tracks structural changes during unfolding, offering detailed insights into their properties and manufacturing consistency.

Article Abstract

Monoclonal antibodies have become the fastest growing protein therapeutics in recent years. The stability and heterogeneity pertaining to its physical and chemical structures remain a big challenge. Tryptophan fluorescence has been proven to be a versatile tool to monitor protein tertiary structure. By modeling the tryptophan fluorescence emission envelope with log-normal distribution curves, the quantitative measure can be exercised for the routine characterization of monoclonal antibody overall tertiary structure. Furthermore, the log-normal deconvolution results can be presented as a two-dimensional plot with tryptophan emission bandwidth vs. emission maximum to enhance the resolution when comparing samples or as a function of applied perturbations. We demonstrate this by studying four different monoclonal antibodies, which show the distinction on emission bandwidth-maximum plot despite their similarity in overall amino acid sequences and tertiary structures. This strategy is also used to demonstrate the tertiary structure comparability between different lots manufactured for one of the monoclonal antibodies (mAb2). In addition, in the unfolding transition studies of mAb2 as a function of guanidine hydrochloride concentration, the evolution of the tertiary structure can be clearly traced in the emission bandwidth-maximum plot.

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Source
http://dx.doi.org/10.1208/s12249-016-0568-1DOI Listing

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