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Chromatographic Methods for Quantitative Analysis of Native,Denatured, and Aggregated Basic Fibroblast Growth Factor in Solution Formulations
Authors:Sluzky  Victoria  Shahrokh  Zahra  Stratton  Pamela  Eberlein  Gert  Wang  Y John
Institution:(1) Pharmaceutical R&D, Scios Nova Inc., Mountain View, California;(2) COR Therapeutics, Inc., South San Francisco, California, 94080
Abstract:High-performance liquid chromatography (HPLC) methods were developed for evaluating stability of human recombinant basic fibroblast growth factor (bFGF) against denaturation and aggregation in solution formulations. Re versed-phase chromatography (RP-HPLC)-insensitive to bFGF tertiary structure-was used to measure total soluble protein; heparin affinity chromatography (HepTSK) provided quantitative analysis of native bFGF species. The folding state of bFGF was determined by fluorescence spectroscopy: Tryptophan emission, which was quenched in native protein, increased upon unfolding. Slow unfolding/refolding kinetics of bFGF in 2 M guanidine hydrochloride made possible the separation of native from denatured species by size exclusion chromatography (SEC). Although the tertiary structure affected bFGF retention times, it did not change the sample recovery by SEC. These chromatographic techniques, which quantitatively measure physical and chemical changes taking place in solution formulations, can be used in future investigations of bFGF stability.
Keywords:fibroblast growth factor  protein stability  formulation  HPLC  denaturation kinetics  fluorescence
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