Improved Fluorescence Methods for High-Throughput Protein Formulation Screening

Author:

Wei Yangjie12,Larson Nicholas R.12,Angalakurthi Siva K.12,Russell Middaugh C.12

Affiliation:

1. Macromolecule and Vaccine Stabilization Center, Department of Pharmaceutical Chemistry, University of Kansas, Lawrence, KS, USA

2. Department of Pharmaceutical Chemistry, University of Kansas, Lawrence, KS, USA

Abstract

The goal of protein formulation development is to identify optimal conditions for long-term storage. Certain commercial conditions (e.g., high protein concentration or turbid adjuvanted samples) impart additional challenges to biophysical characterization. Formulation screening studies for such conditions are usually performed using a simplified format in which the target protein is studied at a low concentration in a clear solution. The failure of study conditions to model the actual formulation environment may cause a loss of ability to identify the optimal condition for target proteins in their final commercial formulations. In this study, we utilized a steady-state/lifetime fluorescence-based, high-throughput platform to develop a general workflow for direct formulation optimization under analytically challenging but commercially relevant conditions. A high-concentration monoclonal antibody (mAb) and an Alhydrogel-adjuvanted antigen were investigated. A large discrepancy in screening results was observed for both proteins under these two different conditions (simplified and commercially relevant). This study demonstrates the feasibility of using a steady-state/lifetime fluorescence plate reader for direct optimization of challenging formulation conditions and highlights the importance of performing formulation optimization under commercially relevant conditions.

Funder

NIH biotechnology training grant

American Association of Pharmaceutical Scientists Foundation

Publisher

Elsevier BV

Subject

Medical Laboratory Technology,Computer Science Applications

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