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Santos, Antonio C. F.; Ahmadzadegan, Adib; Ximenes, Eduardo; Vlachos, Pavlos; Ardekani, Arezoo; Kapur, Shiven; Corvari, Vince; Ladisch, Michael R.
Biotechnology and bioengineering, December 2022, Volume: 119, Issue: 12Journal Article
There are currently more than 560 therapeutic monoclonal antibodies (mAbs) at various stages of research and clinical testing, including candidates for administration by subcutaneous (SC) injection. Preclinical studies based on in vitro measurements of high molecular weight proteins within simulated SC matrices are assisting laboratory studies of interactions of injectable biotherapeutic proteins within the SC environment in relation to bioavailability. We report a new method for directly measuring diffusion of unlabeled, high molecular weight proteins injected into an in vitro matrix that simulates the negatively charged environment of the SC. The matrix consists of 10 mg/ml HA in a repurposed cell culture chamber. The measurement consists of pipetting triplicate 20 μl protein samples into the matrix, placing the chamber in a laboratory scanner, activating tryptophan residues in the protein at 280 nm, and imaging the resulting protein fluorescence at 384 nm over a 0.5–4 h time period thus tracking protein movement. This facile approach enables mapping of protein concentration as a function of time and distance within the matrix, and determination of diffusion coefficients, D, within ±10%. Bovine IgG and BSA gave D = 2.3 ± 0.2*10−7 and 4.6 ± 0.2*10−7 cm2/s at 24°C, respectively, for initial protein concentrations of 21 mg/mL.
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