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Identifying Stabilizers of Plasmid DNA for Pharmaceutical Use
Authors:Yuhong Zeng  Joshua D. Ramsey  Robert King  Michael Leviten  Ruth Mcguire  David B. Volkin  Sangeeta B. Joshi  C. Russell Middaugh
Affiliation:1. Department of Pharmaceutical Chemistry, University of Kansas, Lawrence, Kansas 66047;2. Bayhill Therapeutics, Inc., 1804 Embarcadero Road, Suite 201, Palo Alto, California 94303;3. Joshua D. Ramsey''s present address is School of Chemical Engineering, Oklahoma State University, Stillwater, Oklahoma 74078
Abstract:To better address the need for developing stable formulations of plasmid DNA-based biopharmaceuticals, 37 compounds from a generally regarded as safe library were examined for their potential use as stabilizers. A plasmid DNA-based therapeutic vaccine, BHT-DNA?, was used as a model system. Initial studies were performed to compare the biophysical properties of BHT-DNA? plasmid from bulk drug substance and finished drug product. An agarose gel electrophoresis-based assay was then employed in excipient compatibility studies for the drug product by monitoring supercoiled plasmid DNA content in various formulations. After incubation at 40°C for 30 days, eight out of the 37 excipients tested were able to better retain the supercoil content compared to the control. Sodium citrate appeared to be the most effective stabilizer and its protective capability plateaued at an ionic strength of about 0.4. Several other excipients including malic acid, ethanol, and Pluronic F-68 were also identified as promising stabilizers for BHT-DNA? plasmid DNA. Additionally, compounds, including ferrous chloride, ascorbic acid, human serum albumin, and PEG 1000, which significantly destabilized the supercoiled plasmid DNA were identified. These data may also be applicable to other plasmid DNA-based pharmaceuticals for storage stability improvement, due to chemical and structural similarities of these macromolecules.
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