| Literature DB >> 33304198 |
David A Morris1,2, Micaela A Reeves3, Joshua M Royal1,2,3, Krystal T Hamorsky1,2,4, Nobuyuki Matoba1,2,3.
Abstract
Here we describe refined methods for the isolation and detection of a KDEL-tagged, plant-produced recombinant cholera toxin B subunit (CTB) that exhibits unique mucosal wound healing activity. The protein was transiently overexpressed in Nicotiana benthamiana, which generates some C-terminal KDEL truncated molecular species that are deficient in epithelial repair activity. With a new CHT chromatographical method described herein, these product-derived impurities were successfully separated from CTB with the intact KDEL sequence, as confirmed by mass spectrometry. In addition, an immunoassay capable of specifically detecting GM1 ganglioside-binding CTB with intact KDEL sequences was developed. Coupled together, these methods will aid in the quality control of KDEL-attached CTB produced in plant-based manufacturing systems towards a novel topical biotherapeutic for the treatment of acute and chronic mucosal inflammation.Entities:
Keywords: C-terminal truncation; ER retention; biotherapeutic; ceramic hydroxyapatite chromatography; immunoassay; plant-made pharmaceutical
Year: 2020 PMID: 33304198 PMCID: PMC7723343 DOI: 10.1016/j.procbio.2020.10.018
Source DB: PubMed Journal: Process Biochem ISSN: 1359-5113 Impact factor: 3.757