| Literature DB >> 30262247 |
Martin Burkhardt1, Karine Reiter1, Vu Nguyen1, Motoshi Suzuki2, Raul Herrera1, Patrick E Duffy1, Richard Shimp1, Nicholas J MacDonald1, L Renee Olano2, David L Narum3.
Abstract
Efforts to develop a vaccine for the elimination of malaria include the use of carrier proteins to assemble monomeric antigens into nanoparticles to maximize immunogenicity. Recombinant ExoProtein A (EPA) is a detoxified form of Pseudomonas aeruginosa Exotoxin A which has been used as a carrier in the conjugate vaccine field. A pilot-scale process developed for purification of EPA yielded product that consistently approached a preset upper limit for host cell protein (HCP) content per human dose. To minimize the risk of bulk material exceeding the specification, the purification process was redeveloped using mixed-mode chromatography resins. Purified EPA derived from the primary and redeveloped processes were comparable following full biochemical and biophysical characterization. However, using a process specific immunoassay, the HCP content was shown to decrease from a range of 0.14-0.24% w/w of total protein to below the level of detection with the revised process. The improved process reproducibly yields EPA with highly similar quality characteristics as the original process but with an improved profile for the HCP content. Published by Elsevier Ltd.Entities:
Keywords: ExoProtein A; Host cell protein; Malaria; Mass spectrometry; Mixed-mode chromatography; Purification; Vaccine; Vaccine carrier
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Year: 2018 PMID: 30262247 PMCID: PMC6525083 DOI: 10.1016/j.vaccine.2018.09.037
Source DB: PubMed Journal: Vaccine ISSN: 0264-410X Impact factor: 4.169