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Monoclonal antibody refolding and assembly: Protein disulfide isomerase reaction kinetics |
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| Authors: | Sun?Ho?Park author-information" > author-information__contact u-icon-before" > mailto:parla@mucc.keimyung.ac.kr" title=" parla@mucc.keimyung.ac.kr" itemprop=" email" data-track=" click" data-track-action=" Email author" data-track-label=" " >Email author,D.?Y.?Ryu |
| Affiliation: | (1) Department of Chemical Engineering, Keimyung University, Shinxlang-dong 1000, Jalsen-Ku, 704-701 Taegu, Korea;(2) Department of Chemical Engineering, University of California, 96616 Davis, CA, U.S.A. |
| Abstract: | The protein disulfide isomerase (PDI) reaction kinetics has been studied to evaluate its effect on the monoclonal antibody (MAb) refulding and assembly which accompanies disulfide bond formation. The MAbin vitro assembly experiments showed that the assembly rate of heavy and light chains can be greatly enhanced in the presence of PDI as compared to the rate of assembly obtained by the air-oxidation. The reassembly patterns of MAb intermediates were identical for both with and without PDI, suggesting that the PDI does not determine the MAb assembly pathway, but rather facilitates the rate of MAb assembly by promoting PDI catalyzed disulfide bond formation. The effect of growth rate on PDI activities for MAb production has also been examined by using continuous culture system. The specific MAb productivity of hyboridoma cells decreased as the growth rate increased. However, PDI activities were nearly constant for a wide range of growth rates except very high growth rate, indicating that no direct correlation between PDI activity and specifle MAb productivity exists. |
| Keywords: | monoclonal antibody protein folding and assembly protein disulfide isomerase continuous culture hybridoma |
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