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Anchorage-dependent animal cell culture by using a porous microcarrier
Authors:N Shiragami  H Honda  H Unno
Institution:(1) Department of Bioengineering, Tokyo Institute of Technology, Nagatsuta-cho, Midori-ku, 4259 Yokohama, Japan
Abstract:CHO-K1 cells were cultured by using a porous microcarrier. The effects of microcarrier concentration and agitation rate on cell growth in porous microcarrier cultures were investigated. The specific growth rate of 0.041 h–1 in porous microcarrier cultures was independent of both microcarrier concentration and agitation rate. By estimating the total surface area occupied by cells from the maximum cell number, it was found that not all the surface area of the porous microcarrier was utilizable for cell growth.The maximum cell number decreased with increasing the microcarrier concentration and the agitation rate. From this result, it was also found that not all the cells grown on the interior surface of the porous microcarrier were protected against mechanical damage due to agitation. The protection capacity of the porous microcarrier was estimated to be 300 cells/carrier. The direct gas sparging into the culture broth in porous microcarrier cultures improved the cell density without mechanical damage to animal cells.List of Symbols d m microcarrier diameter - d i m impeller diameter - d p m mean pore diameter - n i s–1 agitation rate - Deltap Pa pressure difference - v m/s velocity of microcarrier - v p m/s average velocity flowing through cyclinder - eegr Pa · s viscosity of medium - theta angle measured from stagnant point - tau Pa average shear stress - tautheta Pa shear stress distribution
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