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高密度细胞培养系统中的工程挑战。

Engineering challenges in high density cell culture systems.

机构信息

Bayer Corporation, Biotechnology, 4th and Parker Streets, 94701, Berkeley, CA, USA.

出版信息

Cytotechnology. 1996 Jan;22(1-3):3-16. doi: 10.1007/BF00353919.

DOI:10.1007/BF00353919
PMID:22358910
Abstract

High density cell culture systems offer the advantage of production of bio-pharmaceuticals in compact bioreactors with high volumetric production rates; however, these systems are difficult to design and operate. First of all, the cells have to be retained in the bioreactor by physical means during perfusion. The design of the cell retention is the key to performance of high density cell culture systems. Oxygenation and media design are also important for maximizing the cell number. In high density perfusion reactors, variable cell density, and hence the metabolic demand, require constant adjustment of perfusion rates. The use of cell specific perfusion rate (CSPR) control provides a constant environment to the cells resulting in consistent production. On-line measurement of cell density and metabolic activities can be used for the estimation of cell densities and the control of CSPR. Issues related to mass transfer and mixing become more important at high cell densities. Due to the difference in mass transfer coefficients for oxygen and CO(2), a significant accumulation of dissolved CO(2) is experienced with silicone tubing aeration. Also, mixing is observed to decrease at high densities. Base addition, if not properly done, could result in localized cell lysis and poor culture performance. Non-uniform mixing in reactors promotes the heterogeneity of the culture. Cell aggregation results in segregation of the cells within different mixing zones. This paper discusses these issues and makes recommendations for further development of high density cell culture bioreactors.

摘要

高密度细胞培养系统具有在紧凑的生物反应器中以高体积产率生产生物制药的优势; 然而,这些系统很难设计和操作。首先,在灌注过程中必须通过物理手段将细胞保留在生物反应器中。细胞保留的设计是高密度细胞培养系统性能的关键。氧合和培养基设计对于最大限度地提高细胞数量也很重要。在高密度灌注反应器中,可变的细胞密度,因此代谢需求,需要不断调整灌注率。使用细胞特异性灌注率 (CSPR) 控制可为细胞提供恒定的环境,从而实现一致的生产。细胞密度和代谢活性的在线测量可用于估计细胞密度和控制 CSPR。在高细胞密度下,传质和混合问题变得更加重要。由于氧气和 CO(2) 的传质系数不同,硅酮管通气会导致溶解的 CO(2 大量积累。此外,在高浓度下观察到混合减少。如果不正确添加碱,可能会导致局部细胞裂解和较差的培养性能。反应器中不均匀的混合会促进培养物的异质性。细胞聚集导致细胞在不同的混合区中分离。本文讨论了这些问题,并为进一步开发高密度细胞培养生物反应器提出了建议。

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