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悬浮聚集体作为一种固定化模式用于在搅拌罐生物反应器中对HEK 293细胞进行高密度灌注培养。

Suspended aggregates as an immobilization mode for high-density perfusion culture of HEK 293 cells in a stirred tank bioreactor.

作者信息

Liu X M, Liu H, Wu B C, Li S C, Ye L L, Wang Q W, Huang P T, Chen Z L

机构信息

Department of Cell Engineering, Beijing Institute of Biotechnology, 20 Dongdajie Street, Fengtai, Beijing 100071, People's Republic of China.

出版信息

Appl Microbiol Biotechnol. 2006 Oct;72(6):1144-51. doi: 10.1007/s00253-006-0409-3. Epub 2006 Mar 28.

Abstract

Cells of the human embryonic kidney cell line (HEK 293) grown in repeated suspension and perfusion systems were characterized and described. Cell aggregates that formed immediately after the HEK 293 cells were inoculated in stirred vessels in serum-containing Dulbecco's modified Eagle's medium (D-MEM)/F-12 medium. The mean diameter of the cell aggregates reflecting the aggregate size increased with culture time, shifting from 63 to 239 mum after 1 and 8 days of culture in spinner flasks, respectively. No significant differences in cell performance were observed between HEK 293 cell populations grown as suspended aggregates and those grown as anchored monolayers. Replacing the D-MEM/F-12 with CD 293 medium caused the compact spherical cell aggregates to dissociate into single cells and small irregular aggregates without any apparent effect on cell performance. Moreover, the spherical cell aggregates could reform from individual cells and small aggregates when exposed to the serum-containing D-MEM/F-12 dominant medium. Perfusion culture of HEK 293 cells grown as suspended aggregates in a 7.5-l stirred tank bioreactor for 17 days resulted in a maximum viable cell density of 1.2 x 10(7) cells ml(-1). These results demonstrate the feasibility and proof-of-concept for using aggregates as an immobilization system in large-scale stirred bioreactors because a small-scale culture can be used as easily as the inoculum for larger bioreactors.

摘要

对在重复悬浮和灌注系统中培养的人胚肾细胞系(HEK 293)细胞进行了表征和描述。将HEK 293细胞接种于含血清的杜尔贝科改良伊格尔培养基(D-MEM)/F-12培养基的搅拌容器中后,立即形成细胞聚集体。反映聚集体大小的细胞聚集体平均直径随培养时间增加,在转瓶中培养1天和8天后分别从63μm增加到239μm。在作为悬浮聚集体生长的HEK 293细胞群体和作为贴壁单层生长的细胞群体之间,未观察到细胞性能的显著差异。用CD 293培养基替代D-MEM/F-12会导致紧密的球形细胞聚集体解离为单个细胞和小的不规则聚集体,对细胞性能没有任何明显影响。此外,当暴露于含血清的D-MEM/F-12为主的培养基时,球形细胞聚集体可从单个细胞和小聚集体重新形成。在7.5升搅拌罐生物反应器中对作为悬浮聚集体生长的HEK 293细胞进行17天的灌注培养,导致最大活细胞密度达到1.2×10⁷个细胞/毫升。这些结果证明了在大规模搅拌生物反应器中使用聚集体作为固定化系统的可行性和概念验证,因为小规模培养可以像接种物一样容易地用于更大的生物反应器。

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