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Protective effect of viral homologues of bcl-2 hybridoma cells under apoptosis-inducing conditions

机译:凋亡诱导条件下bcl-2杂交瘤细胞病毒同源物的保护作用

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摘要

Targets for metabolic engineering have been identified in a hybridoma cell line to make it more robust in culture toward potential limitations inducing apoptosis. The cells were genetically modified with plasmids harboring endogenous bcl-2 gene and also with viral Bcl-2 homologues, particularly ksbcl-2 and bhrf-1 genes. When cells were exposed to apoptosis-inducing conditions (i.e., glutamine-free medium), the control cells exhibited a decrease in viable cell number within the first 12 h, whereas, for the bcl-2 and ksbcl-2 transfected cell cultures, the viable cell number did not exhibit any clear decrease until after 66 h. Furthermore, hybridoma. cells expressing the viral homologue bhrf-1 were even more resistant to cell death, shoving a decrease in viability of only 50% at 72 h of culture in glutamine-deprived medium, substantially lower than the 96% viability decrease observed for the control culture. In addition, and most relevant for further bioprocess applications, the cells genetically modified could be brought back to growth conditions even after being exposed to glutamine-deprived conditions during a significant time window, up to 72 h.
机译:已经在杂交瘤细胞系中鉴定了代谢工程的靶标,以使其在培养中对诱导凋亡的潜在限制更为稳健。用携带内源性bcl-2基因的质粒以及病毒Bcl-2同源物,特别是ksbcl-2和bhrf-1基因,对细胞进行遗传修饰。当细胞暴露于凋亡诱导条件下(即无谷氨酰胺的培养基)时,对照细胞在前12 h内的活细胞数减少,而对于bcl-2和ksbcl-2转染的细胞培养,存活细胞数直到66小时后才显示出任何明显的减少。此外,杂交瘤。表达病毒同源物bhrf-1的细胞对细胞死亡的抵抗力更高,在缺乏谷氨酰胺的培养基中培养72小时时,活力仅下降了50%,远低于对照培养物中96%的活力下降。此外,与进一步的生物工艺应用最相关的是,即使在长达72小时的显着时间窗内暴露于谷氨酰胺剥夺的条件下,经过基因修饰的细胞也可以恢复到生长状态。

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