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Evaluation of monitoring approaches and effects of culture conditions on recombinant protein production in baculovirus-infected insect cells

机译:评价杆状病毒感染昆虫细胞中重组蛋白生产的监测方法和培养条件的影响

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The baculovirus infection process ofSpodoptera frugiperda (Sf9) insect cells in oxygen-controlled bioreactors in serum-free medium was investigated using a recombinantAutographa californica (AcNPV) virus expressing β-galactosidase enzyme as a model system. A variety of monitoring techniques including trypan blue exclusion, fluorescent dye staining, oxygen uptake rate (OUR) measurements, and glucose consumption were applied to infected cells to determine the best way of evaluating cell integrity and assessing the course of baculovirus infection. The metabolism of newly-infected cells increased 90% during the first 24 hours, but as infection proceeded, and cells gradually succumbed to the baculovirus infection, the cytopathic effect of the baculovirus on the cells became evident. Oxygen and glucose uptake rate measurements appeared to more accurately assess the condition of infected cells than conventional trypan blue staining, which tended to overestimate cell viability in the mid stages of infection. The optimal harvest time varied, depending on which technique — SDS-PAGE, chromogenic (ONPG) or fluorometric (C12FDG) — was used to monitor β-galactosidase production. Specific β-galactosidase production was found to be insensitive to a wide range of culture dissolved oxygen tensions, whereas resuspending cells in fresh medium prior to infection increased volumetric productivity approximately two-fold (800,000 units β-galactosidase/ml) compared to cultures infected in batch mode and allowed successful infections to occur at higher cell densities.
机译:使用表达β-半乳糖苷酶的重组加州自噬菌(AcNPV)病毒作为模型系统,研究了无血清培养基中氧气控制的生物反应器中的节食夜蛾(Sf9)昆虫细胞的杆状病毒感染过程。多种监测技术,包括锥虫蓝排斥,荧光染料染色,氧吸收率(OUR)测量和葡萄糖消耗,已应用于感染的细胞,以确定评估细胞完整性和评估杆状病毒感染过程的最佳方法。在最初的24小时内,新感染的细胞的代谢增加了90%,但是随着感染的进行,并且细胞逐渐死于杆状病毒感染,杆状病毒对细胞的细胞病变作用变得明显。与传统的锥虫蓝染色相比,氧气和葡萄糖的摄取速率测量似乎更准确地评估了被感染细胞的状况,后者通常会高估感染中期的细胞活力。最佳收获时间有所不同,具体取决于使用哪种技术(SDS-PAGE,发色(ONPG)或荧光法(C12FDG))来监测β-半乳糖苷酶的产生。发现特定的β-半乳糖苷酶产生对广泛的培养物溶解氧张力不敏感,而与在批处理模式,并允许在更高的细胞密度下成功感染。

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