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Increased productivity of recombinant tissular plasminogen activator (t-PA) by butyrate and shift of temperature: a cell cycle phases analysis

机译:通过丁酸和温度变化提高重组体组织纤溶酶原激活物(t-PA)的生产率:细胞周期阶段分析

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摘要

Directed control of cell metabolism by a modification of the physicochemical conditions (presence of Na-butyrate and modification of the temperature) was used to modulate the productivity of human recombinant tissular plasminogen activator (t-PA) expressed under control of SV40 promoter in Chinese Hamster Ovary (CHO) cell lines. We showed that both by adding Na-butyrate or lowering temperature from 37 °C to 32 °C there is an increase in the amount of t-PA excreted, while cell growth is significantly reduced. The treatments also increased the intracellular amount of t-PA. We measured the distribution of cell cycle phases by cytometry and used a modification of the equations of Kromenaker and Srienc (1991, 1994 a, b) to analyse the intracellular t-PA production rate in the different cell cycle phases. Intracellular t-PA was shown to accumulate in G1 phase in all conditions (at 37 °C, at 32 °C and in presence of butyrate). Moreover, we have shown that the distribution of the time cells treated by butyrate are maintained in the G1cell cycle phase is significantly increased. t-PA produced in the different cell culture conditions tested was analysed by zymogram and western blotting: neither butyrate, neither the shift of temperature changed significantly the overall quality of the protein. The N-glycan patterns of recombinant human t-PA was also analysed with carbohydrate-specific lectins. Butyrate caused a transitory increase in N-linked complex high-mannose oligosaccharides without any effect on the sialic acid content of t-PA.
机译:通过理化条件的改变(丁酸钠的存在和温度的改变)来直接控制细胞代谢,以调节在中国仓鼠的SV40启动子控制下表达的人重组组织纤溶酶原激活物(t-PA)的生产力。卵巢(CHO)细胞系。我们表明,通过添加丁酸钠或将温度从37°C降至32°C,都可以增加t-PA的排泄量,而细胞的生长则明显减少。这些治疗还增加了t-PA的细胞内量。我们通过流式细胞仪测量了细胞周期阶段的分布,并对Kromenaker和Srienc(1991,1994 a,b)方程进行了修改,以分析不同细胞周期阶段中细胞内t-PA的产生率。在所有条件下(37°C,32°C和丁酸存在下),细胞内t-PA均会在G1期积累。此外,我们已经表明,丁酸处理的细胞在G1细胞周期阶段维持的时间分布显着增加。通过酶谱图和蛋白质印迹分析了在测试的不同细胞培养条件下产生的t-PA:没有丁酸盐,没有温度变化显着改变了蛋白质的整体质量。还用碳水化合物特异性凝集素分析了重组人t-PA的N-聚糖模式。丁酸酯引起N连接的复杂高甘露糖寡糖的短暂增加,而对t-PA的唾液酸含量没有任何影响。

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