Brillet Karl, da Conceição Mateus Menegues, Pattus Franc, Pereira Carlos Augusto
Biotechnologie, Integrité du Genome, Transcription et Signalisation, UMR 7100, Ecole Supérieure de Biotechnologie de Strasbourg, Bld Sébastien Brant, BP 10413, 67400, Illkirch, France.
Bioprocess Biosyst Eng. 2006 Apr;28(5):291-3. doi: 10.1007/s00449-005-0033-0. Epub 2005 Dec 7.
The paper describes a recombinant Schneider 2 (rS2) cell culture and protein expression in a bioreactor. S2 cells were transfected with a plasmid containing a fusion protein (human mu opioid receptor, hMOR, and green fluorescent protein, EGFP) under the control of inducible metallothionein promoter. A bioprocess in a bioreactor with 5% dissolved oxygen, 27 degrees C and 120 rpm enabled the cell culture to attain 5.3x10(7 )viable cells/mL at 96 h. The induction decreased the cell multiplication (2.5x10(7) viable cells/mL at 72 h). Glutamine and glucose and low levels of lactate were consumed. A fast recombinant protein synthesis took place and, at 6 h of induction, 2x10(4) receptors/cell could be detected by a functional binding assay. Fluorescence measurements showed a progressive increase of recombinant protein expression with a maximal value of 1.26x10(5) fluo counts/s at 24 h of induction. The data shown in this paper indicate a practical and scaleable cell culture bioprocess procedure for the preparation of recombinant proteins expressed in S2 cells.
本文描述了重组施耐德2(rS2)细胞培养及在生物反应器中的蛋白质表达情况。用含有融合蛋白(人μ阿片受体,hMOR,和绿色荧光蛋白,EGFP)的质粒转染S2细胞,该质粒受诱导型金属硫蛋白启动子控制。在溶解氧为5%、27℃和120转/分钟的生物反应器中进行的生物过程,使细胞培养物在96小时时达到5.3×10⁷个活细胞/毫升。诱导作用降低了细胞增殖(72小时时为2.5×10⁷个活细胞/毫升)。谷氨酰胺、葡萄糖被消耗,乳酸水平较低。发生了快速的重组蛋白合成,在诱导6小时时,通过功能结合测定可检测到每个细胞有2×10⁴个受体。荧光测量显示重组蛋白表达逐渐增加,在诱导24小时时最大值为1.26×10⁵荧光计数/秒。本文所示数据表明了一种用于制备在S2细胞中表达的重组蛋白的实用且可扩展的细胞培养生物过程程序。
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