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Large-scale production and purification of functional recombinant bovine rhodopsin with the use of the baculovirus expression system.

机译:使用杆状病毒表达系统大规模生产和纯化功能重组牛视紫红质。

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摘要

Here we describe a generic procedure for the expression and purification of milligram quantities of functional recombinant eukaryotic integral membrane proteins, exemplified by hexahistidine-tagged bovine rhodopsin. These quantities were obtained with the recombinant baculovirus/Sf9 insect cell-based expression system in large-scale bioreactor cultures with the use of a serum-free and protein-free growth medium. After optimization procedures, expression levels up to 4 mg/l were established. The recombinant rhodopsin could be purified with high overall yield by using immobilized-metal-affinity chromatography on Ni(2+)-agarose. After reconstitution into a native lipid environment, the purified protein was functionally indistinguishable from native rhodopsin with regard to the following parameters: spectral absorbance band, structural changes after photoactivation, and G-protein activation. The procedures developed can be adapted to other membrane proteins. The ability to produce and purify tens of milligrams of functional recombinant eukaryotic membrane protein meets the ever-increasing demand of material necessary to perform detailed biochemical and structural biophysical studies that are essential in unravelling their working mechanism at a molecular level.
机译:在这里,我们描述了表达和纯化毫克级功能重组真核生物整合膜蛋白的通用程序,以六组氨酸标记的牛视紫红质为例。使用无血清和无蛋白质的生长培养基,在大规模生物反应器培养物中,使用基于重组杆状病毒/ Sf9昆虫细胞的表达系统获得这些量。优化程序后,建立了高达4 mg / l的表达水平。重组视紫红质可以通过在Ni(2 +)-琼脂糖上使用固定的金属亲和色谱法以高总收率纯化。重构为天然脂质环境后,就以下参数而言,纯化的蛋白质在功能上与天然视紫红质没有区别:光谱吸收带,光活化后的结构变化和G蛋白活化。开发的程序可以适应其他膜蛋白。产生和纯化数十毫克功能性重组真核细胞膜蛋白的能力满足了对进行详细的生化和结构生物物理研究所必需的材料的不断增长的需求,而这对于在分子水平上揭示其工作机理至关重要。

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