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Inducible expression of calreticulin-N58 in Pichia pastoris by high density cell culture

机译:高密度细胞培养诱导钙网蛋白N58在毕赤酵母中的表达

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Calreticulin-N58 (CRT-N58), an active fragment of calreticulin with anti-angiogenesis activity, was expressed in P. pastoris by high density cell culture. Calreticulin-N58 DNA was synthesized by PCR and cloned to plasmid pPIC9 K resulting in the plasmid pPIC9 K-crt-N58 which was then transformed into P. pastoris GS115. The fermentation was carried out in a 50 l bioreactor with 20 l modified growth medium recommended by Invitrogen at 30°C. The cells were first grown in glycerol-PTM4 trace salts for 24 h. When the cell density was grown to A600 = 135, methanol-PTM4 trace salts was added to induce the expression of calreticulin-N58. During the fermentation, dissolved oxygen level was maintained at 20–30%, pH was controlled at 5 by adding 7 M NH4OH. After 52 h of induction, the yield of secreted calreticulin-N58 was 70 mg/l and biomass growth was 293 as measured by absorption of 600 nm. The secreted calreticulin-N58 was purified to a purity of 100% by the use of SP-Sepharose FF ion-exchange chromatography (Pharmacia Biotech. NJ, USA) and desalted with ultrafiltration device (Millipore, Bedford, MA, USA). The recombinant calreticulin-N58 induced endothelial cell apoptosis and inhibited the angiogenesis on the CAM.
机译:钙网蛋白-N58(CRT-N58)是具有抗血管生成活性的钙网蛋白的活性片段,通过高密度细胞培养在巴斯德毕赤酵母中表达。通过PCR合成钙网蛋白-N58 DNA,并将其克隆至质粒pPIC9 K,得到质粒pPIC9 K-crt-N58,然后将其转化至巴斯德毕赤酵母GS115中。发酵是在50升生物反应器中,用30℃Invitrogen推荐的20升改性生长培养基进行的。首先使细胞在甘油-PTM4微量盐中生长24小时。当细胞密度增长到A 600 = 135时,加入甲醇-PTM4微量盐以诱导钙网蛋白-N58的表达。在发酵过程中,通过添加7 M NH 4 OH将溶解氧水平保持在20%至30%,pH值控制在5。诱导52小时后,通过600nm吸收测定,分泌的钙网蛋白-N58的产量为70mg / l,生物量生长为293。通过使用SP-Sepharose FF离子交换色谱法(Pharmacia Biotech.NJ,美国)将分泌的钙网蛋白-N58纯化至100%的纯度,并用超滤装置(Millipore,Bedford,MA,美国)脱盐。重组钙网蛋白-N58诱导内皮细胞凋亡并抑制CAM上的血管生成。

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