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High throughput purification of recombinant human growth hormone using radial flow chromatography

机译:径向流色谱法高通量纯化重组人生长激素

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Recombinant human growth hormone (r-hGH) was expressed in Escherichia coli as inclusion bodies. Using fed-batch fermentation process, around 670 mg/L of r-hGH was produced at a cell OD600 of 35. Cell lysis followed by detergent washing resulted in semi-purified inclusion bodies with more than 80% purity. Purified inclusion bodies were homogenous in preparation having an average size of 0.6 μm. Inclusion bodies were solubilized at pH 12 in presence of 2 M urea and refolded by pulsatile dilution. Refolded protein was purified with DEAE-anion exchange chromatography using both radial and axial flow column (50 ml bed volume each). Higher buffer flow rate (30 ml/min) in radial flow column helped in reducing the batch processing time for purification of refolded r-hGH. Radial column based purification resulted in high throughput recovery of diluted refolded r-hGH in comparison to axial column. More than 40% of inclusion body protein could be refolded into bioactive form using the above method in a single batch. Purified r-hGH was analyzed by mass spectroscopy and found to be bioactive by Nb2 cell line proliferation assay. Inclusion body enrichment, mild solubilization, pulsatile refolding and radial flow chromatography worked co-operatively to improve the overall recovery of bioactive protein from inclusion bodies.
机译:重组人生长激素(r-hGH)在大肠杆菌中表达为包涵体。使用分批补料发酵过程,OD600为35的细胞产生约670 mg / L的r-hGH。细胞裂解,然后用去污剂洗涤,得到半纯化的包涵体,纯度超过80%。纯化的包涵体在制备中是均质的,平均大小为0.6μm。包涵体在2 M尿素的存在下在pH 12下溶解,并通过脉冲稀释法重新折叠。使用DEAE-阴离子交换色谱法同时使用径向和轴向流色谱柱(每个床体积为50 ml)纯化重折叠的蛋白质。径向流色谱柱中较高的缓冲液流速(30 ml / min)有助于减少用于重新折叠r-hGH纯化的批处理时间。与轴向色谱柱相比,基于径向色谱柱的纯化导致稀释的重折叠r-hGH的高通量回收率。使用上述方法,可以单批将超过40%的包涵体蛋白重折叠成生物活性形式。通过质谱分析纯化的r-hGH,并且通过Nb2细胞系增殖测定法发现其具有生物活性。包涵体富集,温和溶解,脉冲复性和径向流色谱法协同工作,以提高从包涵体中回收生物活性蛋白的整体能力。

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