Increasing the homogeneity, stability and activity of human serum albumin and interferon-α2b fusion protein by linker engineering

连接器 人血清白蛋白 融合蛋白 化学 融合 氨基酸 水解 生物化学 血清白蛋白 生物物理学 重组DNA 生物 哲学 操作系统 基因 语言学 计算机科学
作者
Hong Liang Zhao,Xue Yao,Chong Xue,Yang Wang,Xiang Hua Xiong,Zhi Min Liu
出处
期刊:Protein Expression and Purification [Elsevier BV]
卷期号:61 (1): 73-77 被引量:167
标识
DOI:10.1016/j.pep.2008.04.013
摘要

Previous studies in our laboratory have shown that when the N-terminus of interferon-α2b (IFN-α2b) was directly fused of to the C-terminus of human serum albumin (HSA), the resultant fusion protein (HSA-IFN-α2b) was heterogeneous (migrated as doublets on non-reducing SDS–PAGE) and unstable (prone to form covalent aggregates). The heterogeneity and instability of HSA-IFN-α2b was ascribed to the structural disturbance between HSA and IFN-α2b. To alleviate such structural disturbance, linkers with different lengths (1, 2, 5, 10 amino acid residues) or different conformation (flexible linker (FL, GGGGS), rigid linker (RL, PAPAP) or helix-forming linker (HL, AEAAAKEAAAKA)) were inserted between HSA and IFN-α2b. It was demonstrated that linker with 5 amino acid residues was sufficient to separated HSA and IFN-α2b effectively, as fusion protein with this linker migrated as single band on non-reducing SDS–PAGE. The fusion proteins with FL, RL and HL linkers were purified to homogeneity with yields of 20%, while the recovery rate of HSA-IFN-α2b was only 10%. Accelerated thermal stress tests showed that in contrast to HSA-IFN-α2b, fusion proteins with FL, RL and HL linkers were free of aggregates after stored at 37 °C for 10 days. Stability tests also revealed that fusion proteins with FL, RL and HL linkers had different susceptibility to hydrolysis, with HSA-RL-IFN-α2b being the least susceptible to hydrolysis at pH 6 and 7. Activity assay revealed that the insertion of FL, RL and HL linkers increased the anti-viral activity of fusion protein by 39%, 68% and 115%, respectively.
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