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High yield soluble bacterial expression and streamlined purification of recombinant human interferon α-2a

机译:重组人干扰素α-2a的高产可溶性细菌表达及简化纯化

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Interferon α-2a (IFNA2) is a member of the Type I interferon cytokine family, known for its antiviral and anti-proliferative functions. The role of this family in the innate immune response makes it an attractive candidate for the treatment of many viral and chronic immune-compromised diseases. Recombinant IFNA2 is clinically used to modulate hairy cell leukemia as well as hepatitis c. Historically, IFNA2 has been purified from human leukocytes as well as bacterial expression systems. In most cases, bacterial expression of IFNA2 resulted in inclusion body formation, or required numerous purification steps that decreased the protein yield. Here, we describe an expression and purification scheme for IFNA2 using a pET-SUMO bacterial expression system and a single purification step. Using the SUMO protein as the fusion tag achieved high soluble protein expression. The SUMO tag was cleaved with the Ulp1 protease leaving no additional amino acids on the fusion terminus following cleavage. Mass spectrometry, circular dichroism, 2D heteronuclear NMR, and analytical ultracentrifugation confirmed the amino acid sequence identity, secondary and tertiary protein structures, and the solution behavior of the purified IFNA2. The purified protein also had antiviral and anti-proliferative activities comparable to the WHO International Standard, NIBSC 95/650, and the IFNA2 standard available from PBL Assay Science. Combining the expression and purification protocols developed here to produce IFNA2 on a laboratory scale with the commercial fermenter technology commonly used in pharmaceutical industry may further enhance IFNA2 yields, which will promote the development of interferon-based protein drugs to treat various disorders.
机译:干扰素α-2a(IFNA2)是I型干扰素细胞因子家族的成员,以其抗病毒和抗增殖功能而闻名。该家族在先天免疫应答中的作用使其成为治疗许多病毒和慢性免疫功能低下疾病的有吸引力的候选者。重组IFNA2在临床上用于调节毛细胞白血病和丙型肝炎。历史上,IFNA2已经从人白细胞以及细菌表达系统中纯化出来。在大多数情况下,细菌表达IFNA2会导致包涵体形成,或者需要大量纯化步骤才能降低蛋白质产量。在这里,我们描述了使用pET-SUMO细菌表达系统和单个纯化步骤的IFNA2表达和纯化方案。使用SUMO蛋白作为融合标签可实现高可溶性蛋白表达。用Ulp1蛋白酶切割SUMO标签,切割后在融合末端上不留下额外的氨基酸。质谱,圆二色性,二维异核NMR和分析超速离心证实了氨基酸序列同一性,二级和三级蛋白质结构以及纯化的IFNA2的溶液行为。纯化的蛋白质还具有与WHO国际标准NIBSC 95/650和PBL Assay Science可得的IFNA2标准相当的抗病毒和抗增殖活性。将此处开发的可在实验室规模生产IFNA2的表达和纯化方案与制药行业常用的商业发酵罐技术相结合,可进一步提高IFNA2的产量,这将促进开发基于干扰素的蛋白药物以治疗各种疾病。

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