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单克隆抗体F11分离的VL结构域的表达、重折叠及铁蛋白结合活性

Expression, refolding, and ferritin-binding activity of the isolated VL-domain of monoclonal antibody F11.

作者信息

Dubnovitsky A P, Kravchuk Z I, Chumanevich A A, Cozzi A, Arosio P, Martsev S P

机构信息

Institute of Bioorganic Chemistry, National Academy of Sciences of Belarus, Minsk, 220141, Belarus.

出版信息

Biochemistry (Mosc). 2000 Sep;65(9):1011-8.

PMID:11042491
Abstract

Expression of the VL-domain of mouse monoclonal antibody F11 to human spleen ferritin in Escherichia coli cells is associated with the formation of insoluble protein aggregates (inclusion bodies). The aggregates were solubilized in the presence of guanidine hydrochloride and the recombinant VL-domain was purified by immobilized metal affinity chromatography (IMAC). Subsequent renaturation results in approximately 99% pure preparation with high yield. The VL-domain forms dimers at concentrations from 1 to 10 mg/ml. Monomeric form is detected only at protein concentrations below 0.5 mg/ml. Functional activity of the VL-domain was verified by two variants of ELISA. The affinity of the VL-domain ((0.2-1.2). 108 M(-1)) is similar to the affinity of the full-length parental antibody F11 because when the immobilized VL-domain was used, the binding constant of ferritin to the VL-domain was only 4-6-fold lower than that in the case of F11 antibody. In another ELISA system with immobilized ferritin, affinity was decreased 30-fold. The VL-domain of antibody F11 is the first example of the recombinant variable domain of the immunoglobulin light chain that preserves the antigen-binding activity in the absence of the partner VH-domain. The data indicate that the recombinant VL-domain can be used in construction of chimeric immunotoxins and other antigen-binding proteins in immunotherapy and in studies of correlations between folding, stability, and activity of immunoglobulins.

摘要

小鼠单克隆抗体F11针对人脾铁蛋白的VL结构域在大肠杆菌细胞中的表达与不溶性蛋白质聚集体(包涵体)的形成有关。这些聚集体在盐酸胍存在下被溶解,重组VL结构域通过固定化金属亲和色谱法(IMAC)进行纯化。随后的复性产生了约99%的高纯度制剂。VL结构域在浓度为1至10mg/ml时形成二聚体。仅在蛋白质浓度低于0.5mg/ml时检测到单体形式。VL结构域的功能活性通过两种ELISA变体进行了验证。VL结构域的亲和力((0.2 - 1.2)×10⁸ M⁻¹)与全长亲本抗体F11的亲和力相似,因为当使用固定化的VL结构域时,铁蛋白与VL结构域的结合常数仅比F11抗体情况下低4至6倍。在另一种固定化铁蛋白的ELISA系统中,亲和力降低了30倍。抗体F11的VL结构域是免疫球蛋白轻链重组可变结构域在没有伴侣VH结构域的情况下仍保留抗原结合活性的首个实例。数据表明,重组VL结构域可用于构建嵌合免疫毒素和免疫治疗中的其他抗原结合蛋白,以及用于研究免疫球蛋白的折叠、稳定性和活性之间的相关性。

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