Zhang Jianbing, Liu Xin, Bell Andrea, To Rebecca, Baral Toya Nath, Azizi Ali, Li Jianjun, Cass Brian, Durocher Yves
Institute for Biological Sciences, National Research Council of Canada, 100 Sussex Drive, Ottawa, ON K1A0R6, Canada.
Protein Expr Purif. 2009 May;65(1):77-82. doi: 10.1016/j.pep.2008.10.011. Epub 2008 Oct 26.
Monoclonal antibodies have been successfully engineered as approved therapeutics. However, their large size is considered a major factor preventing them from having a more efficient tissue penetration. As the first step to establish a possibly more efficient antibody platform, we present here transient expression, purification and characterization of six chimeric heavy chain antibodies (cHCAbs), or fusion of camelid single domain antibodies (sdAbs) to human fragment crystallizable (Fc). All six HCAbs have a MW of approximately 80 kDa, expressed well in a HEK293 expression system and have G0, G1 and G2 types of glycosylation. The transient expression also provided a very fast way to generate high milligram to low gram amount of proteins for in vitro assays and preliminary animal studies.
单克隆抗体已成功被设计为获批的治疗药物。然而,其较大的尺寸被认为是阻碍它们更有效地穿透组织的一个主要因素。作为建立一个可能更高效抗体平台的第一步,我们在此展示了六种嵌合重链抗体(cHCAbs)的瞬时表达、纯化及表征,或者是骆驼科动物单域抗体(sdAbs)与人可结晶片段(Fc)的融合。所有六种重链抗体的分子量约为80 kDa,在HEK293表达系统中表达良好,并且具有G0、G1和G2类型的糖基化。瞬时表达还提供了一种非常快速的方法,可产生高达毫克级至低克级量的蛋白质用于体外试验和初步的动物研究。
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