重组DNA
抗体
分子生物学
圆二色性
化学
酶
表面等离子共振
亲和层析
抗原
生物化学
生物
色谱法
基因
免疫学
纳米技术
纳米颗粒
材料科学
作者
Makoto Mizukami,Hiromasa Onishi,Hiroshi Hanagata,Akira Miyauchi,Yuji Ito,Hiroko Tokunaga,Matsujiro Ishibashi,Tsutomu Arakawa,Masao Tokunaga
标识
DOI:10.1016/j.pep.2018.05.013
摘要
The Brevibacillus expression system has been successfully employed for the efficient productions of a variety of recombinant proteins, including enzymes, cytokines, antigens and antibody fragments. Here, we succeeded in secretory expression of Trastuzumab Fab antibody fragments using B. choshinensis/BIC (Brevibacillus in vivocloning) expression system. In the fed-batch high-density cell culture, recombinant Trastuzumab Fab with amino-terminal His-tag (His-BcFab) was secreted at high level, 1.25 g/liter, and Fab without His-tag (BcFab) at ∼145 mg/L of culture supernatant. His-BcFab and BcFab were purified to homogeneity using combination of conventional column chromatographies with a yield of 10-13%. This BcFab preparation exhibited native structure and functions evaluated by enzyme-linked immunosorbent assay, surface plasmon resonance, circular dichroism measurements and size exclusion chromatography. To our knowledge, this is the highest production of Fab antibody fragments in gram-positive bacterial expression/secretion systems.
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