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Studying host cell protein interactions with monoclonal antibodies using high throughput protein A chromatography

机译:使用高通量蛋白质A色谱法研究宿主细胞蛋白质与单克隆抗体的相互作用

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Protein A chromatography is typically used as the initial capture step in the purification of monoclonal antibodies produced in Chinese hamster ovary (CHO) cells. Although exploiting an affinity interaction for purification, the level of host cell proteins in the protein A eluent varies significantly with different feedstocks. Using a batch binding chromatography method, we performed a controlled study to assess host cell protein clearance across both MabSelect Sure and Prosep vA resins. We individually spiked 21 purified antibodies into null cell culture fluid generated with a non-producing cell line, creating mock cell culture fluids for each antibody with an identical composition of host cell proteins and antibody concentration. We demonstrated that antibody-host cell protein interactions are primarily responsible for the variable levels of host cell proteins in the protein A eluent for both resins when antibody is present. Using the additives guanidine HCI and sodium chloride, we demonstrated that antibody-host cell protein interactions may be disrupted, reducing the level of host cell proteins present after purification on both resins. The reduction in the level of host cell proteins differed between antibodies suggesting that the interaction likely varies between individual antibodies but encompasses both an electrostatic and hydrophobic component.
机译:蛋白A色谱通常用作纯化中国仓鼠卵巢(CHO)细胞中产生的单克隆抗体的初始捕获步骤。尽管利用亲和力相互作用进行纯化,但蛋白A洗脱液中宿主细胞蛋白的水平随原料的不同而显着不同。使用批处理结合色谱法,我们进行了一项对照研究,评估了MabSelect Sure和Prosep vA树脂之间的宿主细胞蛋白清除率。我们将21种纯化的抗体单独掺入非生产细胞系产生的无效细胞培养液中,为每种抗体创建具有相同宿主细胞蛋白质组成和抗体浓度的模拟细胞培养液。我们证明,当存在抗体时,两种树脂的蛋白A洗脱液中抗体与宿主细胞蛋白的相互作用主要负责宿主细胞蛋白的可变水平。使用添加剂胍盐酸盐和氯化钠,我们证明了抗体-宿主细胞蛋白相互作用可能被破坏,降低了两种树脂纯化后存在的宿主细胞蛋白的水平。抗体之间宿主细胞蛋白质水平的降低有所不同,这表明各个抗体之间的相互作用可能会有所不同,但同时包含静电和疏水成分。

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