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Enhancement of sialylation on humanized IgG-like bispecific antibody by overexpression of α2,6-sialyltransferase derived from Chinese hamster ovary cells

机译:通过过表达中国仓鼠卵巢细胞的α2,6-唾液酸转移酶来增强人源化IgG样双特异性抗体的唾液酸化作用

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摘要

Improvement of glycosylation is one of the most important topics in the industrial production of therapeutic antibodies. We have focused on terminal sialylation with alpha-2,6 linkage, which is crucial for anti-inflammatory activity. In the present study, we have successfully cloned cDNA of beta-galactosyl alpha-2,6 sialyltransferase (ST6Gal I) derived from Chinese hamster ovary (CHO) cells regardless of reports that stated this was not endogenously expressed in CHO cells. After expressing cloned ST6Gal I in Escherichia coli, the transferase activity was confirmed by HPLC and lectin binding assay. Then, we applied ST6Gal I to alpha-2,6 sialylation of the recombinant antibody; the ST6Gal I expression vector was transfected into the CHO cell line producing a bispecific antibody. The N-glycosylation pattern of the antibody was estimated by HPLC and sialidase digestion. About 70% of the total N-linked oligosaccharide was alpha-2,6 sialylated in the transfected cell line whereas no sialylation was observed in the non-transfected cell line. The improvement of sialylation would be of practical importance for the industrial production of therapeutic antibodies.
机译:糖基化的改善是治疗性抗体的工业生产中最重要的主题之一。我们专注于末端唾液酸化与alpha-2,6链接,这对抗炎活性至关重要。在本研究中,我们成功地克隆了源自中国仓鼠卵巢(CHO)细胞的β-半乳糖基α-2,6唾液酸转移酶(ST6Gal I)cDNA,尽管有报道称这不是在CHO细胞中内源表达的。在大肠杆菌中表达克隆的ST6Gal I后,通过HPLC和凝集素结合测定法确认转移酶活性。然后,我们将ST6Gal I应用于重组抗体的α-2,6唾液酸化;将ST6Gal I表达载体转染到CHO细胞系中,产生双特异性抗体。通过HPLC和唾液酸酶消化来估计抗体的N-糖基化模式。 N-连接的寡糖总量中约70%在转染的细胞系中被唾液酸化为α-2,6,而在未转染的细胞系中未观察到唾液酸化。唾液酸化的改善对于治疗性抗体的工业生产将具有实际重要性。

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