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重组人干扰素-γ。糖基化和蛋白水解加工的差异导致分批培养中的异质性。

Recombinant human interferon-gamma. Differences in glycosylation and proteolytic processing lead to heterogeneity in batch culture.

作者信息

Curling E M, Hayter P M, Baines A J, Bull A T, Gull K, Strange P G, Jenkins N

机构信息

Biological Laboratory, University of Kent, Canterbury, U.K.

出版信息

Biochem J. 1990 Dec 1;272(2):333-7. doi: 10.1042/bj2720333.

Abstract

Recombinant human interferon-gamma (Hu-IFN-gamma) produced by Chinese-hamster ovary (CHO) cells was analysed by immunoprecipitation and SDS/PAGE. Up to twelve molecular-mass variants were secreted by this cell line. Three variants were recovered after enzymic removal of all N-linked oligosaccharides or when glycosylation was inhibited by tunicamycin. The presence of three polypeptide forms rather than a single form suggested that proteolytic cleavage had occurred at two sites in both the glycosylated and non-glycosylated forms. Proteolytically cleaved IFN-gamma was more prevalent in cell lysates than in the secreted glycoprotein. In common with naturally produced IFN-gamma, both fully glycosylated IFN-gamma (asparagine residues 28 and 100 occupied) and partially glycosylated product (thought to be substituted at position Asn28) were secreted. This was deduced from the Mr of the glycosylated products and the relative amounts of sialic acid expressed by each variant. In contrast with naturally produced IFN-gamma, non-glycosylated IFN-gamma was also secreted by the transfected CHO cells. When the cells were grown in batch culture in serum-free medium under pH and dissolved-oxygen control, the proportion of non-glycosylated IFN-gamma increased from 3 to 5% after 3 h, to 30% of the total IFN-gamma present after 195 h. This change in the proportion of glycosylated protein produced was not seen when metabolically labelled IFN-gamma was incubated for 96 h with cell-free supernatant from actively growing CHO cells. This implied that an alteration in intracellular glycosylation was occurring rather than a degradation of oligosaccharide side chains after secretion. The decrease in IFN-gamma glycosylation was independent of the glucose concentration in the culture medium, but could be related to specific growth and IFN-gamma production rates, as these declined steadily after 50 h of culture, in line with the increased production of non-glycosylated IFN-gamma.

摘要

采用免疫沉淀和SDS/PAGE方法分析了中国仓鼠卵巢(CHO)细胞产生的重组人干扰素-γ(Hu-IFN-γ)。该细胞系分泌多达12种分子量变异体。用酶去除所有N-连接寡糖后或用衣霉素抑制糖基化时,回收了3种变异体。存在三种多肽形式而非单一形式,这表明在糖基化和非糖基化形式中均在两个位点发生了蛋白水解切割。蛋白水解切割的IFN-γ在细胞裂解物中比在分泌的糖蛋白中更普遍。与天然产生的IFN-γ一样,完全糖基化的IFN-γ(天冬酰胺残基28和100被占据)和部分糖基化产物(认为在Asn28位置被取代)均被分泌。这是根据糖基化产物的相对分子质量以及每种变异体表达的唾液酸相对量推断出来的。与天然产生的IFN-γ不同,转染的CHO细胞也分泌非糖基化的IFN-γ。当细胞在pH和溶解氧控制下的无血清培养基中进行分批培养时,非糖基化IFN-γ的比例在3小时后从3%增加到5%,在195小时后占总IFN-γ的30%。当用代谢标记的IFN-γ与活跃生长的CHO细胞的无细胞上清液孵育96小时时,未观察到产生的糖基化蛋白比例的这种变化。这意味着发生了细胞内糖基化改变,而不是分泌后寡糖侧链的降解。IFN-γ糖基化的降低与培养基中的葡萄糖浓度无关,但可能与特定的生长和IFN-γ产生速率有关,因为在培养50小时后这些速率稳步下降,这与非糖基化IFN-γ产量的增加一致。

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