Wen Dingyi, Vecchi Malgorzata M, Gu Sheng, Su Lihe, Dolnikova Jana, Huang Yao-Ming, Foley Susan F, Garber Ellen, Pederson Nels, Meier Werner
Biogen Idec Inc., 14 Cambridge Center, Cambridge, Massachusetts 02412, USA.
J Biol Chem. 2009 Nov 20;284(47):32686-94. doi: 10.1074/jbc.M109.059360. Epub 2009 Sep 25.
Misincorporation of amino acids in proteins expressed in Escherichia coli has been well documented but not in proteins expressed in mammalian cells under normal recombinant protein production conditions. Here we report for the first time that Ser can be incorporated at Asn positions in proteins expressed in Chinese hamster ovary cells. This misincorporation was discovered as a result of intact mass measurement, peptide mapping analysis, and tandem mass spectroscopy sequencing. Our analyses showed that the substitution was not related to specific protein molecules or DNA codons and was not site-specific. We believe that the incorporation of Ser at sites coded for Asn was due to mischarging of tRNA(Asn) rather than to codon misreading. The rationale for substitution of Asn by Ser and not by other amino acids is also discussed. Further investigation indicated that the substitution was due to the starvation for Asn in the cell culture medium and that the substitution could be limited by using the Asn-rich feed. These observations demonstrate that the quality of expressed proteins should be closely monitored when altering cell culture conditions.
在大肠杆菌中表达的蛋白质中氨基酸的错误掺入已有充分记录,但在正常重组蛋白生产条件下哺乳动物细胞中表达的蛋白质中尚未见报道。在此,我们首次报道在中华仓鼠卵巢细胞中表达的蛋白质中,丝氨酸(Ser)可掺入天冬酰胺(Asn)位置。这种错误掺入是通过完整质量测量、肽图谱分析和串联质谱测序发现的。我们的分析表明,这种取代与特定蛋白质分子或DNA密码子无关,也不是位点特异性的。我们认为,在编码天冬酰胺的位点掺入丝氨酸是由于tRNA(Asn)的错误负载,而不是密码子误读。本文还讨论了用丝氨酸取代天冬酰胺而非其他氨基酸的原理。进一步研究表明,这种取代是由于细胞培养基中天冬酰胺缺乏,并且通过使用富含天冬酰胺的培养基可以限制这种取代。这些观察结果表明,在改变细胞培养条件时,应密切监测表达蛋白的质量。
