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首页> 外文期刊>Proceedings of the National Academy of Sciences of the United States of America >Site-specific Chemical Modification Of Recombinant Proteins Produced In Mammalian Cells By Using The Genetically Encoded Aldehyde Tag
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Site-specific Chemical Modification Of Recombinant Proteins Produced In Mammalian Cells By Using The Genetically Encoded Aldehyde Tag

机译:通过使用基因编码的醛标记在哺乳动物细胞中产生的重组蛋白的定点化学修饰。

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摘要

The properties of therapeutic proteins can be enhanced by chemical modification. Methods for site-specific protein conjugation are critical to such efforts. Here, we demonstrate that recombinant proteins expressed in mammalian cells can be site-specifically modified by using a genetically encoded aldehyde tag. We introduced the peptide sequence recognized by the endoplasmic retic-ulum (ER)-resident formylglycine generating enzyme (FGE), which can be as short as 6 residues, into heterologous proteins expressed in mammalian cells. Cotranslational modification of the proteins by FGE produced products bearing a unique aldehyde group. Proteins bearing this "aldehyde tag" were chemically modified by selective reaction with hydrazide- or aminooxy-functionalized reagents. We applied the technique to site-specific modification of monoclonal antibodies, the fastest growing class of biopharmaceuticals, as well as membrane-associated and cytosolic proteins expressed in mammalian cells.
机译:治疗性蛋白质的性质可以通过化学修饰来增强。位点特异性蛋白结合的方法对于此类努力至关重要。在这里,我们证明了哺乳动物细胞中表达的重组蛋白可以通过使用遗传编码的醛标记进行位点特异性修饰。我们将内质网(ER)驻留的甲酰甘氨酸生成酶(FGE)识别的肽序列(短至6个残基)引入哺乳动物细胞中表达的异源蛋白质中。 FGE对蛋白质进行共翻译修饰,产生的产物带有独特的醛基。通过与酰肼或氨基氧基官能化试剂的选择性反应,对带有“醛标签”的蛋白质进行了化学修饰。我们将该技术应用于单克隆抗体的位点特异性修饰,发展最快的一类生物药物以及在哺乳动物细胞中表达的膜相关蛋白和胞质蛋白。

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