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Utility of the Phenacyl Protecting Group in Traceless Protein Semisynthesis through Ligation–Desulfurization Chemistry

机译:苯甲酰基保护基在通过连接-脱硫化学进行无痕蛋白质半合成中的应用

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摘要

Semisynthesis of proteins via expressed protein ligation is a widely applicable method, even more so because of the possibility of ligation at non‐cysteine sites using β‐mercapto amino acids that can be converted to the corresponding native amino acids by desulfurization. A drawback of this ligation– desulfurization approach is the removal of any unprotected native cysteine residues within the ligated protein segments. Here, we show that the phenacyl (PAc) moiety can be successfully used to protect cysteines within recombinantly generated protein segments. As such, this group was selectively appended onto cysteine side chains within bacterially expressed polypeptides following intein cleavage, which reveals a rather sensitive thioester at the C‐terminus. The PAc group proved to be compatible with native chemical ligation, radical desulfurization, and reverse‐phase HPLC conditions, and was smoothly removed at the end. The utility of the PAc protecting group was then demonstrated by the ‘traceless’ semisynthesis of two proteins containing one or two native cysteines: human small heat shock protein Hsp27 and murine prion protein.
机译:通过表达的蛋白质连接来半合成蛋白质是一种广泛应用的方法,甚至更是如此,因为使用β-巯基氨基酸可以在非半胱氨酸位点进行连接,并且可以通过脱硫将其转化为相应的天然氨基酸。这种连接-脱硫方法的缺点是去除了连接蛋白片段中任何未保护的天然半胱氨酸残基。在这里,我们表明,苯甲酰基(PAc)部分可以成功地用于保护重组生成的蛋白质片段内的半胱氨酸。因此,在内含肽切割后,该组被选择性地附加到细菌表达的多肽内的半胱氨酸侧链上,这揭示了C端相当敏感的硫酯。事实证明,PAc组与天然化学连接,自由基脱硫和反相HPLC条件兼容,最后被顺利去除。然后,通过“无痕”半合成两种包含一种或两种天然半胱氨酸的蛋白质来证明PAc保护基的效用:人小热休克蛋白Hsp27和鼠病毒蛋白。

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