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Application of reverse-phase HPLC to quantify oligopeptide acetylation eliminates interference from unspecific acetyl CoA hydrolysis

机译:应用反相HPLC定量寡肽乙酰化可消除非特异性乙酰辅酶A水解的干扰

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摘要

Protein acetylation is a common modification that plays a central role in several cellular processes. The most widely used methods to study these modifications are either based on the detection of radioactively acetylated oligopetide products or an enzyme-coupled reaction measuring conversion of the acetyl donor acetyl CoA to the product CoASH. Due to several disadvantages of these methods, we designed a new method to study oligopeptide acetylation. Based on reverse phase HPLC we detect both reaction products in a highly robust and reproducible way. The method reported here is also fully compatible with subsequent product analysis, e.g. by mass spectroscopy. The catalytic subunit, hNaa30p, of the human NatC protein N-acetyltransferase complex was used for N-terminal oligopeptide acetylation. We show that unacetylated and acetylated oligopeptides can be efficiently separated and quantified by the HPLC-based analysis. The method is highly reproducible and enables reliable quantification of both substrates and products. It is therefore well-suited to determine kinetic parameters of acetyltransferases.
机译:蛋白质乙酰化是一种常见的修饰,在几种细胞过程中起着核心作用。研究这些修饰的最广泛使用的方法是基于放射性乙酰化寡核苷酸产物的检测,或者是测量乙酰基供体乙酰基CoA向产物CoASH转化的酶联反应。由于这些方法的几个缺点,我们设计了一种研究寡肽乙酰化的新方法。基于反相HPLC,我们以高度耐用且可重现的方式检测两种反应产物。此处报告的方法也与后续产品分析完全兼容,例如通过质谱。人类NatC蛋白N-乙酰基转移酶复合物的催化亚基hNaa30p用于N端寡肽乙酰化。我们显示未乙酰化和乙酰化的寡肽可以有效地分离和量化基于HPLC的分析。该方法具有很高的重现性,可以对底物和产物进行可靠的定量。因此非常适合确定乙酰转移酶的动力学参数。

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