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首页> 外文期刊>Proteomics >Top-down analysis of recombinant histone H3 and its methylated analogs by ESI/FT-ICR mass spectrometry.
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Top-down analysis of recombinant histone H3 and its methylated analogs by ESI/FT-ICR mass spectrometry.

机译:通过ESI / FT-ICR质谱从上至下分析重组组蛋白H3及其甲基化类似物。

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Detailed characterization of the amino acid (aa) compositions of recombinant histone H3 (Xenopus laevis) and its Lys-9 mono-, di-, and trimethylated isoforms was carried out by ESI/FT-ICR-MS. The measured molecular masses of these four proteins did not agree with those predicted from the published wild-type histone H3 sequence. Using MS/MS with both collision-activated dissociation and electron capture dissociation, three aa substitutions (Gly102Ala, Cys110Ala, and Gly111Ala) were unambiguously identified in each protein by protein database searching and de novo peptide tag sequencing. In addition, it was determined through accurate mass measurement and elemental composition generation that Lys-9, to which the methyl groups are attached, is not in fact a lysine. Instead, it was identified as a chemical analog of lysine--aminoethylcysteine--in the methylated proteins. After incorporation of these three aa substitutions and the aminoethylcysteine into the protein sequences, the re-calculated molecular masses of four proteins were completely consistent with the measured values within 1 ppm. This work demonstrates the power of top-down MS for a detailed structural confirmation of recombinant proteins, even without prior information on aa substitutions or modifications.
机译:通过ESI / FT-ICR-MS对重组组蛋白H3(非洲爪蟾)及其Lys-9单,二和三甲基化同工型的氨基酸(aa)组成进行了详细表征。这四种蛋白质的测量分子量与根据已发表的野生型组蛋白H3序列预测的分子量不同。使用同时具有碰撞激活解离和电子捕获解离的MS / MS,通过蛋白质数据库搜索和从头肽标记测序,可以在每种蛋白质中明确鉴定出三个氨基酸取代(Gly102Ala,Cys110Ala和Gly111Ala)。另外,通过精确的质量测量和元素组成的产生,确定甲基所连接的Lys-9实际上不是赖氨酸。相反,它被鉴定为甲基化蛋白质中赖氨酸的化学类似物-氨基乙基半胱氨酸。将这三个氨基酸取代和氨基乙基半胱氨酸并入蛋白质序列后,四种蛋白质的重新计算分子量与1 ppm内的测量值完全一致。这项工作证明了自上而下的MS能够对重组蛋白进行详细的结构确认,甚至无需事先获得有关氨基酸置换或修饰的信息。

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