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首页> 外文期刊>Analytical and bioanalytical chemistry >Can Edman degradation be used for quantification? Isotope-dilution liquid chromatography-electrospray ionization tandem mass spectrometry and the long-term stability of 20 phenylthiohydantoin-amino acids Amino Acid Analysis
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Can Edman degradation be used for quantification? Isotope-dilution liquid chromatography-electrospray ionization tandem mass spectrometry and the long-term stability of 20 phenylthiohydantoin-amino acids Amino Acid Analysis

机译:埃德曼退化可以用于量化吗?同位素稀释液相色谱-电喷雾串联质谱法和20苯基硫代乙内酰脲氨基酸的长期稳定性氨基酸分析

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摘要

Edman degradation is a well-known method for obtaining amino acid (AA) sequences from a peptide by means of sequential reactions that release the N-terminal AAs from the peptide as a phenylthiohydantoin (PTH) derivative. Because of unexpected loss during the reaction and handling, there are few reports of use of this reaction for quantification. This manuscript describes the development of isotope-dilution liquid chromatography-electrospray ionization tandem mass spectrometry for 20 PTH-AA derivatives, and long-term stability testing of PTH-AAs to ensure quantitative quality in the reaction. The 20 corresponding [~(13)C_6]-PTH-AAs were prepared by use of a one-pot reaction involving a mixture of [~(13)C_6]-Edman reagent and 20 AAs. Good linearity was observed for standard curves for the PTH-AAs, using the corresponding [~(13)C_6]-PTH-AAs as internal standards (1-100 pmol per injection, r ~2 = 0.989-1.000). Serum albumin (human), pepsin (porcine stomach mucosa), α-casein (bovine milk), ribonuclease A (bovine), lysozyme (chicken egg white), and insulin (bovine) subjected to Edman degradation were examined as model proteins and peptides for N-terminal AA analysis. The results of the impurity test were satisfactory. Yield from the entire reaction with human serum albumin was estimated to be at least 75 %, indicating great potential for absolute quantification of proteins without protein standards. [Figure not available: see fulltext.]
机译:埃德曼降解法是一种众所周知的方法,其通过顺序反应从肽中获得氨基酸(AA)序列,该顺序反应从肽中释放出N末端AA作为苯基硫代乙内酰脲(PTH)衍生物。由于在反应和处理过程中意外损失,很少有报道使用该反应进行定量。该手稿描述了用于20种PTH-AA衍生物的同位素稀释液相色谱-电喷雾串联质谱的开发以及对PTH-AA的长期稳定性测试以确保反应中定量质量的发展。通过使用一锅反应制备20种相应的[〜(13)C_6] -PTH-AAs,该反应涉及[〜(13)C_6] -Edman试剂和20个AAs的混合物。使用相应的[〜(13)C_6] -PTH-AAs作为内标物,对于PTH-AAs的标准曲线观察到良好的线性(每次注射1-100 pmol,r〜2 = 0.989-1.000)。检查了经过埃德曼降解的血清白蛋白(人),胃蛋白酶(猪胃粘膜),α-酪蛋白(牛乳),核糖核酸酶A(牛),溶菌酶(鸡蛋白)和胰岛素(牛)作为模型蛋白质和多肽用于N端AA分析。杂质测试的结果令人满意。与人血清白蛋白的整个反应的产率估计至少为75%,这表明在没有蛋白质标准品的情况下对蛋白质进行绝对定量的巨大潜力。 [图不可用:请参见全文。]

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