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Primary structure of rat spermidine synthase: an example of refining the cDNA-derived amino acid sequence.

机译:大鼠亚精胺合酶的一级结构:完善cDNA衍生氨基酸序列的一个例子。

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摘要

The primary structure of rat spermidine synthase having the N-terminal acetylated methionine and 98.7% homology with that of the mouse enzyme is presented using a limited amount of the homogeneous enzyme. The study strategy was principally to compare the molecular masses of liberated peptides determined by three specific cleavage methods with those expected from known cDNA-derived amino acid sequences of mouse and human enzymes using matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI TOF-MS). The cleavage methods involved two enzymatic methods using lysylendopeptidase and arginylendopeptidase, and a chemical method for cleaving at the cysteine residue using 2-nitro-5-thiocyanobenzoic acid. Their usefulness was clearly demonstrated. Column-switching semimicro reversed-phase HPLC, which permits application of the entire reaction mixture, was useful for collecting a small amount of peptides containing the N-terminal amino acid, to confirm acetylation of the N-terminal methionine by MALDI TOF-MS. It was necessary in this approach to examine the amino acid sequence of certain peptides. The Edman method was used for the sequence analysis, and this will be replaced by an improved MALDI TOF-MS now available in a few laboratories.
机译:使用有限量的均质酶呈现了具有亚基N-末端蛋氨酸和与小鼠酶具有98.7%同源性的大鼠亚精胺合酶的一级结构。该研究策略主要是通过基质辅助激光解吸/电离飞行时间质谱法比较三种特定裂解方法测定的释放肽的分子量与小鼠和人类酶的已知cDNA衍生氨基酸序列所预期的分子量(MALDI TOF-MS)。裂解方法包括使用赖氨酰内肽酶和精氨酰内肽酶的两种酶促方法,以及使用2-硝基-5-硫代氰基苯甲酸在半胱氨酸残基上裂解的化学方法。清楚地证明了它们的有用性。允许应用整个反应混合物的色谱柱切换半微量反相HPLC可用于收集少量含有N末端氨基酸的肽,以通过MALDI TOF-MS确认N末端甲硫氨酸的乙酰化。用这种方法必须检查某些肽的氨基酸序列。埃德曼方法用于序列分析,现在将由少数实验室中提供的改良的MALDI TOF-MS代替。

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