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首页> 外文期刊>Journal of chromatography, A: Including electrophoresis and other separation methods >DETERMINATION OF PROTEIN AMINO ACIDS AS BENZYLTHIOCARBAMYL DERIVATIVES COMPARED WITH PHENYLTHIOCARBAMYL DERIVATIVES BY REVERSED-PHASE HIGH-PERFORMANCE LIQUID CHROMATOGRAPHY, ULTRAVIOLET DETECTION AND PRECOLUMN DERIVATIZATION
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DETERMINATION OF PROTEIN AMINO ACIDS AS BENZYLTHIOCARBAMYL DERIVATIVES COMPARED WITH PHENYLTHIOCARBAMYL DERIVATIVES BY REVERSED-PHASE HIGH-PERFORMANCE LIQUID CHROMATOGRAPHY, ULTRAVIOLET DETECTION AND PRECOLUMN DERIVATIZATION

机译:反相高效液相色谱,紫外检测和柱前衍生

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摘要

All 22 protein amino acids were successfully derivatized to benzylthiocarbamyl (BZTC) derivatives by precolumn reaction at 50 degrees C for 30 min with benzylisothiocyanate (BZITC) and separated in 35 min on a reversed-phase Nova-Pak C-18 column (30 cmX3.9 mm, 4 mu m). However, phenylthiocarbamyl-derivatives were not completely separated on this column; in particular cystine and cysteine were resolved into a single peak. The optimum wavelength for determination of BZTC derivatives was 246 nm although the strong absorption wavelengths were 220 nm and 238 nm. The relative standard deviations (R.S.D.) of the relative molar response to the internal standard (norleucine) were less than 5%, except for cysteine (7.22%); however for the PTC derivatives, glutamine, proline, threonine, alanine, leucine, cystine+cysteine and lysine the R.S.D. values exceeded 5%. Standard calibration curves showed good linearity in the measured range from 0.125 to 5 nmol. The correlation coefficient of cystine was the lowest, 0.952. The stability of BZTC derivatives of standard amino acids was about 120 h except for threonine, alanine, cystine and serine. The detection limit was about 3.9 pmol at 0.05 AUFS in both of BZTC and PTC derivatives. The compositions of amino acids of soybean and bovine serum albumin (BSA) analyzed with both derivatives were similar to the results found in the literature and food composition tables, except for cysteine. The BZTC derivatives of cystine and cysteine in soybean and BSA could be determined separately, but the PTC derivatives could not, nor could data on separate dertermination of cysteine and cystine be found in the literature studied.
机译:通过在50摄氏度下与异硫氰酸苄酯(BZITC)在50摄氏度下进行预柱反应,将所有22个蛋白质氨基酸成功衍生为苄硫基甲酰胺(BZTC)衍生物,并在35分钟的反相Nova-Pak C-18色谱柱(30 cmX3)上分离。 9毫米,4微米)。但是,苯硫代氨基甲酰基衍生物在此色谱柱上并未完全分离。特别是胱氨酸和半胱氨酸被解析为一个峰。尽管强吸收波长为220 nm和238 nm,但用于测定BZTC衍生物的最佳波长为246 nm。相对于内标(正亮氨酸)的相对摩尔反应的相对标准偏差(R.S.D.)小于5%(半胱氨酸除外)(7.22%);但是对于PTC衍生物,谷氨酰胺,脯氨酸,苏氨酸,丙氨酸,亮氨酸,胱氨酸+半胱氨酸和赖氨酸的R.S.D.值超过5%。标准校准曲线在0.125至5 nmol的测量范围内显示出良好的线性。胱氨酸的相关系数最低,为0.952。除苏氨酸,丙氨酸,胱氨酸和丝氨酸外,标准氨基酸的BZTC衍生物的稳定性约为120小时。 BZTC和PTC衍生物在0.05 AUFS下的检出限约为3.9 pmol。用这两种衍生物分析的大豆和牛血清白蛋白(BSA)的氨基酸组成与文献和食品组成表中的结果相似,除了半胱氨酸。大豆和BSA中的半胱氨酸和半胱氨酸的BZTC衍生物可以分别测定,但是PTC衍生物不能,在研究的文献中也找不到半胱氨酸和半胱氨酸分别测定的数据。

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