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用于通过高效液相色谱法在两种不同样品中同时检测肽和蛋白质的荧光试剂的合成与评价。

Synthesis and evaluation of fluorogenic reagents for simultaneous detection of peptides and proteins by HPLC in two different samples.

作者信息

Saimaru Hiroshi, Yasui Eiko, Takamura Norio, Imai Kazuhiro

机构信息

Research Institute of Pharmaceutical Sciences, Musashino University, Nishitokyo-shi, Tokyo, Japan.

出版信息

Biomed Chromatogr. 2006 Jun-Jul;20(6-7):576-84. doi: 10.1002/bmc.681.

Abstract

To find the pairs of fluorogenic reagents having similar retention times in HPLC but with different fluorescent characteristics, six fluorogenic reagents bearing benzoxadiazole or benzoselenadiazole skeletons were synthesized. The resultant derivatives obtained from the reaction of peptides and proteins with reagents which have a benzoselenadiazole skeleton showed different fluorescence characteristics from those with a benzoxadiazole skeleton. Since each corresponding derivatives of trypsin inhibitor and BSA with DAABD-Cl and 7-fluoro-N-[2-(diethylamino)ethyl]-2,1,3-benzoselenadiazole-4-sulfonamide (DEAEABSeD-F) have similar retention times, the pair of reagents was adopted for the sensitive simultaneous detection of proteins in two different samples. When the soluble fraction of mouse hippocampus was divided into the two samples (A and B), each was reacted with DEAEABSeD-F for A and DAABD-Cl for B, respectively. The two reaction solutions were combined and subjected to HPLC analysis with two fluorescent detectors in series (excitation and emission at different wavelengths for A and B, respectively). The resultant two chromatograms had quite similar patterns for each other. The new pair of fluorogenic reagents (DAABD-Cl and DEAEABSeD-F) would be applicable to proteomics studies using the previously reported FD-LC-MS/MS method.

摘要

为了找到在高效液相色谱(HPLC)中保留时间相似但荧光特性不同的荧光试剂对,合成了六种带有苯并恶二唑或苯并硒二唑骨架的荧光试剂。肽和蛋白质与具有苯并硒二唑骨架的试剂反应得到的衍生物,其荧光特性与具有苯并恶二唑骨架的试剂反应得到的衍生物不同。由于胰蛋白酶抑制剂和牛血清白蛋白(BSA)与4-氯-7-(二乙氨基)-2,1,3-苯并恶二唑(DAABD-Cl)和7-氟-N-[2-(二乙氨基)乙基]-苯并[ c ]硒二唑-4-磺酰胺(DEAEABSeD-F)的相应衍生物具有相似的保留时间,因此采用这对试剂对两个不同样品中的蛋白质进行灵敏的同时检测。将小鼠海马体的可溶部分分成两个样品(A和B),分别使A与DEAEABSeD-F反应,B与DAABD-Cl反应。将两种反应溶液合并,并用串联的两个荧光检测器进行HPLC分析(分别在不同波长下对A和B进行激发和发射)。得到的两个色谱图彼此模式非常相似。这对新的荧光试剂(DAABD-Cl和DEAEABSeD-F)将适用于使用先前报道的荧光检测液相色谱-串联质谱(FD-LC-MS/MS)方法的蛋白质组学研究。

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