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Fluorescent Sensor for Imidazole Derivatives Based on Monomer-Dimer Equilibrium of a Zinc Porphyrin Complex in a Polymeric Film

机译:基于聚合物膜中锌卟啉配合物的单体-二聚物平衡的咪唑衍生物荧光传感器

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A new zinc(II) porphyrin conjugate with an appended pyrene subunit has been synthesized and shown to exhibit significant and analytical usefulness for fluorescence sensing toward imidazole derivatives. The molecular recognition was based on the bridging interaction of the imidazole ring of analyte with the zinc(II) center of the porphyrin, while the transduction signal for the recognition process was the pyrene excimer fluorescence. The sensor was constructed and applied for fluorescence assay of histidine in aqueous solution by immobilizing the sensing material in a plasticized PVC membrane. When the membrane was bathed in an alkaline solution void of histidine, zinc(II) porphyrin was present in the monomer form, and pyrene emitted monomer fluorescence at 378 and 397 nm. With the presence of histidine in the sample solution, histidine was extracted into the membrane phase and bridged with the Zn(II) center of the porphyrin, causing the monomer porphyrin to be converted to its dimeric species. Since the formation of porphyrin dimer was accompanied by the enhancement of pyrene excimer emission at 454 nm, the chemical recognition process could be directly translated into a fluorescent signal. With the optode membrane M1 described, histidine in sample solution from 6.76×10~(-7) to 5.01×10~(-3) M can be determined. The limit of detection was 1.34×10~(-7) M. The optical selectivity coefficient obtained for histidine over biologically relevant amino acids and anions met the selectivity requirements for the determination of histidine in biological samples. Serum histidine values obtained by the optode membrane fell in the normal range of the content reported in the literature and were in good agreement with those obtained by HPLC.
机译:已经合成了具有附加的sub亚基的新型锌(II)卟啉共轭物,并显示出对咪唑衍生物进行荧光传感的显着和分析有用性。分子识别基于分析物的咪唑环与卟啉锌(II)中心的桥连作用,而识别过程的转导信号是was准分子荧光。通过将传感材料固定在增塑的PVC膜中,可以构建传感器并将其用于水溶液中组氨酸的荧光分析。当将膜浸入没有组氨酸的碱性溶液中时,卟啉锌(II)以单体形式存在,并且pyr在378和397nm处发射单体荧光。在样品溶液中存在组氨酸的情况下,组氨酸被萃取到膜相中并与卟啉的Zn(II)中心桥接,从而使卟啉单体转化为其二聚体。由于卟啉二聚体的形成伴随着exc准分子在454 nm处发射的增强,因此化学识别过程可以直接转化为荧光信号。利用所述的光电二极管膜M1,可以确定样品溶液中的组氨酸为6.76×10〜(-7)M至5.01×10〜(-3)M。检测限为1.34×10〜(-7)M。组氨酸在生物相关氨基酸和阴离子上的光学选择系数满足生物样品中组氨酸测定的选择性要求。通过光电二极管膜获得的血清组氨酸值在文献报道的含量的正常范围内,并且与通过HPLC获得的组氨酸值非常一致。

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