Novel sodium-selective fluorescent PET and optically based chemosensors: towards Na+ determination in serum

T. Gunnlaugsson, M. Nieuwenhuyzen, L. Richard, V. Thoss
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引用次数: 23

Abstract

The anthracene based fluorescent PET chemosensor 1 and the azo-dye based chemosensor 2 show high selectivity for Na+ over other alkali and alkaline-earth metal cations in the 12–300 mM concentration range in 50 ∶ 50 MeOH–H2O at pH 7.4. Chemosensor 1 shows fluorescence ‘off-on’ switching upon Na+ complexation with λFmax of 440 nm and a log βNa of 2.5 (±0.05) and a pKa of 5.3 with no concomitant changes in the absorption spectra. Conversely, 2 displays only a weak fluorescent emission at around 520–640 nm, and large changes in its absorption spectra upon addition of Na+, with a log βNa of 1.25 (±0.05) and a pKa of 3.9. In 100% water the sensitivity of 2 for Na+ was somewhat lower with a log βNa of 0.8 (±0.05). The crystal structure of 2, and its corresponding protonated form (2·H+) were obtained, showing 2 in its trans conformation with the crown ether moiety at a 75° angle to the plane of the chromophore. These results, in conjunction with 1H NMR measurements of 2, and UV–VIS measurements of the ion receptor 3, suggest that upon complexation of Na+, the 2′-methoxy group of the crown receptor participates in the Na+ complexation through chelation to the Na+ ion. We propose that this interaction forces the amine moiety of the crown ether to twist out of the plane of the chromophore, inducing loss of conjugation which gives rise to large Na+-induced spectral changes in the absorption spectra, which are most noticeable for 2.
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新型钠选择性荧光PET和光学化学传感器:用于血清中Na+的测定
蒽基荧光PET化学传感器1和偶氮染料化学传感器2在pH 7.4、50∶50 MeOH-H2O、12 ~ 300 mM浓度范围内对Na+有较高的选择性。Chemosensor 1在Na+络合时显示荧光“off-on”开关,λFmax为440 nm, log βNa为2.5(±0.05),pKa为5.3,吸收光谱无变化。相反,2在520-640 nm附近只有微弱的荧光发射,在加入Na+后,其吸收光谱变化很大,对数βNa为1.25(±0.05),pKa为3.9。在100%水中,2对Na+的敏感性略低,对数βNa为0.8(±0.05)。得到了2的晶体结构及其对应的质子化形式(2·H+),显示出2的反式构象,其冠醚部分与发色团平面成75°角。这些结果,结合2的1H NMR测量和离子受体3的UV-VIS测量,表明在Na+络合时,冠受体的2 ' -甲氧基通过与Na+离子的螯合参与Na+络合。我们提出,这种相互作用迫使冠醚的胺部分扭曲出发色团平面,导致共轭丧失,从而导致吸收光谱中Na+诱导的大光谱变化,这在2中最为明显。
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