对温度和多胺反应的荧光尼罗蓝官能化聚(N-异丙基丙烯酰胺)微凝胶

SmartMat Pub Date : 2024-01-02 DOI:10.1002/smm2.1254
Qiming Shen, Changhao Fang, Liang Hu, M. Serpe
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引用次数: 0

摘要

我们合成了荧光聚(N-异丙基丙烯酰胺-尼罗河蓝)(pNIPAm-co-NB)微凝胶,这种微凝胶的荧光强度变化与水温有关。众所周知,NB 的荧光强度取决于环境的疏水性,而 pNIPAm 基微凝胶在温度高于 32 °C 时会从膨胀(亲水性)转变为塌陷(相对疏水性);因此,我们将上述行为归因于微凝胶的疏水性随温度升高而变化。这一现象归根结底是由于 NB 二聚体(荧光相对熄灭)在微凝胶的疏水环境中被破坏,从而导致荧光相对增强。我们接着证明,在 pNIPAm-co-NB 微凝胶中引入葫芦[7]脲(CB[7])可增强其荧光,使其可用于多胺(如精胺 [SPM])检测。具体来说,CB[7] 与微凝胶中的 NB 形成主客体相互作用,从而防止 NB 二聚化并增强其荧光。当 SPM 存在时,它形成的主-客复合物比 CB[7]-NB 的主-客相互作用更有利,从而释放 NB 使其二聚化并导致荧光淬灭。因此,我们可以生成一种 SPM 传感器,能够在血清和尿液等复杂基质中检测低至 ~0.5 µmol/L 的 SPM。
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Fluorescent Nile blue‐functionalized poly (N‐isopropylacrylamide) microgels responsive to temperature and polyamines
Fluorescent poly(N‐isopropylacrylamide‐co‐Nile blue) (pNIPAm‐co‐NB) microgels were synthesized that exhibited fluorescence intensity changes in a water temperature‐dependent fashion. NB is well known to exhibit fluorescence intensity that depends on the hydrophobicity of the environment, while pNIPAm‐based microgels are well known to transition from swollen (hydrophilic) to collapsed (relatively hydrophobic) at temperatures greater than 32 °C; hence, we attribute the above behavior to the hydrophobicity changes of the microgels with increasing temperature. This phenomenon is ultimately due to NB dimers (relatively quenched fluorescence) being broken in the hydrophobic environment of the microgels leading to relatively enhanced fluorescence. We went on to show that the introduction of cucurbit[7]uril (CB[7]) into the pNIPAm‐co‐NB microgels enhanced their fluorescence allowing them to be used for polyamine (e.g., spermine [SPM]) detection. Specifically, CB[7] forms a host–guest interaction with NB in the microgels, which prevents NB dimerization and enhances their fluorescence. When SPM is present, it forms a host–guest complex that is favored over the CB[7]‐NB host–guest interaction, which frees the NB for dimerization and leads to fluorescence quenching. As a result, we could generate an SPM sensor capable of SPM detection down to ~0.5 µmol/L in complicated matrixes such as serum and urine.
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