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基于亲和蛋白的荧光共振能量转移工具,用于壳聚糖纳米颗粒的细胞示踪和聚合物乙酰化度的测定。

Affinity protein-based FRET tools for cellular tracking of chitosan nanoparticles and determination of the polymer degree of acetylation.

机构信息

IBBP, Westfälische Wilhelms-Universität Münster Schlossgarten 3, 48149, Münster, Germany.

出版信息

Biomacromolecules. 2014 Jul 14;15(7):2532-9. doi: 10.1021/bm500394v. Epub 2014 Jun 9.

Abstract

Chitosan (CS) is a family of linear polysaccharides with diverse applications in medicine, agriculture, and industry. Its bioactive properties are determined by parameters such as the degree of acetylation (DA), but current techniques to measure the DA are laborious and require large amounts of substrate and sophisticated equipment. It is also challenging to monitor the fate of chitosan-based nanoparticles (CS-NPs) in vitro because current tools cannot measure their enzymatic or chemical degradation. We have developed a method based on the Förster resonance energy transfer (FRET) that occurs between two independent fluorescent proteins fused to a CS-binding domain, who interact with CS polymers or CS-NPs. We used this approach to calibrate a simple and rapid analytical method that can determine the DA of CS substrates. We showed unequivocally that FRET occurs on the surface of CS-NPs and that the FRET signal is quenched by enzymatic degradation of the CS substrate. Finally, we provide in vitro proof-of-concept that these approaches can be used to label CS-NPs and colocalize them following their interactions with mammalian cells.

摘要

壳聚糖(CS)是一组具有多种应用的线性多糖,包括医学、农业和工业等领域。其生物活性取决于乙酰化度(DA)等参数,但目前测量 DA 的技术既繁琐又需要大量的底物和复杂的设备。此外,由于当前的工具无法测量壳聚糖纳米颗粒(CS-NPs)的酶或化学降解,因此体外监测 CS-NPs 的命运也具有挑战性。我们开发了一种基于荧光共振能量转移(FRET)的方法,该方法发生在两个独立的荧光蛋白与壳聚糖结合域融合后,它们与 CS 聚合物或 CS-NPs 相互作用。我们使用这种方法对一种简单快速的分析方法进行了校准,该方法可以确定 CS 底物的 DA。我们明确表明,FRET 确实发生在 CS-NPs 的表面,并且 CS 底物的酶促降解会猝灭 FRET 信号。最后,我们提供了体外概念验证,证明这些方法可用于标记 CS-NPs 并在其与哺乳动物细胞相互作用后对其进行共定位。

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