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葫芦脲-四甲基罗丹明缀合物用于直接传感和细胞成像。

Cucurbit[7]uril-Tetramethylrhodamine Conjugate for Direct Sensing and Cellular Imaging.

机构信息

Department of Chemistry and Biochemistry, University of Maryland , College Park, Maryland 20742, United States.

出版信息

J Am Chem Soc. 2016 Dec 21;138(50):16549-16552. doi: 10.1021/jacs.6b11140. Epub 2016 Dec 8.

Abstract

This paper describes the design and synthesis of a conjugate (Q7R) comprising the synthetic host cucurbit[7]uril (Q7) linked to the fluorescent dye tetramethylrhodamine (TMR), and the characterization of its optical and guest-binding properties as well as its cellular uptake. Q7R was synthesized in two steps from monofunctionalized azidobutyl-Q7 and NHS-activated TMR. The fluorescence of Q7R is quenched upon guest binding, and this observable was used to determine equilibrium dissociation constant (K) values. Unexpectedly, the K values for guests binding to Q7R and to unmodified Q7 were essentially identical. Therefore, Q7R can directly report binding to Q7 without an energetic penalty due to the conjugated fluorophore. This result demonstrates a potentially general strategy for the design of single-component host-indicator conjugates that respond sensitively to analytes without perturbing the binding properties of the host. The unique properties of Q7R enabled measurement of K values across 3 orders of magnitude and at concentrations as low as 0.7 nM. This result is particularly relevant given the unmatched range of guests and binding affinities demonstrated for Q7. Confocal fluorescence microscopy of live and fixed HT22 neurons revealed the cellular uptake of Q7R and its punctate localization in the cytoplasm. Q7R did not alter cell growth at concentrations up to 2.2 μM over 4 days. These experiments demonstrate the feasibility of Q7R as a direct sensor for guest binding and as a cell-permeable compound for imaging applications.

摘要

本文描述了一种缀合物(Q7R)的设计和合成,该缀合物由合成主体葫芦[7]脲(Q7)与荧光染料四甲基罗丹明(TMR)连接而成,并对其光学和客体结合特性以及细胞摄取进行了表征。Q7R 由单官能化叠氮丁基-Q7 和 NHS 活化的 TMR 两步合成。Q7R 的荧光在客体结合时被猝灭,可利用这一可观察现象来确定平衡解离常数(K)值。出人意料的是,与 Q7R 和未修饰的 Q7 结合的客体的 K 值基本相同。因此,Q7R 可以直接报告与 Q7 的结合,而不会由于共轭荧光团而产生能量损失。该结果表明,对于设计对分析物敏感而不改变主体结合特性的单组分主体指示剂缀合物,这可能是一种通用策略。Q7R 的独特性质使 K 值的测量范围跨越 3 个数量级,浓度低至 0.7 nM。鉴于 Q7 所展示的无与伦比的客体范围和结合亲和力,这一结果尤其相关。活细胞和固定 HT22 神经元的共聚焦荧光显微镜显示了 Q7R 的细胞摄取及其在细胞质中的点状定位。在 4 天内,浓度高达 2.2 μM 时,Q7R 不会改变细胞生长。这些实验证明了 Q7R 作为客体结合的直接传感器以及用于成像应用的细胞通透性化合物的可行性。

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