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Near-infrared luminescent metallacrowns for combined in vitro cell fixation and counter staining

机译:近红外发光金属漆用于体外细胞固定和反染

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摘要

Cell fixation is an essential approach for preserving cell morphology, allowing the targeting and labelling of biomolecules with fluorescent probes. One of the key requirements for more efficient fluorescent labelling is the preservation of cell morphology, which usually requires a combination of several fixation techniques. In addition, the use of a counter stain is often essential to improve the contrast of the fluorescent probes. Current agents possess significant limitations, such as low resistance toward photobleaching and sensitivity to changes in the microenvironment. Luminescent Ln3+ ‘encapsulated sandwich’ metallacrowns (MCs) overcome these drawbacks and offer complementary advantages. In particular, they emit sharp emission bands, possess a large difference between excitation and emission wavelengths and do not photobleach. Herein, MCs formed with pyrazinehydroxamic acid (Ln3+[Zn(ii)MCpyzHA], Ln3+ = Yb, Nd) were used, combined with near-infrared (NIR) counter staining and fixation agents for HeLa cells upon an initial five minute exposure to UV-A light. The validity and quality of the cell fixation were assessed with Raman spectroscopy. Analysis of the NIR luminescence properties of these MCs was performed under different experimental conditions, including in a suspension of stained cells. Moreover, the high emission intensity of Ln3+[Zn(ii)MCpyzHA] in the NIR region allows these MCs to be used for imaging with standard CCD cameras installed on routine fluorescence microscopes. Finally, the NIR-emitting Ln3+[Zn(ii)MCpyzHA] compounds combine, within a single molecule, features such as cell fixation and staining abilities, good photostability and minimal sensitivity of the emission bands to the local microenvironment, and they are highly promising for establishing the next generation of imaging agents with a single biodistribution.
机译:细胞固定是保存细胞形态的一种必不可少的方法,可以用荧光探针靶向和标记生物分子。高效荧光标记的关键要求之一是保持细胞形态,这通常需要结合多种固定技术。另外,通常需要使用抗染剂来改善荧光探针的对比度。当前的试剂具有显着的局限性,例如对光漂白的低抗性和对微环境变化的敏感性。发光的Ln 3 + “封装三明治”金属漆克服了这些缺点,并提供了互补的优势。特别地,它们发射出尖锐的发射带,在激发和发射波长之间具有很大的差异,并且不会光漂白。在此,使用由吡嗪异羟肟酸(Ln 3 + [Zn(ii)MCpyzHA],Ln 3 + = Yb,Nd)形成的MC,并与近红外( NIR)在最初暴露于UV-A光5分钟后对HeLa细胞的抗染色和固定剂。用拉曼光谱法评估细胞固定的有效性和质量。这些MC的NIR发光特性的分析是在不同的实验条件下进行的,包括在染色细胞的悬浮液中进行。此外,NIR区域中Ln 3 + [Zn(ii)MCpyzHA]的高发射强度使这些MC可用于安装在常规荧光显微镜上的标准CCD相机进行成像。最后,发射NIR的Ln 3 + [Zn(ii)MCpyzHA]化合物在单个分子中结合,具有细胞固定和染色能力,良好的光稳定性和发射带对光的最小敏感性等特征。它们是当地的微环境,对于建立具有单一生物分布的下一代显像剂非常有希望。

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