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首页> 外文期刊>Journal of Microscopy >Using conventional fluorescent markers for far-field fluorescence localization nanoscopy allows resolution in the 10-nm range.
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Using conventional fluorescent markers for far-field fluorescence localization nanoscopy allows resolution in the 10-nm range.

机译:使用常规的荧光标记物进行远场荧光定位纳米检查可实现10 nm范围内的分辨率。

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We present a novel technique of far-field localization nanoscopy combining spectral precision distance microscopy with widely used fluorochromes like the Green Fluorescent Protein (GFP) derivatives eGFP, EmGFP, Yellow Fluorescent Protein (YFP) and eYFP, synthetic dyes like Alexa 488 and Alexa 568, as well as fluoresceine derivates. Spectral precision distance microscopy allows the surpassing of conventional resolution limits in fluorescence far-field microscopy by precise object localization after the optical isolation of single signals in time. Based on the principles of this technique, our novel nanoscopic method was realized for laser optical precision localization and image reconstruction with highly enhanced optical resolution in intact cells. This allows for spatial assignment of individual fluorescent molecules with nanometre precision. The technique is based on excitation intensity dependent reversible photobleaching of the molecules used combined with fast time sequential imaging under appropriate focusing conditions. A meaningful advantage of the technique is the simple applicability as a universal tool for imaging and investigations to the major part of already available preparations according to standard protocols. Using the above mentioned fluorophores, the positions of single molecules within cellular structures were determined by visible light with an estimated localization precision down to 3 nm; hence distances in the range of 10-30 nm were resolved between individual fluorescent molecules allowing to apply different quantitative structure analysis tools.
机译:我们提出了一种新的远场定位纳米技术,结合了光谱精确距离显微镜技术和广泛使用的荧光染料,例如绿色荧光蛋白(GFP)衍生物eGFP,EmGFP,黄色荧光蛋白(YFP)和eYFP,合成染料如Alexa 488和Alexa 568以及荧光素衍生物。光谱精密距离显微镜通过在对单个信号进行光学隔离后进行精确的对象定位,可以超越荧光远场显微镜中的常规分辨率极限。基于此技术的原理,我们实现了新颖的纳米方法,可用于激光光学精确定位和图像重建,并在完整细胞中大大提高了光学分辨率。这允许以纳米精度对各个荧光分子进行空间分配。该技术基于与激发强度有关的分子可逆光漂白,结合适当的聚焦条件下的快速时间顺序成像。该技术的一个有意义的优点是,它可以简单地用作通用工具,用于按照标准方案对已经可用的制剂的主要部分进行成像和研究。使用上述荧光团,细胞结构内单分子的位置由可见光确定,估计的定位精度低至3 nm。因此,可以解析各个荧光分子之间10-30 nm范围内的距离,从而可以应用不同的定量结构分析工具。

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