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数字成像荧光显微镜:单个细胞中光漂白速率常数的空间异质性

Digital imaging fluorescence microscopy: spatial heterogeneity of photobleaching rate constants in individual cells.

作者信息

Benson D M, Bryan J, Plant A L, Gotto A M, Smith L C

出版信息

J Cell Biol. 1985 Apr;100(4):1309-23. doi: 10.1083/jcb.100.4.1309.

Abstract

Photobleaching and related photochemical processes are recognized experimental barriers to quantification of fluorescence by microscopy. We have measured the kinetics of photobleaching of fluorophores in living and fixed cells and in microemulsions, and have demonstrated the spatial variability of these processes within individual cells. An inverted fluorescence microscope and a high-sensitivity camera, together with high-speed data acquisition by a computer-controlled image processor, have been used to control precisely exposure time to excitation light and to record images. To improve the signal-to-noise ratio, 32 digital images were integrated. After correction for spatial variations in camera sensitivity and background fluorescence, the images of the relative fluorescence intensities for 0.065 micron2 areas in the object plane were obtained. To evaluate photobleaching objectively, an algorithm was developed to fit a three-parameter exponential equation to 20 images recorded from the same microscope field as a function of illumination time. The results of this analysis demonstrated that the photobleaching process followed first-order reaction kinetics with rate constants that were spatially heterogeneous and varied, within the same cell, between 2- and 65-fold, depending on the fluorophore. The photobleaching rate constants increased proportionally with increasing excitation intensity and, for benzo(a)pyrene, were independent of probe concentration over three orders of magnitude (1.25 microM to 1.25 mM). The propensity to photobleach was different with each fluorophore. Under the cellular conditions used in these studies, the average rates of photobleaching decreased in this order: N-(7-nitrobenz-2-oxa-1,3-diazole)-23,24-dinor-5-cholen-22-amine-3 beta-ol greater than acridine orange greater than rhodamine-123 greater than benzo(a)pyrene greater than fluorescein greater than tetramethylrhodamine greater than 1,1'dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine. The photobleaching appears to be an oxidation reaction, in that the addition of saturated solutions of Na2S2O5 to mineral oil microemulsions eliminated photobleaching of N-(7-nitrobenz-2-oxa-1,3-diazole)-23,24-dinor-5-cholen-22-amine-3 beta-ol or benzo(a)pyrene. We identified experimental conditions to observe, without detectable photobleaching, fluorophores in living cells, which can not be studied anaerobically. Useful images were obtained when excitation light was reduced to eliminate photobleaching, as determined from zero-time images calculated from the exponential fit routine.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

光漂白及相关光化学过程是通过显微镜对荧光进行定量分析时公认的实验障碍。我们已测量了活细胞、固定细胞以及微乳液中荧光团的光漂白动力学,并证明了这些过程在单个细胞内的空间变异性。使用倒置荧光显微镜、高灵敏度相机以及由计算机控制的图像处理器进行高速数据采集,精确控制激发光的曝光时间并记录图像。为提高信噪比,对32幅数字图像进行了整合。在校正相机灵敏度和背景荧光的空间变化后,获得了物平面中0.065平方微米区域的相对荧光强度图像。为客观评估光漂白,开发了一种算法,将一个三参数指数方程拟合到从同一显微镜视野记录的20幅图像上,作为光照时间的函数。该分析结果表明,光漂白过程遵循一级反应动力学,速率常数在空间上是异质的,在同一细胞内,根据荧光团的不同,其变化幅度在2至65倍之间。光漂白速率常数随激发强度的增加成比例增加,对于苯并(a)芘,在三个数量级(1.25微摩尔至1.25毫摩尔)范围内与探针浓度无关。每种荧光团的光漂白倾向不同。在这些研究中使用的细胞条件下,光漂白的平均速率按以下顺序降低:N-(7-硝基苯并-2-恶唑-1,3-二氮杂萘)-23,24-二降胆甾-22-胺-3β-醇>吖啶橙>罗丹明-123>苯并(a)芘>荧光素>四甲基罗丹明>1,1'-二辛基-3,3,3',3'-四甲基吲哚羰花青。光漂白似乎是一种氧化反应,因为向矿物油微乳液中添加饱和的连二亚硫酸钠溶液可消除N-(7-硝基苯并-2-恶唑-1,3-二氮杂萘)-23,24-二降胆甾-22-胺-3β-醇或苯并(a)芘的光漂白。我们确定了在不可进行厌氧研究的活细胞中观察荧光团而不发生可检测到的光漂白的实验条件。当根据指数拟合程序计算的零时图像确定激发光减少以消除光漂白时,获得了有用的图像。(摘要截短至400字)

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