首页> 外文期刊>Journal of Biophotonics >Visualising apoptosis in live zebrafish using fluorescence lifetime imaging with optical projection tomography to map FRET biosensor activity in space and time
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Visualising apoptosis in live zebrafish using fluorescence lifetime imaging with optical projection tomography to map FRET biosensor activity in space and time

机译:使用荧光寿命断层成像和光学投影层析成像技术来可视化活斑马鱼的凋亡,以绘制FRET生物传感器的时空分布图

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摘要

Fluorescence lifetime imaging (FLIM) combined with optical projection tomography (OPT) has the potential to map Forster resonant energy transfer (FRET) readouts in space and time in intact transparent or near transparent live organisms such as zebrafish larvae, thereby providing a means to visualise cell signalling processes in their physiological context. Here the first application of FLIM OPT to read out biological function in live transgenic zebrafish larvae using a genetically expressed FRET biosensor is reported. Apoptosis, or programmed cell death, is mapped in 3-D by imaging the activity of a FRET biosensor that is cleaved by Caspase 3, which is a key effector of apoptosis. Although apoptosis is a naturally occurring process during development, it can also be triggered in a variety of ways, including through gamma irradiation. FLIM OPT is shown here to enable apoptosis to be monitored over time, in live zebrafish larvae via changes in Caspase 3 activation following gamma irradiation at 24 hours post fertilisation. Significant apoptosis was observed at 3.5 hours post irradiation, predominantly in the head region.
机译:荧光寿命成像(FLIM)与光学投影层析成像(OPT)结合,可以在完整的透明或接近透明的活生物体(例如斑马鱼幼虫)中绘制时空上的Forster共振能量转移(FRET)读数,从而提供可视化方法细胞在生理环境中的信号传导过程。在这里,首次报道了FLIM OPT使用遗传表达的FRET生物传感器读取活的转基因斑马鱼幼虫的生物学功能的应用。通过成像被凋亡关键因子Caspase 3裂解的FRET生物传感器的活性,可以在3-D中定位凋亡或程序性细胞死亡。尽管细胞凋亡是发育过程中自然发生的过程,但它也可以通过多种方式触发,包括通过伽马射线照射。此处显示的FLIM OPT使活的斑马鱼幼虫能够在受精后24小时接受伽马射线照射后通过Caspase 3激活的变化来监测随时间变化的凋亡。在照射后3.5小时观察到明显的细胞凋亡,主要在头部区域。

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