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Studying biological tissue with fluorescence lifetime imaging: microscopy, endoscopy, and complex decay profiles

机译:使用荧光寿命成像研究生物组织:显微镜,内窥镜和复杂的衰变曲线

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We have applied fluorescence lifetime imaging (FLIM) to the autolluorescence of different kinds of biological tissue in vitro, including animal tissue sections and knee joints as well as human teeth, obtaining two-dimensional maps with functional contrast. We find that fluorescence decay profiles of biological tissue are well described by the stretched exponential function (StrEF), which can represent the complex nature of tissue. The StrEF yields a continuous distribution of fluorescence lifetimes, which can be extracted with an inverse Laplace transformation, and additional information is provided by the width of the distribution. Our experimental results from FLIM microscopy in combination with the StrEF analysis indicate that this technique is ready for clinical deployment, including portability that is through the use of a compact picosecond diode laser as the excitation source. The results obtained with our FLIM endoscope successfully demonstrated the viability of this modality, though they need further optimization. We expect a custom-designed endoscope with optimized illumination and detection efficiencies to provide significantly improved performance. (C) 2003 Optical Society of America. [References: 28]
机译:我们已经将荧光寿命成像(FLIM)应用于体外各种生物组织的自发荧光,包括动物组织切片和膝关节以及人的牙齿,从而获得具有功能对比的二维图。我们发现,生物组织的荧光衰减谱很好地描述了拉伸指数函数(StrEF),它可以代表组织的复杂性质。 StrEF产生荧光寿命的连续分布,可以通过逆拉普拉斯变换将其提取出来,并且通过分布的宽度可以提供其他信息。我们从FLIM显微镜得到的实验结果与StrEF分析相结合,表明该技术已为临床部署做好了准备,包括通过使用紧凑型皮秒二极管激光器作为激发源的便携性。尽管我们需要进一步优化,但使用我们的FLIM内窥镜获得的结果成功证明了这种方法的可行性。我们期望具有优化的照明和检测效率的定制设计内窥镜能够显着改善性能。 (C)2003年美国眼镜学会。 [参考:28]

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