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Application of the stretched exponential function to fluorescence lifetime imaging of biological tissue

机译:拉伸指数函数在生物组织荧光寿命成像中的应用

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The fluorescence decay in fluorescence lifetime imaging (FLIM) is typically fitted to a multi-exponential model with discrete lifetimes. The interaction between fluorophores in heterogeneous samples (e.g. biological tissue) can, however, produce complex decay characteristics that do not correspond to such models. Although they appear to provide a better fit to fluorescence decay data than the assumption of a mono-exponential decay, the assumption of multiple discrete components is essentially arbitrary and often erroneous. The stretched exponential function (StrEF) describes fluorescence decay profiles using a continuous lifetime distribution as has been reported for tryptophan, being one of the main fluorophores in tissue. We have demonstrated that this model represents our time-domain FLIM data better than multi-exponential discrete decay components, yielding excellent contrast in tissue discrimination without compromising the goodness of fit, and it significantly decreases the required processing time. The addition, the stretched exponential decay model can provide a direct measure of the sample heterogeneity and the resulting heterogeneity map can reveal subtle tissue differences that other models fail to show.
机译:在荧光寿命成像(FLIM)的荧光衰减典型地装配到多指数模型具有离散的寿命。异质样品中的荧光团之间的(例如生物组织)的相互作用可以,但是,产生不对应于这样的模型复杂的衰变特性。虽然它们显示,以提供更好的贴合荧光衰减数据比单指数衰减的假设下,多个分立元件的假设基本上是任意的,并且往往是错误的。拉伸指数函数(StrEF)描述了使用连续寿命分布如已被报道用于色氨酸,是在组织中的主要荧光团的一个荧光衰减曲线。我们已经证明,这种模式比多指数的离散衰减成分更好地代表我们的时域FLIM数据,产生于组织的歧视出色的对比度不影响拟合度,并降低显著所需的处理时间。添加,拉伸指数衰减模型可提供样品异质性的直接测量所得的异质性地图可以发现细微差别的组织,其他车型无法显示。

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