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Influence of optical properties on two-photon fluorescence imaging in turbid samples

机译:光学性质对混浊样品中双光子荧光成像的影响

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摘要

A numerical model was developed to simulate the effects of tissue optical properties, objective numerical aperture (N.A.), and instrument performance on two-photon-excited fluorescence imaging of turbid samples. Model data are compared with measurements of fluorescent microspheres in a tissuelike scattering phantom. Our results show that the measured two-photon-excited signal decays exponentially with increasing focal depth. The overall decay constant is a function of absorption and scattering parameters at both excitation and emission wavelengths. The generation of two-photon fluorescence is shown to be independent of the scattering anisotropy, g, except for g>0.95. The N.A. for which the maximum signal is collected varies with depth, although this effect is not seen until the focal plane is greater than two scattering mean free paths into the sample. Overall, measurements and model results indicate that resolution in two-photon microscopy is dependent solely on the ability to deliver sufficient ballistic photon density to the focal volume. As a result we show that lateral resolution in two-photon microscopy is largely unaffected by tissue optical properties in the range typically encountered in soft tissues, although the, maximum imaging depth is strongly dependent on absorption and scattering coefficients, scattering anisotropy, and objective N.A..
机译:建立了一个数值模型来模拟组织光学特性,客观数值孔径(N.A.)和仪器性能对混浊样品的双光子激发荧光成像的影响。将模型数据与组织状散射体模中荧光微球的测量值进行比较。我们的结果表明,所测量的两光子激发信号随着焦深的增加呈指数衰减。总衰减常数是激发和发射波长下吸收和散射参数的函数。除g> 0.95外,双光子荧光的产生与散射各向异性g无关。收集最大信号的N.A.随深度而变化,尽管直到焦平面大于进入样品的两个散射平均自由程才看到这种效果。总体而言,测量和模型结果表明,双光子显微镜的分辨率仅取决于将足够的弹道光子密度传递给焦点体积的能力。结果表明,尽管最大成像深度强烈取决于吸收和散射系数,散射各向异性和物镜,但在软组织中通常遇到的范围内,双光子显微镜的横向分辨率在很大程度上不受组织光学特性的影响。 。

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