首页> 外文会议>Conference on Multiphoton Microscopy in the Biomedical Sciences Ⅱ Jan 20-22, 2002 San Jose, USA >Combined Two-Photon Excited Fluorescence and Second-Harmonic Generation Backscattering Microscopy of Turbid Tissues
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Combined Two-Photon Excited Fluorescence and Second-Harmonic Generation Backscattering Microscopy of Turbid Tissues

机译:混浊组织的组合双光子激发荧光和二次谐波产生反向散射显微镜。

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摘要

A broad range of excitation wavelengths (730-880nm) was used to demonstrate the co-registration of two-photon excited fluorescence (TPEF) and second-harmonic generation (SHG) in unstained turbid tissues in reflection geometry. The composite TPEF/SHG microscopic technique was applied to imaging an organotypic tissue model (RAFT). The origin of the image-forming signal from the various RAFT constituents was determined by spectral measurements. It was shown that at shorter excitation wavelengths the signal emitted from the extracellular matrix (ECM) is a combination of SHG and TPEF from collagen, whereas at longer excitation wavelengths the ECM signal is exclusively due to SHG. The cellular signal is due to TPEF at all excitation wavelengths. The reflected SHG intensity followed a quadratic dependence on the excitation power and exhibited a spectral dependence in accordance with previous theoretical studies. Understanding the structural origin of signal provided a stratagem for enhancing contrast between cellular structures, and components of the extracellular matrix. The use of SHG and TPEF in combination provides complementary information that allows non-invasive, spatially localized in vivo characterization of cell-ECM interactions and pathology.
机译:宽范围的激发波长(730-880nm)用于证明在反射几何学中未染色的混浊组织中双光子激发荧光(TPEF)和二次谐波产生(SHG)的共配准。 TPEF / SHG复合显微镜技术已应用于对器官型组织模型(RAFT)进行成像。来自各种RAFT成分的成像信号的起源是通过光谱测量确定的。结果表明,在较短的激发波长下,细胞外基质(ECM)发出的信号是胶原蛋白的SHG和TPEF的组合,而在较长的激发波长下,ECM信号完全是由SHG引起的。蜂窝信号归因于所有激发波长下的TPEF。根据先前的理论研究,反射的SHG强度遵循对激发功率的二次依赖性,并表现出光谱依赖性。理解信号的结构起源为增强细胞结构与细胞外基质成分之间的对比提供了策略。 SHG和TPEF的组合使用可提供互补信息,从而可以对细胞ECM相互作用和病理学进行无创,空间定位的体内表征。

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