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Pulse-Shaping-Based Nonlinear Microscopy: Development and Applications.

机译:基于脉冲整形的非线性显微镜:开发与应用。

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摘要

The combination of optical microscopy and ultrafast spectroscopy make the spatial characterization of chemical kinetics on the femtosecond time scale possible. Commercially available octave-spanning Ti:Sapphire oscillators with sub-8 fs pulse durations can drive a multitude of nonlinear transitions across a significant portion of the visible spectrum with minimal average power. Unfortunately, dispersion from microscope objectives broadens pulse durations, decreases temporal resolution and lowers the peak intensities required for driving nonlinear transitions. In this dissertation, pulse shaping is used to compress laser pulses after the microscope objective. By using a binary genetic algorithm, pulse-shapes are designed to enable selective two-photon excitation. The pulse-shapes are demonstrated in two-photon fluorescence of live COS-7 cells expressing GFP-variants mAmetrine and tdTomato. The pulse-shaping approach is applied to a new multiphoton fluorescence resonance energy transfer (FRET) stoichiometry method that quantifies donor and acceptor molecules in complex, as well as the ratio of total donor to acceptor molecules. Compared to conventional multi-photon imaging techniques that require laser tuning or multiple laser systems to selectively excite individual fluorophores, the pulse-shaping approach offers rapid selective multifluorphore imaging at biologically relevant time scales. By splitting the laser beam into two beams and building a second pulse shaper, a pulse-shaping-based pump-probe microscope is developed. The technique offers multiple imaging modalities, such as excited state absorption (ESA), ground state bleach (GSB), and stimulated emission (SE), enhancing contrast of structures via their unique quantum pathways without the addition of contrast agents. Pulse-shaping based pump-probe microscopy is demonstrated for endogenous chemical-contrast imaging of red blood cells.In the second section of this dissertation, ultrafast spectroscopic techniques are used to characterize structure-function relationships of two-photon absorbing GFP-type probes and optical limiting materials. Fluorescence lifetimes of GFP-type probes are shown to depend on functional group substitution position, therefore, enabling the synthesis of designer probes for the possible study of conformation changes and aggregation in biological systems. Similarly, it is determined that small differences in the structure and dimensionality of organometallic macrocycles result in a diverse set of optical properties, which serves as a basis for the molecular level design of nonlinear optical materials.
机译:光学显微镜和超快速光谱学的结合使飞秒时间尺度上化学动力学的空间表征成为可能。低于8 fs脉冲持续时间的商用倍频跨度的Ti:Sapphire振荡器可以以最小的平均功率驱动可见光谱中很大一部分的大量非线性跃迁。不幸的是,来自显微镜物镜的色散会加宽脉冲持续时间,降低时间分辨率,并降低驱动非线性跃迁所需的峰值强度。本文采用脉冲整形技术对显微镜物镜后的激光脉冲进行压缩。通过使用二进制遗传算法,设计了脉冲形状以实现选择性的双光子激发。在表达GFP变体mAmetrine和tdTomato的活COS-7细胞的两光子荧光中证实了脉冲形状。脉冲整形方法已应用于一种新的多光子荧光共振能量转移(FRET)化学计量方法,该方法可定量分析复合物中的供体和受体分子,以及总供体与受体分子的比例。与需要激光调谐或多个激光系统以选择性激发单个荧光团的常规多光子成像技术相比,脉冲整形方法可在生物学相关的时标上提供快速的选择性多荧光团成像。通过将激光束分成两束并构建第二个脉冲整形器,开发了基于脉冲整形的泵浦探针显微镜。该技术提供了多种成像方式,例如激发态吸收(ESA),基态漂白剂(GSB)和受激发射(SE),可通过其独特的量子途径增强结构的对比度,而无需添加造影剂。基于脉冲整形的泵浦探针显微镜被证明用于红细胞的内源性化学对比成像。在本文的第二部分,超快光谱技术用于表征双光子吸收GFP型探针的结构-功能关系和光学限制材料。 GFP型探针的荧光寿命显示取决于官能团的取代位置,因此,可以合成设计探针以用于研究生物系统中的构象变化和聚集。同样,可以确定,有机金属大环的结构和尺寸上的微小差异会导致形成多种多样的光学性质,这是非线性光学材料分子水平设计的基础。

著录项

  • 作者

    Flynn Daniel Christopher;

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  • 年度 2014
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  • 原文格式 PDF
  • 正文语种 en_US
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