首页> 外文会议>Conference on Multiphoton Microscopy in the Biomedical Sciences; 20080120-22; San Jose,CA(US) >Determination of two-photon excitation and emission spectra of fluorescent molecules in single living cells
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Determination of two-photon excitation and emission spectra of fluorescent molecules in single living cells

机译:单个活细胞中荧光分子的双光子激发和发射光谱的测定

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Modelocked Ti:Sapphire lasers are widely used in two-photon microscopes (TPM), partly due to their tunability over a broad range of wavelengths (between 700 nm and 1000 nm). Many biophysical applications, including quantitative Forster Resonance Energy Transfer (FRET) and photoswitching of fluorescent proteins between dark and bright states, require wavelength tuning without optical realignment, which is not easily done in tunable Ti:Sapphire lasers. In addition, for studies of dynamics in biological systems the time required for tuning the excitation should be commensurate with the shortest of the time scales of the processes investigated. A set-up in which a modelocked Ti:Sapphire oscillator providing broad-bandwidth (i.e., short) pulses with fixed center wavelength is coupled to a pulse shaper incorporating a spatial light modulator placed at the Fourier plane of a zero-dispersion two-grating setup, represents a faster alternative to the tunable laser. A pulse shaping system and a TPM with spectral resolution allowed us to acquire two-photon excitation and emission spectra of fluorescent molecules in single living cells. Such spectra may be exploited for mapping intracellular pH and for quantitative studies of protein localization and interactions in vivo.
机译:Modelocked Ti:Sapphire激光器被广泛用于双光子显微镜(TPM),部分是由于它们在很宽的波长范围(700 nm至1000 nm)中具有可调性。许多生物物理应用,包括定量的Forster共振能量转移(FRET)和在暗态和亮态之间荧光蛋白的光开关,都需要波长调整而不进行光学调整,这在可调谐的Ti:Sapphire激光器中不容易做到。另外,为了研究生物系统中的动力学,调节激发所需的时间应与所研究过程中最短的时间尺度相称。一种装置,其中提供具有固定中心波长的宽带(即短)脉冲的锁模Ti:蓝宝石振荡器耦合到脉冲整形器,该脉冲整形器在零色散两光栅的傅立叶平面上结合了空间光调制器设置代表了可调谐激光器的更快替代方案。脉冲整形系统和具有光谱分辨率的TPM允许我们获取单个活细胞中荧光分子的双光子激发和发射光谱。可以利用这种光谱来绘制细胞内pH,并用于体内蛋白质定位和相互作用的定量研究。

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