Second harmonic imaging microscopy

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Second harmonic imaging microscopy (SHIM) is based on a nonlinear optical effect known as second harmonic generation (SHG). SHIM has been established as a viable microscope imaging contrast mechanism for visualization of cell and tissue structure and function. A second harmonic microscope obtains contrasts from variations in a specimen’s ability to generate second harmonic light from the incident light while a conventional optical microscope obtains its contrast by detecting variations in optical density, path length, or refractive index of the specimen. SHG requires intense laser light passing through a material with a noncentrosymmetric molecular structure. Second-harmonic light emerging from an SHG material is exactly half the wavelength (frequency doubled) of the light entering the material. While two-photon-excited fluorescence (TPEF) is also a two photon process, TPEF loses some energy during the relaxation of the excited state, and SHG is energy conserving. Typically, an inorganic crystal is used to produce SHG light such as lithium niobate (LiNbO3), potassium titanyl phosphate (KTP = KTiOPO4), and lithium triborate (LBO = LiB3O5). Though SHG requires a material to have specific molecular orientation in order for the incident light to be frequency doubled, some biological materials can be highly polarizable, and assemble into fairly ordered, large noncentrosymmetric structures. Biological materials such as collagen, microtubules, and muscle myosin can produce SHG signals. The SHG pattern is mainly determined by the phase matching condition. A common setup for an SHG imaging system will have a laser scanning microscope with a titanium sapphire mode-locked laser as the excitation source. The SHG signal is propagated in the forward direction. However, some experiments have shown that objects on the order of about a tenth of the wavelength of the SHG produced signal will produce nearly equal forward and backward signals.

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[edit] Advantages

SHIM offers several advantages for live cell and tissue imaging. SHG doesn’t involve the excitation of molecules like other techniques such as fluorescence microscopy therefore, the molecules shouldn’t suffer the effects of phototoxicity or photobleaching. Also, since many biological structures produce strong SHG signals, the labeling of molecules with exogenous probes is not required which can also alter the way a biological system functions. By using near infrared wavelengths for the incident light, SHIM has the ability to construct three dimensional images of specimens by imaging deeper into thick tissues.

[edit] History

Before SHG was used for imaging, the first demonstration of SHG was done in 1962 by Kleinman on crystalline quartz. This then, SHG producing crystals have been used to frequency double lasers to obtain shorter wavelengths. In 1968, SHG from interfaces was discovered by Bloembergen and has since been used as a tool for characterizing surfaces and probing interface dynamics. In 1974, Hellwarth and Christensen first reported the integration of SHG and microscopy by imaging SHG signals from polycrystalline ZnSe. In 1977, Sheppard imaged various SHG crystals with a scanning optical microscope. The first biological imaging experiments were done by Freund in 1986 to study the orientation of collagen fibers in rat tail tendon. In 1993, Lewis examined the second harmonic response of styryl dyes in electric fields. He also showed worked on imaging live cells.

[edit] Applications

SHG polarization anisotropy can be used to determine the orientation and degree of organization of proteins in tissues since SHG signals have well-defined polarizations. By using the anisotropy equation:

\frac{I_{par}-I_{perp}}{I_{par}+2I_{perp}}=r

and acquiring the intensities of the polarizations in the parallel and perpendicular directions. A high r value indicates an anisotropic orientation where as a low r value indicates an isotropic structure. In work done by Campagnola and Loew, it was found that collagen fibers formed well-aligned structures with an r = 0.7 value.

It has also been used to prove that backpropagating action potentials invade dendritic spines without voltage attenuation, establishing a sound basis for future work on Long-term potentiation. Its use here was that it provided a way to accuratly measure the voltage in the tiny dendritic spines with an accuracy unattainable with standard two-photon microscopy.[1]

[edit] Sources

  • P. J. Campagnola, H.A. Clark, W.A. Mohler, A. Lewis and L.M. Loew, “Second-harmonic Imaging Microscopy of Living Cells,“ J. Biomed. Opt. 6, 277-286 (2001)
  • P. J. Campagnola, H.A. Clark, W.A. Mohler, A. Lewis and L.M. Loew, “Second-harmonic imaging microscopy for visualizing biomolecular arrays in cells, tissues and organisms,“ Nature Biotech. 21, 1356-1360 (2003)
  • P. Stoller, K.M. Reiser, P.M. Celliers, & A.M. Rubenchik, “Polarization-modulated second harmonic generation in collagen.” Biophys. J. 82, 3330-3342 (2002)
  • M. Han, G. Giese, and J. F. Bille, “Second harmonic generation imaging of collagen fibrils in cornea and sclera,” Opt. Express 13, 5791-5797 (2005)
  1. ^ Mutsuo Nuriya, Jiang Jiang, Boaz Nemet et al, Imaging Membrane Potential in Dendritic Spines, PNAS, 2005