4.4 Review

Two-photon microscopy: Shedding light on the chemistry of vision

Journal

BIOCHEMISTRY
Volume 46, Issue 34, Pages 9674-9684

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/bi701055g

Keywords

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Funding

  1. NEI NIH HHS [EY014850, R01 EY014850, R01 EY014850-05] Funding Source: Medline
  2. NIDDK NIH HHS [T32 DK007319-30, T32-DK07319, T32 DK007319, U24 DK076174] Funding Source: Medline

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Two-photon microscopy (TPM) has come to occupy a prominent place in modern biological research with its ability to resolve the three-dimensional distribution of molecules deep inside living tissue. TPM can employ two different types of signals, fluorescence and second harmonic generation, to image biological structures with subcellular resolution. Two-photon excited fluorescence imaging is a powerful technique with which to monitor the dynamic behavior of the chemical components of tissues, whereas second harmonic imaging provides novel ways to study their spatial organization. Using TPM, great strides have been made toward understanding the metabolism, structure, signal transduction, and signal transmission in the eye. These include the characterization of the spatial distribution, transport, and metabolism of the endogenous retinoids, molecules essential for the detection of light, as well as the elucidation of the architecture of the living cornea. In this review, we present and discuss the current applications of TPM for the chemical and structural imaging of the eye. In addition, we address what we see as the future potential of TPM for eye research. This relatively new method of microscopy has been the subject of numerous technical improvements in terms of the optics and indicators used, improvements that should lead to more detailed biochemical characterizations of the eyes of live animals and even to imaging of the human eye in vivo.

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