Polarization characteristic measuring method and apparatus

Optics: measuring and testing – By polarized light examination

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356367, 356369, 250225, 359385, 359386, G01J 400, G02F 101, G02B 2106

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060259175

DESCRIPTION:

BRIEF SUMMARY
TECHNICAL FIELD

This invention relates to a polarization characteristic measuring apparatus and method for measuring a characteristic of polarization of fluorescence or Raman-scattered light appearing when a sample is exposed to light.


BACKGROUND ART

When a sample is exposed to light, light of the same wavelength as that of the illuminating light appears in the form of reflected light and scattered light and, in addition thereto, there are cases where light of wavelengths different from that of the illuminating light is emergent (for example, fluorescence and Raman-scattered light). Useful information about the sample can be obtained by measuring the intensity of this fluorescence or Raman-scattered light, and useful information about the sample can also be obtained by measuring the characteristic of polarization of these beams.
For example, when a sample containing a fluorescent probe is exposed to excitation light and when depolarization of fluorescence emitted from the sample is measured, we can know whether there exists the fluorescent probe bound to a target. More specifically, when the sample containing the fluorescent probe is excited with linearly polarized pulsed light, fluorescence is emitted from the fluorescent probe. The polarization state of the fluorescence is almost linearly polarized at the beginning of exposure to the excitation light; but irregular rotation of the fluorescent probe because of the Brownian motion will disturb the molecular axes of excited fluorescent probe molecules, so that the fluorescence will become gradually depolarized with a lapse of time and a unpolarized state will result finally. The rate of this depolarization of the free fluorescent probe is different from that of the fluorescent probe bound to the target and, therefore, we can know whether the fluorescent probe bound to the target is present, by making use of the difference in the rate of depolarization.
Accordingly, if a two-dimensional image of degrees of this fluorescence depolarization can be measured under a microscope, a location of the fluorescent probe bound to the target can be specified and the behavior or the like of the target in the sample can be analyzed; it is, therefore, expected that this method can contribute to elucidation of various functions in cells, for example. Similarly, it is also expected that useful information concerning the sample can be obtained by measurement of a two-dimensional image of polarization characteristic of the Raman-scattered light under the microscope.
Incidentally, the technique for observing the two-dimensional image of the polarization state of fluorescence is described in D. Axelrod, "Carbocyanine Dye Orientation in Red Cell Membrane studied by Microscopic Fluorescence Polarization," Biophys. J., Vol. 26, pp. 557-574 (1979) and K. Suzuki et al., "Spatiotemporal Relationships Among Early Events of Fertilization in Sea Urchin Eggs Revealed by Multiview Microscopy," Biophys. J., Vol. 68, pp. 739-748 (1995).
The technique described in the paper of D. Axelrod concerns the method for measuring states of polarization of fluorescence generated under irradiation of steady-state light (linearly polarized excitation light), under the microscope and thereby analyzing orientation and mobility of fluorescent dye in a biomembrane. A photodetector used herein is a photomultiplier tube, which obtains a two-dimensional image of fluorescence polarization by scanning the diaphragm on the fluorescent image plane. A problem arising in measuring such fluorescence polarization is measurement errors caused by different responses of the photodetector and the optical system except for the polarizing device to different directions of polarization. In the technique described in this paper, the measurement errors are corrected (polarization response correction) by allowing fairly unpolarized light to pass through a light detecting optical system (an optical system from the sample to the photodetector) and the photodetector.
The technique described in the paper of K. Suzuki concerns the

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patent: 5552889 (1996-09-01), Meier
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Toyonaga et al.; "Detection of Minute Quantities of Substances in Organisms", vol. 26, No. 9, place & date of publication not known.
Axelrod, Daniel; "Carbocyanine Dye Orientation in Red Cell Membrane Studied by Microscopic Fluorescence Polarization", Biophysical Journal, vol. 26, Jun. 1979, pp. 557-573.
Dix et al.; "Mapping of fluorescence anisotrophy in living cells by ratio imaging"; Biophysical Journal, vol. 57, Feb. 1990, pp. 231-241.
Lakowicz et al.; "Time-Resolved Fluorescence.Intensity and Anisotropy Decays of 2,5-Diphenyloxazole by Two-Photon Excitation and Frequency-Domain Fluorometry", Journal of Physical Chemistry, vol. 96, No. 7, 1992, pp. 3000-3006.
Lakowicz et al.; "Anomalous differential polarized phase angles for two-photon excitation with isotropic depolarizing rotations" Chem. Phys. Letters, vol. 191, No. 1,2 Mar. 27, 1992, pp. 47-53.
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Suzuki et al.; "Spatiotemporal Relationships Among Early Events of Fertilization in Sea Urchin Eggs Revealed by Multiview Microscopy", Biophysical Journal, vol. 68, Mar. 1995, pp. 739-748.

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