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Literature DB >> 22082987

Measuring and interpreting point spread functions to determine confocal microscope resolution and ensure quality control.

Richard W Cole¹, Tushare Jinadasa, Claire M Brown.

Abstract

This protocol outlines a procedure for collecting and analyzing point spread functions (PSFs). It describes how to prepare fluorescent microsphere samples, set up a confocal microscope to properly collect 3D confocal image data of the microspheres and perform PSF measurements. The analysis of the PSF is used to determine the resolution of the microscope and to identify any problems with the quality of the microscope's images. The PSF geometry is used as an indicator to identify problems with the objective lens, confocal laser scanning components and other relay optics. Identification of possible causes of PSF abnormalities and solutions to improve microscope performance are provided. The microsphere sample preparation requires 2-3 h plus an overnight drying period. The microscope setup requires 2 h (1 h for laser warm up), whereas collecting and analyzing the PSF images require an additional 2-3 h.

Entities: Disease Gene

Mesh：

Year: 2011 PMID： 22082987 DOI： 10.1038/nprot.2011.407

Source DB: PubMed Journal: Nat Protoc ISSN： 1750-2799 Impact factor: 13.491

13 in total

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5. Fluctuation correlation spectroscopy with a laser-scanning microscope: exploiting the hidden time structure.

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Review 6. Quantitative fluorescence microscopy and image deconvolution.

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Review 7. Evaluating optical aberration using fluorescent microspheres: methods, analysis, and corrective actions.

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8. Experimental test of an analytical model of aberration in an oil-immersion objective lens used in three-dimensional light microscopy.

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9. Determination of three-dimensional imaging properties of a light microscope system. Partial confocal behavior in epifluorescence microscopy.

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10. Paxillin dynamics measured during adhesion assembly and disassembly by correlation spectroscopy.

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Journal: Nat Protoc Date: 2015-11-05 Impact factor: 13.491

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Measuring and interpreting point spread functions to determine confocal microscope resolution and ensure quality control.

1. A workingperson's guide to deconvolution in light microscopy.

Review 2. Live cell imaging using wide-field microscopy and deconvolution.

3. Spatial mapping of integrin interactions and dynamics during cell migration by image correlation microscopy.

4. Measuring fast dynamics in solutions and cells with a laser scanning microscope.

5. Fluctuation correlation spectroscopy with a laser-scanning microscope: exploiting the hidden time structure.

Review 6. Quantitative fluorescence microscopy and image deconvolution.

Review 7. Evaluating optical aberration using fluorescent microspheres: methods, analysis, and corrective actions.

8. Experimental test of an analytical model of aberration in an oil-immersion objective lens used in three-dimensional light microscopy.

9. Determination of three-dimensional imaging properties of a light microscope system. Partial confocal behavior in epifluorescence microscopy.

10. Paxillin dynamics measured during adhesion assembly and disassembly by correlation spectroscopy.

1. Imaging fluorescence (cross-) correlation spectroscopy in live cells and organisms.

2. Online correction of licking-induced brain motion during two-photon imaging with a tunable lens.

3. Native serotonin 5-HT2C receptors are expressed as homodimers on the apical surface of choroid plexus epithelial cells.

4. 3D structure tensor analysis of light microscopy data for validating diffusion MRI.

5. Superresolution live imaging of plant cells using structured illumination microscopy.

6. Any Way You Slice It-A Comparison of Confocal Microscopy Techniques.

7. High numerical aperture Fourier ptychography: principle, implementation and characterization.

8. Identification of a multienzyme complex for glucose metabolism in living cells.

9. Unraveling the Thousand Word Picture: An Introduction to Super-Resolution Data Analysis.

10. STED imaging performance estimation by means of Fourier transform analysis.