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Efficient real-time confocal microscopy with white light sources
R Juskaitis, T Wilson, MA Neil, M Kozubek
Language English Country Great Britain
Document type Research Support, Non-U.S. Gov't
Grant support
IZ2636
MZ0
CEP Register
Digital library NLK
Full text - Article
Source
NLK
ProQuest Central
from 1990-01-04 to 1 year ago
Nursing & Allied Health Database (ProQuest)
from 1990-01-04 to 1 year ago
Health & Medicine (ProQuest)
from 1990-01-04 to 1 year ago
Psychology Database (ProQuest)
from 1990-01-04 to 1 year ago
Public Health Database (ProQuest)
from 1990-01-04 to 1 year ago
PubMed
8893003
Knihovny.cz E-resources
- MeSH
- Microscopy, Confocal * instrumentation MeSH
- Mice MeSH
- Osteoclasts cytology MeSH
- Light MeSH
- Thalamus anatomy & histology MeSH
- Whales MeSH
- Animals MeSH
- Check Tag
- Mice MeSH
- Animals MeSH
- Publication type
- Research Support, Non-U.S. Gov't MeSH
The main advantage of confocal microscopes over their conventional counterparts arises from their ability to optically 'section' nearly transparent materials; the thin image slices thus obtained can be used to reconstruct three-dimensional images, a capability which is particularly useful for the study of biological specimens. Confocal microscopes have previously used either a single laser-illuminated point-source and single point-detector (which are scanned in tandem across the object) or white-light illumination with multiple point-sources and detectors. Single-point-source systems, however, do not usually form images in real time and are restricted to using available laser wavelengths. Multiple-point-source systems, on the other hand, produce images in real time but use light very inefficiently--typically 1% or less is used for imaging. Here we demonstrate a white-light, multiple-point-source method which can in principle produce images in real time with light efficiencies as high as 50%. This system is likely to find broad practical application, particularly in the imaging of weakly reflecting or weakly fluorescent specimens.
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- $a The main advantage of confocal microscopes over their conventional counterparts arises from their ability to optically 'section' nearly transparent materials; the thin image slices thus obtained can be used to reconstruct three-dimensional images, a capability which is particularly useful for the study of biological specimens. Confocal microscopes have previously used either a single laser-illuminated point-source and single point-detector (which are scanned in tandem across the object) or white-light illumination with multiple point-sources and detectors. Single-point-source systems, however, do not usually form images in real time and are restricted to using available laser wavelengths. Multiple-point-source systems, on the other hand, produce images in real time but use light very inefficiently--typically 1% or less is used for imaging. Here we demonstrate a white-light, multiple-point-source method which can in principle produce images in real time with light efficiencies as high as 50%. This system is likely to find broad practical application, particularly in the imaging of weakly reflecting or weakly fluorescent specimens.
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