Background Rejection in Two-Photon Fluorescence Image Scanning Microscopy

Background Rejection in Two-Photon Fluorescence Image Scanning Microscopy

We discuss the properties of signal strength and integrated intensity in two-photon excitation confocal microscopy and image scanning microscopy. The resolution, optical sectioning and background rejection are all improved over nonconfocal two-photon microscopy. Replacing the pinhole of confocal two...

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Veröffentlicht in:Photonics 2023-05, Vol.10 (5), p.601
Hauptverfasser: Sheppard, Colin J. R., Castello, Marco, Tortarolo, Giorgio, Zunino, Alessandro, Slenders, Eli, Bianchini, Paolo, Vicidomini, Giuseppe, Diaspro, Alberto
Format: Artikel
Sprache:eng
Schlagworte:
Approximation
Arrays
Confocal microscopy
Detectors
Fluorescence
Fluorescence microscopy
image scanning microscopy
Ions
Microscopy
Optical sectioning
Photons
Pinholes
Point spread functions
Rejection
Scanning microscopy
Sectioning
Sensors
Signal strength
two-photon microscopy
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Beschreibung
Zusammenfassung:We discuss the properties of signal strength and integrated intensity in two-photon excitation confocal microscopy and image scanning microscopy. The resolution, optical sectioning and background rejection are all improved over nonconfocal two-photon microscopy. Replacing the pinhole of confocal two-photon microscopy with a detector array increases the peak intensity of the point spread function. The outer pixels of a detector array give signals from defocused regions, and thus the processing of these, such as through subtraction, can further improve optical sectioning and background rejection.
ISSN:2304-6732
2304-6732
DOI:10.3390/photonics10050601