LZ2 - Zeiss Lightsheet Z.1
From BioDIP
(Difference between revisions)
(creation of page, copy whole page content from LZ1) |
|||
Line 10: | Line 10: | ||
|Institute-logo=Logo MPI-CBG.jpg | |Institute-logo=Logo MPI-CBG.jpg | ||
|description=The lightsheet fluorescence microscopy (also known as SPIM) is a revolutionary development in microscopy. The laser beam illuminates the sample from the side and excites fluorophores along a single line inside of the specimen. A pair of laser scanners moves the excitation laser line vertically and horizontally. An optically sectioned image is recorded by rapidly scanning an entire plane in the specimen and detecting the fluorescence at a right angle to the illumination axis. This technique reduces photobleaching and phototoxic effects in live samples, allowing for long-term imaging in real time in three and four dimensions. | |description=The lightsheet fluorescence microscopy (also known as SPIM) is a revolutionary development in microscopy. The laser beam illuminates the sample from the side and excites fluorophores along a single line inside of the specimen. A pair of laser scanners moves the excitation laser line vertically and horizontally. An optically sectioned image is recorded by rapidly scanning an entire plane in the specimen and detecting the fluorescence at a right angle to the illumination axis. This technique reduces photobleaching and phototoxic effects in live samples, allowing for long-term imaging in real time in three and four dimensions. | ||
− | |applications=Live imaging in 3D and 4D | + | |applications=Live imaging of larger specimen in 3D and 4D<br> |
+ | imaging of larger cleared samples | ||
|image=LZ1 - Zeiss Lightsheet Z.1.jpg | |image=LZ1 - Zeiss Lightsheet Z.1.jpg | ||
|stand-name=Zeiss - LightSheet LZ1 Stand | |stand-name=Zeiss - LightSheet LZ1 Stand | ||
Line 41: | Line 42: | ||
|software=ZEN Imaging Software 2012 (Black edition)<br>LightSheet Z.1 Multiview Processing<br>3D VisArt<br>Deconvolution | |software=ZEN Imaging Software 2012 (Black edition)<br>LightSheet Z.1 Multiview Processing<br>3D VisArt<br>Deconvolution | ||
|incubation=Cage incubator (T+CO2) | |incubation=Cage incubator (T+CO2) | ||
− | |||
}} | }} |
Revision as of 16:46, 3 February 2016
Directions
Booking
https://python-srv1.mpi-cbg.de/lmf-ipf/cgi-bin/index.py
Details
microscope | Zeiss - LightSheet LZ1 Stand, 3D stand, - | ||
objectives |
| ||
illumination | |||
detection | Two sCMOS cameras; pixel size: 6.5 µm | ||
reflectors | Laser blockers: 405/488/561 405/488/561/640 405/488/640 ND4 (RGB) Secondary beam splitters and associated emission filters: | ||
features | The system is equipped with a telescopic lens, which allows to zoom out up to 0.36x, and to zoom in up to 2.5x with any detection lens. | ||
software | ZEN Imaging Software 2012 (Black edition) LightSheet Z.1 Multiview Processing 3D VisArt Deconvolution"ZEN Imaging Software 2012 (Black edition)<br />LightSheet Z.1 Multiview Processing<br />3D VisArt<br />Deconvolution" cannot be used as a page name in this wiki. | ||
incubation | Cage incubator (T+CO2) | ||
links |
| ||
inv.nr. |