Short Description
The Cell IQ V2 MLF Cell Imaging and Analysis System is a live cell imaging system with integrated platform for quantitative image analysis. To this end, 'machine vision technology' is used, in particular to enable automatic pattern recognition, morphometry and quantification.
The automated microscopy has motorized positioning of the object plane and x y and z direction, thus allowing 3D photogrammetric image recording over time. Microscopic observation with different lighting modes such as bright field, phase contrast and three fluorescence conditions are possible.
Due to the temperature control and atmospheric conditioning of the measuring chamber, living cells can be analyzed for arbitrarily long periods of time.
Two microtiter plates can be cultivated simultaneously under different gas conditions. The platform includes the analysis software Imagen ™ system control for image processing, automatic stitching and simple conversion of individual image files into high definition videos.
The physiology of the cells can be compared in the high throughput format (48-, 96-plate format) and presented as video in the form of phase contrast or fluorescence (3 channels). The analysis of certain standard assays (scratch assays, cell migration, etc.) is integrated into the software.
Contact Person
Prof. Dr. Günter Lepperdinger
Research Services
Life cell imaging
Cell-based assays
Toxicology
Drug-Testing
Assay Development
Methods & Expertise for Research Infrastructure
The Cell-IQ allows the continuous microscopic recording of cultivated cells over several days offering means for "long-term imaging" or "cell monitoring".
The device additionally allows the quantification of proliferating, apoptotic, and necrotic cells in these cultures without the need of additional markers (label-free), which avoids possible influencing of the cells by the labeling substance itself.
The physiology of the cells can be compared in the high throughput format (48-, 96-plate format) and presented as video in the form of phase contrast or fluorescence (3 channels) images. The analysis of certain standard assays (scratch assays, cell migration, etc.) is included and can be processed by the software.
Allocation to research infrastructure
Mario Gimona, PMU Salzburg
Frank Edenhofer, Universität Innsbruck
Claudio Franceschi, Universität Bologna
Werner Balika, Sony DADC Biosciences
Johannes Grillari, BOKU Wien
Francisco Domingues, EURAC Bozen
Regina Brunauer, BUCK Institute USA
STRATEC Consumables Anif Austria
TECAN Grödig Austria
Molecular Devices, Wals Austria
Eurolyser, Salzburg Austria
Profactor, Steyr, Austria
Fachbereich Molekulare Biologie, Universität Salzburg
Schwerpunkt ACBN, Universität Salzburg
1/01/20 - 31/08/22
Lepperdinger G.
ChinaBone
https://uni-salzburg.elsevierpure.com/de/projects/chinabone
Regulation of cutaneous tissue-repair by a specialized population of CD4+ T cells
2017 - 2022
Iris K. Gratz & Daniel J. Campbell
Fördergeber National Institute of Health / Partner Daniel J. Campbell - Benaroya Research Institute Seattle, WA, USA
https://www.plus.ac.at/biosciences/the-department/research-groups/gratz/projects/?lang=en
2021
Marozin S, Simon-Nobbe B, Irausek S, Chung LWK, Lepperdinger G.
Scientific Reports.
https://pubmed.ncbi.nlm.nih.gov/34035368/
doi: 10.1038/s41598-021-90161-2.