Single‐cell analysis of yeast, mammalian cells, and fungal spores with a microfluidic pressure‐driven chip‐based system
- 17 May 2004
- journal article
- Published by Wiley in Cytometry Part A
- Vol. 59A (2) , 246-253
- https://doi.org/10.1002/cyto.a.20049
Abstract
Background Cytomics aims at understanding the function of cellular systems by analysis of single cells. Recently, there has been a growing interest in single cell measurements being performed in microfluidic systems. These systems promise to integrate staining, measurement, and analysis in a single system. One important aspect is the limitation of allowable cell sizes due to microfluidic channel dimensions. Here we want to demonstrate the broad applicability of microfluidic chip technology for the analysis of many different cell types. Methods We have developed a microfluidic chip and measurement system that allows flow cytometric analysis of fluorescently stained cells from different organisms. In this setup, the cells are moved by pressure‐driven flow inside a network of microfluidic channels and are analyzed individually by fluorescence detection. Results We have successfully applied the system to develop a methodology to detect viable and dead cells in yeast cell populations. Also, we have measured short interfering RNA (siRNA) mediated silencing of protein expression in mammalian cells. In addition, we have characterized the infection state of Magnaportae grisea fungal spores. Conclusions Results obtained with the microfluidic system demonstrate a broad applicability of microfluidic flow cytometry to measurement of various cell types.Keywords
Funding Information
- Grant Agency of the Czech Republic (204/02/0650)
- Ministry of Education, Youth, and Sport (LA141)
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