Abstract
The acknowledged genetic malleability of fission yeast has been matched by impressive cytology to drive major advances in our understanding of basic molecular cell biological processes. In many of the more recent studies, traditional approaches of fixation followed by processing to accommodate classical staining procedures have been superseded by live-cell imaging approaches that monitor the distribution of fusion proteins between a molecule of interest and a fluorescent protein. Although such live-cell imaging is uniquely informative for many questions, fixed-cell imaging remains the better option for others and is an important-sometimes critical-complement to the analysis of fluorescent fusion proteins by live-cell imaging. Here, we discuss the merits of fixed- and live-cell imaging as well as specific issues for fluorescence microscopy imaging of fission yeast.
| Original language | English |
|---|---|
| Pages (from-to) | pdb.top079830 |
| Journal | Cold Spring Harbor Protocols |
| Volume | 2016 |
| Issue number | 7 |
| DOIs | |
| Publication status | Published - 2016 |
Research Beacons, Institutes and Platforms
- Manchester Cancer Research Centre