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SYTO 82 is a cell-permeant, non-exclusive nucleic acid stain that shows a large fluorescence enhancement upon binding. In both live and dead eukaryotic cells, SYTO 82 generally shows cytoplasmic or mitochondrial as well as nuclear staining. In addition, SYTO 82 will stain most live and permeabilized bacteria.
1. Culture cells in an appropriate medium and vessel for fluorescence microscopy. |
2. Remove the medium. |
3. Wash the cells 1–3 times in a phosphate-free buffer to remove the medium. |
4. Prepare the SYTO 82 staining solution by diluting the stock solution 1:1,000 (5 µM) in a phosphate-free buffer. |
5. Add sufficient staining solution to cover the cells. |
6. Incubate for 5–30 minutes, protected from light. |
7. Remove the staining solution. |
8. Wash sample 3 times in a phosphate-free buffer. |
9. Image the cells. |
SYTO 82 | |
---|---|
Excitation/Emission (nm) | 541/560 |
Standard filter set | TRITC |
EVOS Light Cube | RFP |
Storage conditions | ≤–20°C |
Cells stained with SYTO 82 dye and imaged with the Thermo Scientific CellInsight High-Content System.