Loading for native or denaturing agarose- and polyacrylamide gels
HighRange RNA-Ladder has to be mixed with Loading buffer 2X before use (use the same amount of RNA relating to 1 µg of loaded marker)

- Thaw the ladder on ice and mix well by pipetting or gentle vortexing
- For 8 mm lane width prepare:
- 2 μl 2x Loading buffer with 2 μl RNA-Ladder
- Vortex briefly and spin down
- Heat at 70 °C for 10 minutes
- Chill quickly on ice and load the gel
- Use 0.5 μl (0.125 μg) per mm lane width
After finishing gel electrophoresis stain the gel with ethidium bromide.

Use the same volume of RNA samples and marker. Dilute the samples with 2x Loading buffer and DEPC water. Additionally the concentration of loading buffer in
samples and marker should be equal.


Note: RNA is sensitive to degradation by ribonucleases. Working with any RNA Ladder of GeneOn all components have to be prepared fresh. All required tools and consumables should be treated with e.g. diethyl pyrocarbonate. Protect your hands with resistant gloves and your eyes with goggles!
 
Transportation: Shipped on blue ice

Storage: at -20°C/ -70°C for 12 months

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