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RNA Ladders » RNA Ladder LowRange ready-to-use
RNA Ladder LowRange ready-to-use
RNA Ladders from GeneOn are ideal for sizing and quantification of single-stranded RNA fragments
| Cat.-no |
Description |
Amount |
Price € |
Shop |
| 300025 |
RNA Ladder LowRange, 100 - 1000 b, rtu |
5 x 40 µl |
129.00 |
add |
| 300026 |
RNA Ladder LowRange, 100 - 1000 b, rtu |
15 x 40 µl |
359.00 |
add |
RNA Marker LowRange: Order by E-mail
RNA Marker LowRange: Datasheet
RNA Marker LowRange: Deutsche Beschreibung
Features:
The ladder is designed for qualitative and quantitative analysis of RNA on agarose gels with ethidium bromide or Sybr-Green II as dyes.
Description:
Mixture of 7 RNA transcripts from specific templates including l-sequences and a fragment of the pTZ19R poly linker, re-dissolved in 1 mM EDTA (pH 6.0). The RNA-Ladder is suitable for the analysis of RNA in native or denatured agarose gels (1.7 – 2.5 %) and polyacrylamide gels (4 – 8 %) and can be stained by ethidium bromide. The ladder is supplied in 1X Loading buffer and is ready-to-use.
Concentration: 0.25 mg RNA/ml
2X RNA Tracking dye (included):
95 % formamide, 0.025 % SDS, 0.025 % bromphenol blue, 0.025 % xylene cyanol, 0.025% ethidium bromide and 0.5 mM EDTA
1X Loading buffer (included): 10 mM K-Acetate (pH 4.5), 47.5 % formamide, 0.0125 % SDS, 0.0125 % bromophenol blue, 0.0125 % xylene cyanol, 0.0125 % ethidium bromide and 0.25 mM EDTA
Storage Buffer: 1 mM EDTA (pH 6.0)
Number of bands: 1000, 800, 600, 400, 300, 200 and 100 bases
Quality control/results:
- Absence of ribunucleases
- Determination of RNA concentration by spectralphotometer
- free of degraded RNA and NTP's
Electrophoresis:
- denaturing formaldehyde agarose with MOPS buffer
- denaturing polyacrylamide gel electrophoresis in TBE buffer
- native 2% agarose with TAE buffer
- denaturing glyoxal/DMSO agarose with sodium phosphate buffer
Loading for native or denaturing agarose gels:
LowRange RNA-Ladder is pre-mixed with Loading buffer (1X)
- Use the supplied 2X RNA Loading Dye both for sample
RNA and RNA ladder and mix equal volumes of the 2X RNA
Loading dye and RNA sample
- Thaw the ladder on ice and mix well by pipetting or gentle
vortexing
- Use 0.5 μl (0.125 μg) per mm lane widthready-to-use RNA
Ladder in fresh tube
- Vortex briefly and spin down
- Heat at 70 °C for 10 minutes
- Chill quickly on ice and load the gel
After finishing gel electrophoresis stain the gel with ethidium bromide
Loading of equal volumes of the sample and the ladder is recommended
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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