RNA Sample Loading Buffer, Without ethidium bromide

Code: r1386-5vl D2-231

Not available outside of the UK & Ireland.

Application

Suitable for use with formaldehyde-agarose gels used in Northern blotting procedures.

RNA sample loading buffer is especially formulated for electrophoresis...


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$146.45 EACH

Not available outside of the UK & Ireland.

Application

Suitable for use with formaldehyde-agarose gels used in Northern blotting procedures.

RNA sample loading buffer is especially formulated for electrophoresis of RNA on formaldehyde-agarose gels with or without ethidium bromide. Ethidium bromide is not recommended for gel staining prior to Northern blot detection because the presence of ethidium bromide in agarose gels or the loading buffer can cause poor transfer efficiency.

Components

Deionized formamide 62.5% (v/v), formaldehyde 1.14 M, bromphenol blue 200 µg/mL, xylene cyanole 200 µg/mL, MOPS-EDTA-sodium acetate at 1.25× working concentration.

RNA loading buffer contains 62.5% deionized formamide, 1.14M formaldehyde, 200 µg/ml bromphenol blue, 200 µg/ml xylene cyanole, in MOPS-EDTA-sodium acetate at 1.25x working concentration.

General description

RNA loading buffer is used as a tracking dye during RNA electrophoresis. The dye has a slight negative charge and will migrate the same direction as RNA, allowing the user to monitor the progress of molecules moving through the gel. The rate of migration varies with gel composition. Dilute 1:3 to 1:6 with sample, heat to 65C for ten minutes and chill on ice before loading.

Quantity

Recommended usage: Add 1 volume sample to 2-5 volumes of sample loading buffer and mix well. The sample should be heated to 65 °C for 10 minutes, and then chilled on ice immediately before loading on the gel.

foreign activityRNase, none detected
formsolution
gradefor molecular biology
Quality Level200
storage temp.−20°C
This product has met the following criteria: