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ROTI®Load DNA orange 1 (with glycerol)

ROTI®Load DNA orange 1 (with glycerol)

SKU HP04.1
€ 73,08
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ROTI®Load DNA orange 1 (with glycerol)
Product Details
P-phrases: P201 P280 P308+P313
H-phrases: H360FD
HS code: 29054500
Brand: Carl Roth
ROTI®Load DNA orange 1 (with glycerol), 6x DNA gel load. buffer,ready-t-use, DNase-free, Density (D) 1,15 g/cm³, Boiling point (bp) ~100 °C, Storage temp. -20 °C

The Carl ROTH gel loading buffers are special buffer mixtures for nucleic acid electrophoresis, which are used as sample additives during gel loading. The gel loading buffers are ready-to-use solutions, which may be used directly.


ROTI®Load DNA buffer solutions contain Tris, sodium acetate and EDTA, with additional tracking dyes. For increasing the density when loading the gel, they are available in three different variations - with glycerol, ficoll and saccharose.


Arbeidsconcentratie

ROTI®Load DNA can either be added directly to the dissolved sample or the precipitated RNA can be solubilised directly in ROTI®Load DNA. ROTI®Load DNA gel loading buffer is usually used as 1x concentrated solution.



ROTI®Load DNA orange 1 (with glycerol) 6x conc., DNase-free
Gebruiksinstructies

ROTI®Load DNA-orange 1 (with glycerol) is a special gel loading buffer with orange G as the only dye optimized for very short runs. Orange G runs in the very small fragment range and shows the maximum running distance for very short runs (see lane 6 in the product image). Also well suited if bromophenol blue or xylene cyanol could mask important DNA bands.


Glycerin is the standard reagent for increasing sample density.


Each batch is tested for its functionality in electrophoresis and proved to be DNAse-free.



Technische informatie
Kleurstof Orange G
Incl. DNA-kleuring nee
Toepassing Very short separation distances, small fragments, high concentrated or High Resolution agarose
Selecting a Suitable ROTI®Load Gel Loading Buffer for Nucleic Acids

Care should be taken to ensure that the dyes contained in the gel stop before smallest relevant DNA bands. This ensures that the buffer can be stopped in time. However, the selected dyes may overlay the bands shown. In this case, select a loading buffer that does not contain any unwanted dyes.
Bromophenol blue and xylene cyanol can be used as colour markers in all standard gels. If a relevant band is overlaid by one of these colour markers, choose a gel loading buffer containing Orange G. If small fragments are to be assayed, the gel loading buffer should contain Orange G in order to mark the run. If relevant bands are overlaid, however, a choice can be made between bromophenol blue or xylene cyanol depending on the size of the bands. A loading buffer without xylene cyanol is usually used for assaying large fragments.

Glycerine is the standard reagent for increasing the density of samples.
Ficoll® 400 produces particularly well-defined bands.


Each batch is functionally tested for its suitability in electrophoresis and for DNAse-freeness.
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