Agarose High Resolution

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Catalogue No: abx299904
Price: US$406.00
(Size: 100 g)

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Datasheet

The High resolution agarose is a high strength gel agarose and high resolution, suitable for the routine analysis of different fragments of nucleic acids, in separation techniques such as electrophoresis, chromatography, blotting and others, used in the field of Biochemistry and Molecular Biology.

Specification:

Moisture≤ 10%
Gel strength (1.5% gel)≥ 1600 g/cm2
Gelling point (1.5% gel)41-45 °C
Melting point (1.5% gel)84-88 °C


Target Agarose High Resolution
Storage Store at room temperature.
Availability Shipped within 10-15 working days.
Note This product is for research use only.
Directions for use Preparation of agarose gel in the microwave.
1. Define the quantity needed to prepare the gel at the desired concentration.
2. Add necessary volume of run buffer (TAE, TBE to 1X).
3. Homogenize and microwave for 2 - 4 minutes, considering cycles of 30 seconds, until the sample is completely dissolved. Caution: Use necessary protection for the handling of hot material. Suggestion: Work in microwave at medium power.
4. Add selected staining agent (e.g. Ethidium Bromide or other) and homogenize
5. Allow to cool to 60° C - at room temperature - load electrophoresis mold and let gel.
6. Remove mold from wells, mount electrophoresis chamber, load samples and run buffer - same buffer with which the gel was prepared - and start the electrophoretic run.

Preparation agarose gel in heating plate.
1. Define the mass needed to prepare the gel at the desired concentration.
2. Add necessary volume of run buffer (TAE, TBE to 1X).
3. Homogenize and carry out a heating plate with stirring. Once the boiling has started, measure 20 minutes (use a lid or refrigerant system to avoid concentrating the sample).
4. Add selected staining agent (e.g. Ethidium Bromide or other) and homogenize.
5. Allow to cool to 60° C - at room temperature - load electrophoresis mold and let gel.
6. Remove mold from wells, mount electrophoresis chamber, load samples and run buffer - same buffer with which the gel was prepared - and start the electrophoretic run.
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