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Invitrogen™ E-Gel™ SizeSelect™ II Agarose Gels, 2%
Description
Includes
Includes 10 gels, and 1 vial 10X Sample Loading Buffer
Electrophoresis using E-Gel SizeSelect II Agarose Gels is a convenient method for accurate size selection of DNA libraries for next-generation sequencing (NGS) applications. With E-Gel SizeSelect II gels, you can separate and recover DNA for library construction in three easy steps: load, run and retrieve.
E-Gel SizeSelect II agarose gels enable you to:
- Save time—no need to prepare a gel and gel-purify after electrophoresis
- Simplify DNA recovery—retrieve purified DNA directly from the recovery well with a pipette
- Improve result consistency—achieve accurate and consistent size selection
Fast and accurate DNA size selection in three easy steps
DNA fragment library size selection with E-Gel SizeSelect II precast gels is a simple 3-step procedure that eliminates conventional gel purification. To extract the DNA band of interest, load the sample into the loading wells, run the gel until the band reaches the recovery wells, and retrieve the sample. The resulting fragment library demonstrates a sharp fragment cut-off and is ready for use in an NGS workflow without any need for re-purification. Multiple bands from the one loading well can be collected during the same gel run.
DNA fragment libraries extracted from E-Gel SizeSelect II gels is compatible with the Ion Torrent sequencing workflow.
Real-time control of the sample
SYBR Gold II DNA Gel Stain is incorporated into the gel itself, allowing you to visually monitor DNA band migration progress on the blue-light transilluminator of the E-Gel Power Snap Electrophoresis Device. The gel has reference marks for better control of the sample prior to the sample recovery step. If the target DNA passes the recovery well, the Reverse gel protocol allows for re-capture of the DNA band.
Enables better results
Even a short exposure of your DNA sample to UV light during visualization may lead to DNA damage. Using E-Gel SizeSelect II gels together with the blue-light transilluminator minimizes the risk of UV damage compared to a conventional gel purification workflow. The direct access to your sample from the retrieval well allows you to avoid excising gel band slices and the risk of losing your DNA during a gel purification step.
Specifications
Specifications
| Compatible Ladders | E-Gel™ Sizing DNA Ladder |
| Content And Storage | Store at room temperature. |
| Gel Percentage | 2% |
| Gel Type | E-Gel |
| Label or Dye | SYBR Gold |
| Wells | 7-well |
| Quantity | 10 gels |
| Shipping Condition | Room Temperature |
| Product Type | Agarose Gel |
Frequently Asked Questions (FAQs)
You can use the Reverse E-Gel Program to run the band back into the collection gel.
Here are some suggestions:
- Try cleaning the cassettes with alcohol and Kimwipes wipers.
- Try cleaning the camera lens.
- Try to adjust the exposure time and brightness options of the documentation system you are using.
Please ensure that you have not overloaded the well and that the wells were not damaged during comb removal.
While we recommend storage at room temperature, these gels will still be usable. Bring the gels to room temperature prior to the run for optimal conditions.
Loading buffer is optional. Samples can be loaded directly into the wells if no buffer is used, or you can dilute them with deionized water or TE buffer. If you want to use a loading buffer, please see the recipes below:
E-Gel agarose gels (including EX)
10 mM Tris-HCl, pH 7.5
1 mM EDTA
0.005% bromophenol blue
0.005% xylene cyanol FF
E-Gel CloneWell II and E-Gel SizeSelect II agarose gels
10 mM Tris-HCl, pH 7.5
1 mM EDTA
Alternatively, you can use 10X BlueJuice Gel Loading Buffer or TrackIt Loading Buffer. Dilute this buffer 50- to 200-fold to obtain optimal results with E-Gel agarose gels.
For Research Use Only. Not for use in diagnostic procedures.
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