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Silver Stain Kit [for Electrophoresis]
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Product Information
- Components : Solution-1 (Enhancing solution) 50 mL, Solution-2 (Staining solution) 50 mL, Solution-3 (Developer solution #1) 50 mL, Solution-4 (Developer solution #2) 50 mL
- Size : 50 tests (90 mm x 80 mm, 1 mm gel)
Description
- Silver staining is a highly-sensitive and rapid detection method for SDS-PAGE separated proteins or nucleic acids. It is several times more sensitive than the commonly used EtBr or CBB staining methods.
Direction for Use
[Solution Preparation]
- Agitate each included solution well, and prepare the following 4 solutions in advance.
The volumes of reagents given below is based on a gel size of 90 mm x 80 mm x 1 mm. For different sizes of gel, the volume of reagents should be adjusted accordingly. For methanol and acetic acid, it is recommended to use special grade or any other higher grade. - Fixing Solution : Deionized water : 40 mL + Methanol : 50 mL + Acetic acid : 10 mL + Solution-1 (Enhancing solution) : 1 mL
- Staining Solution : Deionized water : 100 mL + Solution-2 (Staining solution) : 1 mL
- Developer Solution : Deionized water : 200 mL + Solution-3 (Developer solution #1) : 1 mL + Solution-4 (Developer solution #2) : 1 mL
- Stop Solution : Deionized water : 100 mL + Acetic acid : 1 mL
[Usage]
- Soak the gel in 100 mL of Fixing Solution in a clean tray and incubate it with shaking for 10 minutes.
- Remove the solution from step 1, and wash gel with 100 mL of deionized water with shaking for 10 minutes.
(Repeat a total of three times) - Remove the solution from step 2, and add 100 mL of Staining Solution. Allow to incubate with shaking for 5 minutes.
*When disposing of Solution-2 (i.e. Staining Solution), add hydrochloric acid or sodium chloride to the container to precipitate out silver chloride. - Remove the solution from step 3, and add 100 mL of deionized water. Incubate with shaking for 30 seconds.
- Remove the solution from step 4, and add 100 mL of Developer Solution. Incubate with shaking for 30 seconds.
- Remove the solution from step 5, and add 100 mL of Developer Solution. Allow to incubate with shaking until developed bands appear.
*Developing time will vary by sample, temperature, and thickness of gel, so adjust accordingly.
*A 90 mm x 80 mm x 1 mm gel will take approximately 5-10 minutes. - Remove the solution from step 6, and add 100 mL of Stop Solution. Incubate with shaking for 10 minutes.
- Remove the solution from step 7, and wash with 100 mL of deionized water, incubating with shaking for 5 minutes between washes. (Repeat a total of three times.)
Storage
- Store at 4 ºC. This product is photosensitive and should be protected from light. Use within 1 year.
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