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GelRed Nucleic Acid Stain 10,000X in water - 0.5 ml

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High-sensitivity nucleic acid stain for gel electrophoresis, providing clear, sharp bands, supplied by Gentaur's warehouse.

GelRed™ Staining Protocol (Precast Method)

Product: GelRed™ Nucleic Acid Stain, 10,000X in water

Volume: 0.5 ml (sufficient for 100+ gels depending on usage)

Applications: dsDNA, ssDNA, RNA visualization


 I. Materials Required

Agarose


TAE or TBE buffer


DNA samples + loading dye


GelRed™ 10,000X in water


Gel casting tray and combs


Microwave or hot plate


Electrophoresis apparatus


UV or Blue LED transilluminator


🧫 II. Precasting Gel with GelRed™

This method avoids post-staining and reduces handling time.


1. Prepare Agarose Gel:

Dissolve agarose in 1X TAE or TBE buffer (e.g., 1 g agarose in 100 mL buffer for 1% gel).


Heat until completely melted (microwave or hot plate).


2. Cool Gel:

Let the gel solution cool to about 60°C (touch warm, not hot).


3. Add GelRed™:

Add 5 µL of 10,000X GelRed™ to 50 mL of molten agarose.


Mix gently (avoid bubbles).


✅ Dilution Factor: 1:10,000

 Do not add GelRed™ to very hot agarose — may degrade stain.


4. Cast the Gel:

Pour into tray, insert combs, and allow to solidify (~30 minutes).


5. Run the Gel:

Load samples and run electrophoresis as usual.


6. Visualize DNA:

Use UV or blue light transilluminator (blue preferred to reduce DNA damage).


Use orange filter if imaging with blue light.


🧪 III. Post-Staining Method (if desired)

If not precast, you can post-stain:


1. Dilute GelRed™:

Add 5 µL of 10,000X GelRed™ to 50 mL water or buffer.


2. Stain Gel:

Submerge gel in staining solution.


Incubate 30 minutes with gentle agitation (light-protected).


🔐 Storage & Safety

Store at room temp (RT) or 4°C, protected from light.


Non-mutagenic, safer than ethidium bromide (see Biotium's safety data).


Dispose of according to institutional biosafety guidelines.

210.00 € 210.0 EUR 210.00 € Tax Excluded

210.00 € Tax Excluded

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