10X EDTA buffer pH 8.0
Novus Biologicals, part of Bio-Techne | Catalog # NB900-66730
Key Product Details
Applications
Immunohistochemistry
Product Specifications
Specificity
10x EDTA Buffer pH 8.0 for Heat Induced Epitote Recovery
Application Notes
The antigen retrieval protocol is recommended for use in tissues that have been fixed in formalin only. Ensure that the fixed sections are adequately embedded in paraffin. Cut tissue sections to 4-5 microns.
Preparation of Working Solutions
1. The 10X concentrated format should be diluted tenfold with distilled or deionized water.
2. Mix one part of concentrated Antigen Retrieval Solution with nineparts of deionized or distilled water.
3. Shake the bottle vigorously to completely mix the components of theconcentrate (the solution may separate into phases over time).
4. Store with cap tightly secured.
Protocol Recommendations
1. Deparaffinize and rehydrate tissue sections.
2. Place slides into 1X retrieval solution in a slide container (e.g. Coplinjar, Tissue-Tek, staining dish or metal slide canister).
3. Retrieve sections under pressure
4. After take-off reagent jar containing slides from pressure cooker, allow the slides to cool for 20 minutes to reach room temperature.
5. Wash slides in deionized water and then with wash buffer. Proceed with immunostaining recommendations in the antibody datasheet.
6. Gently rinse by gradually adding DI water to the solution, thenremove slides and rinse with DI water.
Preparation of Working Solutions
1. The 10X concentrated format should be diluted tenfold with distilled or deionized water.
2. Mix one part of concentrated Antigen Retrieval Solution with nineparts of deionized or distilled water.
3. Shake the bottle vigorously to completely mix the components of theconcentrate (the solution may separate into phases over time).
4. Store with cap tightly secured.
Protocol Recommendations
1. Deparaffinize and rehydrate tissue sections.
2. Place slides into 1X retrieval solution in a slide container (e.g. Coplinjar, Tissue-Tek, staining dish or metal slide canister).
3. Retrieve sections under pressure
4. After take-off reagent jar containing slides from pressure cooker, allow the slides to cool for 20 minutes to reach room temperature.
5. Wash slides in deionized water and then with wash buffer. Proceed with immunostaining recommendations in the antibody datasheet.
6. Gently rinse by gradually adding DI water to the solution, thenremove slides and rinse with DI water.
Formulation, Preparation, and Storage
Formulation
Dilute one part buffer with nine parts de-ionized or distilled water.
Preservative
No Preservative
Concentration
Please see the protocols for proper use of this product. If no protocol is available, contact technical services for assistance.
Shipping
The product is shipped with polar packs. Upon receipt, store it immediately at the temperature recommended below.
Storage
Store at room temperature.
Background: 10X EDTA buffer pH 8.0
Additional 10X EDTA buffer pH 8.0 Products
Product Specific Notices for 10X EDTA buffer pH 8.0
This product is for research use only and is not approved for use in humans or in clinical diagnosis. Support products are guaranteed for 6 months from date of receipt.
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