Testing Data
RIPA Reagent
RIPA Lysis Buffer
Synonyms
RIPA; RIPA Lysis Buffer; RIPA reagent
Form/Format
Liquid. 50mM Tris-HCl pH7.6, 150mM NaCl, 1% NP-40, 0.5% sodium deoxycholate, 0.1% SDS
Concentration
Recommended working concentration
10mL RIPA Lysis Buffer per gram of tissue
0.5mL RIPA Lysis Buffer per 5.0x10^6 cells in suspension
0.5mL RIPA Lysis Buffer per 5.0x10^6 adherent mammalian cells (varies by lot)
10mL RIPA Lysis Buffer per gram of tissue
0.5mL RIPA Lysis Buffer per 5.0x10^6 cells in suspension
0.5mL RIPA Lysis Buffer per 5.0x10^6 adherent mammalian cells (varies by lot)
Compatibility with reagents
Fully compatible with Broad Spectrum Protease Inhibitor Cocktail and Broad Spectrum Phosphatase Inhibitor Cocktail
Reagent Type
Western Blotting related reagent; Cell lysis buffer; Universal tissue extraction buffer; Detergent solution
Usage
Extraction of cytoplasmic, membrane and nuclear proteins
Important Product Information
If desired, add protease inhibitor and phosphatase inhibitor to the lysis buffer to prevent proteolysis and maintain phosphorylation status of proteins.
Some protein kinases and other enzymes may be sensitive to the components of the RIPA Lysis Buffer, resulting in their decreased activity. In such cases, prepare a RIPA Lysis Buffer that does not contain sodium deoxycholate and SDS.
Some protein kinases and other enzymes may be sensitive to the components of the RIPA Lysis Buffer, resulting in their decreased activity. In such cases, prepare a RIPA Lysis Buffer that does not contain sodium deoxycholate and SDS.
Additional Materials Required
Protease inhibitor and phosphatase inhibitor
2mL microcentrifuge tubes
Tissue homogenizer
Microcentrifuge capable of spinning at 10,000 xg
Cell scraper
2mL microcentrifuge tubes
Tissue homogenizer
Microcentrifuge capable of spinning at 10,000 xg
Cell scraper
Procedure for Lysis of Monolayer-cultured Adherent Mammalian Cells
Note: Pre-chill an appropriate volume of RIPA Lysis Buffer at 4 degree C. If desired, add protease inhibitor and phosphatase inhibitor to the lysis buffer immediately before use.
1. In a microcentrifuge tube, resuspend 5x10^6 cells in the growth media by scraping the cells off the surface of the plate with a cell scraper. Centrifuge harvested cell suspension at 600xg for 5min, then carefully remove and discard the supernatant.
2. Resuspend the cells in chilled PBS. Centrifuge at 600xg for 5min, then carefully remove and discard the supernatant.
3. Add 0. 5mL of chilled RIPA lysis buffer to the cell pellet. Vortex briefly. Incubate on ice for 30 minutes.
4. Centrifuge samples at 14000xg for 10 minutes.
5. Transfer supernatant to a new tube for further analysis.
Note: RIPA lysis buffer can be added directly to the flask containing cells. Please see the following procedures.
1. Carefully remove culture medium from adherent cells.
2. Wash cells with chilled PBS. Carefully remove PBS.
3. Add chilled RIPA lysis buffer to the cells. Vortex briefly. Incubate on ice for 30 minutes. (For the volume of the lysis buffer, follow the instructions listed below)
SIZE of the plate/surface area: Volume of the lysis buffer
100mm: 500-1000uL
60mm: 250-500uL
6-well plate: 200-400uL per well
-well plate: 100-200uL per well
96-well plate: 50-100uL per well
4. Centrifuge samples at 14000xg for 10 minutes.
5. Transfer supernatant to a new tube for further analysis.
1. In a microcentrifuge tube, resuspend 5x10^6 cells in the growth media by scraping the cells off the surface of the plate with a cell scraper. Centrifuge harvested cell suspension at 600xg for 5min, then carefully remove and discard the supernatant.
2. Resuspend the cells in chilled PBS. Centrifuge at 600xg for 5min, then carefully remove and discard the supernatant.
3. Add 0. 5mL of chilled RIPA lysis buffer to the cell pellet. Vortex briefly. Incubate on ice for 30 minutes.
4. Centrifuge samples at 14000xg for 10 minutes.
5. Transfer supernatant to a new tube for further analysis.
Note: RIPA lysis buffer can be added directly to the flask containing cells. Please see the following procedures.
1. Carefully remove culture medium from adherent cells.
2. Wash cells with chilled PBS. Carefully remove PBS.
3. Add chilled RIPA lysis buffer to the cells. Vortex briefly. Incubate on ice for 30 minutes. (For the volume of the lysis buffer, follow the instructions listed below)
SIZE of the plate/surface area: Volume of the lysis buffer
100mm: 500-1000uL
60mm: 250-500uL
6-well plate: 200-400uL per well
-well plate: 100-200uL per well
96-well plate: 50-100uL per well
4. Centrifuge samples at 14000xg for 10 minutes.
5. Transfer supernatant to a new tube for further analysis.
Procedure for Lysis of Suspension-cultured Mammalian Cells
Note: Pre-chill an appropriate volume of RIPA Lysis Buffer at 4 degree C. If desired, add protease inhibitor and phosphatase inhibitor to the lysis buffer immediately before use.
1. In a microcentrifuge tube, harvest 5x106 cells by centrifugation at 600xg for 5min. Carefully remove and discard the supernatant.
2. Resuspend the cells in chilled PBS. Centrifuge at 600xg for 5min, then carefully remove and discard the supernatant.
3. Add 0. 5mL of chilled RIPA lysis buffer to the cell pellet. Vortex briefly. Incubate on ice for 30 minutes.
4. Centrifuge samples at 14000xg for 10 minutes.
5. Transfer supernatant to a new tube for further analysis.Procedure for Lysis of Tissues:
Note: Pre-chill an appropriate volume of RIPA Lysis Buffer at 4 degree C. If desired, add protease inhibitor and phosphatase inhibitor to the lysis buffer immediately before use.
1. Place the fresh tissue into chilled PBS and rinse several times. Mince the tissue into small pieces.
2. Add RIPA Lysis Buffer to the tissue at 10:1. (i.e. Add 10mL cilled lysis buffer per gram of tissue.) Use a smaller volume of reagent if a more concentrated protein extract is required.
3. Homogenize for several minutes at high speed until no tissue chunks remain.
4. Incubate on ice for 30 minutes.
5. Centrifuge at ~10000 x g for 10 minutes.
6. Transfer supernatant to a new tube for further analysis.
1. In a microcentrifuge tube, harvest 5x106 cells by centrifugation at 600xg for 5min. Carefully remove and discard the supernatant.
2. Resuspend the cells in chilled PBS. Centrifuge at 600xg for 5min, then carefully remove and discard the supernatant.
3. Add 0. 5mL of chilled RIPA lysis buffer to the cell pellet. Vortex briefly. Incubate on ice for 30 minutes.
4. Centrifuge samples at 14000xg for 10 minutes.
5. Transfer supernatant to a new tube for further analysis.Procedure for Lysis of Tissues:
Note: Pre-chill an appropriate volume of RIPA Lysis Buffer at 4 degree C. If desired, add protease inhibitor and phosphatase inhibitor to the lysis buffer immediately before use.
1. Place the fresh tissue into chilled PBS and rinse several times. Mince the tissue into small pieces.
2. Add RIPA Lysis Buffer to the tissue at 10:1. (i.e. Add 10mL cilled lysis buffer per gram of tissue.) Use a smaller volume of reagent if a more concentrated protein extract is required.
3. Homogenize for several minutes at high speed until no tissue chunks remain.
4. Incubate on ice for 30 minutes.
5. Centrifuge at ~10000 x g for 10 minutes.
6. Transfer supernatant to a new tube for further analysis.
Precautions
All steps of protein lysis should be operated on ice or at 4 degree C.
Use BCA Protein Assay kit to quantify lysed proteins. Bradford Protein Assay kit is not recommended.
There might be some transparent gel complex containing genomic DNA in lysed proteins. The protein fractions can be used for further analysis after centrifugation if target proteins have little connection with genomic DNA. When detecting target proteins related closely to genomic DNA, sonicate gel complex and then centrifuge to collect supernatant for further analysis. Common transcription factors such as NFKB, p53 can be detected without sonication.
Use BCA Protein Assay kit to quantify lysed proteins. Bradford Protein Assay kit is not recommended.
There might be some transparent gel complex containing genomic DNA in lysed proteins. The protein fractions can be used for further analysis after centrifugation if target proteins have little connection with genomic DNA. When detecting target proteins related closely to genomic DNA, sonicate gel complex and then centrifuge to collect supernatant for further analysis. Common transcription factors such as NFKB, p53 can be detected without sonication.
Preparation and Storage
Upon receipt store at 4 degree C. RIPA Lysis Buffer is stable for one year. Product is shipped on ice.
Testing Data
Testing Data
Related Product Information for RIPA reagent
Description: RIPA Lysis Buffer is a complete cell lysis solution reagent used for rapid and efficient total cell lysis and solubilization of proteins from both adherent and suspension cultured mammalian cells, effectively extracting cytoplasmic, nuclear and membrane proteins. Protein lysis can be finished in 60 minutes.
Background: RIPA lysis extraction buffer contains non-ionic and ionic detergents which are able to extract protein from wide variety of cell types and membrane structures. RIPA buffer ensures efficient cell lysis and protein solubilization preventing protein degradation and interference with protein immunoreactivity and biological activity. Since most antibodies and protein antigens are not adversely affected by the components of this solution, RIPA buffer-conducted protein extraction is compatible with various downstream immunoprecipitation and molecular pull-down assays, including reporter assays, protein assays, immunoassays and protein purification. RIPA buffer reagent minimizes non-specific protein-binding interactions to keep background low, while allowing most specific interactions to occur, enabling studies of relevant protein-protein interactions.
Background: RIPA lysis extraction buffer contains non-ionic and ionic detergents which are able to extract protein from wide variety of cell types and membrane structures. RIPA buffer ensures efficient cell lysis and protein solubilization preventing protein degradation and interference with protein immunoreactivity and biological activity. Since most antibodies and protein antigens are not adversely affected by the components of this solution, RIPA buffer-conducted protein extraction is compatible with various downstream immunoprecipitation and molecular pull-down assays, including reporter assays, protein assays, immunoassays and protein purification. RIPA buffer reagent minimizes non-specific protein-binding interactions to keep background low, while allowing most specific interactions to occur, enabling studies of relevant protein-protein interactions.
Product Categories/Family for RIPA reagent
Similar Products
Product Notes
The RIPA (Catalog #AAA1753872) is a Reagent and is intended for research purposes only. The product is available for immediate purchase. It is sometimes possible for the material contained within the vial of "RIPA, Reagent" to become dispersed throughout the inside of the vial, particularly around the seal of said vial, during shipment and storage. We always suggest centrifuging these vials to consolidate all of the liquid away from the lid and to the bottom of the vial prior to opening. Please be advised that certain products may require dry ice for shipping and that, if this is the case, an additional dry ice fee may also be required.Precautions
All products in the AAA Biotech catalog are strictly for research-use only, and are absolutely not suitable for use in any sort of medical, therapeutic, prophylactic, in-vivo, or diagnostic capacity. By purchasing a product from AAA Biotech, you are explicitly certifying that said products will be properly tested and used in line with industry standard. AAA Biotech and its authorized distribution partners reserve the right to refuse to fulfill any order if we have any indication that a purchaser may be intending to use a product outside of our accepted criteria.Disclaimer
Though we do strive to guarantee the information represented in this datasheet, AAA Biotech cannot be held responsible for any oversights or imprecisions. AAA Biotech reserves the right to adjust any aspect of this datasheet at any time and without notice. It is the responsibility of the customer to inform AAA Biotech of any product performance issues observed or experienced within 30 days of receipt of said product. To see additional details on this or any of our other policies, please see our Terms & Conditions page.Item has been added to Shopping Cart
If you are ready to order, navigate to Shopping Cart and get ready to checkout.
