30ml Ripa Lysis Buffer Weak Immunol Precipitation Lysis Solution
China 30ml Ripa Lysis Buffer Weak Immunol Precipitation Lysis Solution, Find details about China Ripa Lysis Buffer, Western Blot Lysis Buffer from 30ml Ripa Lysis Buffer Weak Immunol Precipitation Lysis Solution
Basic Info.
Model NO.
G2033-30ML
Habit Appellation
Special Reagent
Application
Industry, Scientific Research
Property
Biochemical Reagent
Trademark
Servicebio
Specification
30ML
Origin
China
Model NO.
G2033-30ML
Habit Appellation
Special Reagent
Application
Industry, Scientific Research
Property
Biochemical Reagent
Trademark
Servicebio
Specification
30ML
Origin
China
Product Desciption
Product introduction:
RIPA Lysis Buffer (RIPA Lysis Buffer) is a traditional cell and tissue rapid lysis Buffer. The protein sample after lysis with RIPA lysis Buffer can be used for regular Western, IP, etc. There are many formulas for RIPA lysis Buffer, which can be divided into strong, medium and weak according to the effect. This lysate is RIPA weak lysate, and its main components are 50 mM Tris-Hcl, 150 mM NaCl, 1 mM EDTA-Na2, 1% NP-40, 0.25% Sodium deoxycholate.
Package Contents:
Storage conditions: Store at 4ºC in the dark, valid for 12 months.
Instructions:
For tissue samples:
1. The tissue pieces are washed with cold PBS to remove blood stains. Cut into small pieces and place in a homogenizer.
2. Add 10 times the volume of the tissue to this reagent (add protease inhibitor within a few minutes before use) and homogenize thoroughly with a high-speed tissue grinder.
3. Transfer the homogenate to a 1.5 mL centrifuge tube and shake. In the ice bath for 30 minutes, pipette repeatedly to ensure complete cell lysis.
For cultured cell samples:
1. For adherent cells:
A. Wash the cells 2-3 times with PBS. Thoroughly absorb the remaining liquid one last time.
2. For suspension cells:
Collect the cells by centrifugation, add about 250 uL of this reagent (add protease inhibitor within a few minutes before use) per 6-well plate cells, and shake.
Ice bath for 30 minutes, during which time, pipette with a 200uL pipette several times every 10 minutes to ensure that the cells are completely lysed.
Precautions:
For tissue samples:
Approximately 1mL of this reagent is added to lyse every 50mg tissue. For tissues such as cartilage and skin, the dosage of reagents can be appropriately reduced to increase the protein concentration.
For cultured cell samples:
1. Under normal cell density, add about 250uL of lysate to each 6-well plate cell.
2. It may appear thicker during cracking. It can be pipetted repeatedly until it is liquid. If it has been thicker, you can use a vortex to shake or add an appropriate amount of lysate.
RIPA Lysis Buffer (RIPA Lysis Buffer) is a traditional cell and tissue rapid lysis Buffer. The protein sample after lysis with RIPA lysis Buffer can be used for regular Western, IP, etc. There are many formulas for RIPA lysis Buffer, which can be divided into strong, medium and weak according to the effect. This lysate is RIPA weak lysate, and its main components are 50 mM Tris-Hcl, 150 mM NaCl, 1 mM EDTA-Na2, 1% NP-40, 0.25% Sodium deoxycholate.
Package Contents:
| Product Item No. | Product Name | Specification |
| G2033 | RIPA Lysis Buffer | 30ml/100 mL |
Storage conditions: Store at 4ºC in the dark, valid for 12 months.
Instructions:
For tissue samples:
1. The tissue pieces are washed with cold PBS to remove blood stains. Cut into small pieces and place in a homogenizer.
2. Add 10 times the volume of the tissue to this reagent (add protease inhibitor within a few minutes before use) and homogenize thoroughly with a high-speed tissue grinder.
3. Transfer the homogenate to a 1.5 mL centrifuge tube and shake. In the ice bath for 30 minutes, pipette repeatedly to ensure complete cell lysis.
- Centrifuge at 12000g for 5 min, and collect the supernatant, which is the total protein solution.
For cultured cell samples:
1. For adherent cells:
A. Wash the cells 2-3 times with PBS. Thoroughly absorb the remaining liquid one last time.
- Add an appropriate volume of this reagent (add protease inhibitor within a few minutes before use) in the culture plate and bottle for 3-5 min. During this period, the culture plate and bottle were shaken repeatedly to make the reagents fully contact the cells.
- Scrape the cells and reagents with a cell scraper and collect them in a 1.5 mL centrifuge tube.
2. For suspension cells:
Collect the cells by centrifugation, add about 250 uL of this reagent (add protease inhibitor within a few minutes before use) per 6-well plate cells, and shake.
Ice bath for 30 minutes, during which time, pipette with a 200uL pipette several times every 10 minutes to ensure that the cells are completely lysed.
- Centrifuge at 12000g for 5 min, and collect the supernatant, which is the total protein.
Precautions:
For tissue samples:
Approximately 1mL of this reagent is added to lyse every 50mg tissue. For tissues such as cartilage and skin, the dosage of reagents can be appropriately reduced to increase the protein concentration.
For cultured cell samples:
1. Under normal cell density, add about 250uL of lysate to each 6-well plate cell.
2. It may appear thicker during cracking. It can be pipetted repeatedly until it is liquid. If it has been thicker, you can use a vortex to shake or add an appropriate amount of lysate.
3.This reagent is harmful to the human body, please protect it appropriately.
You Might Also Like
Zinc It Done Water-Based Galvanizing Spray Paint Aqueous Gal......
EPA/Carb Certificated Fuel Line Fuel Hose for Garden Machine......
100g high performance desiccant in Tyvek
Truck Spare Parts Weichai Engine Intake Rocker Arm Best
Art Glass Smoking Water Pipe ( AY 020)
Pdadmac 40% Cationic Polymer for Sludge Dewatering
Hot-Sale HDI Multilayer Printed Circuit Board Fr4 PCB Power ......
High-End Wall Mounted Storage Holder Rack for Kitchen Goldmi......
Rth -1100A Non Woven Sheet Cutting Machine Sheet Label Cutti......
Non Crosslinked Hyaluronic Acid Meso Filler for Lip Injectio......