RNAi專用的轉染試劑


                        RNAifectin™ Transfection Reagent, G073



 


【太鼎生物科技有限公司02-86609496abmgood台灣總代理


 










Cat.No.:G073
Quantity:1.0ml (100-500 transfections)





















Description



Escpecially developed for the efficient transfection of eukaryotic cells with RNAi oligo's. This transfection reagent is perfect for any of your RNAi transfection needs.



Application



RNAi knockdown experiments in a wide variety of cell lines (HeLa, HEK-293 etc). Highly specific and non-toxic transfection.



Protocol





Storage



Store at 4ºC. Do not freeze.



Notes



This product is distributed for laboratory research only. Caution: Not for diagnostic use .



產品介紹 Description


ANAifectin™ is a transfection reagent specially formulated with multiple cationic polymers. It is suitable for the transfection of RNAi oligoes into cultured eukaryotic cells.


RNAi轉染操件手冊:


These conditions are recommended as guidelinesonly. A 6-well or 35mm dish is adequate for most applications, but larger vessels are sometimes required. In that case, consult table 1.



1. In a 6-well plate, seed cells at a density of 1-3x10⁵ per well in 2.0ml of the appropriate
growth medium (with serum if cells are cultured in presence of serum). Incubate the cells at 37°C until cells are 60-90% confluent. This will usually take 18-24 hours, depending on cell types. Since transfection efficiency is sensitive to culture confluence, it is important to maintain a standard seeding protocol from experiment to experiment


2. Prepare the following solutions in sterile 12x75 mm or microcentrifuge tubes: Solution A: For each transfection, dilute 1-3μg of RNAi oligoes into 125μl serum-free
medium. Solution B: For each transfection, dilute 4-10μl of
RNAifectin™ reagent into 125μl of serum-free medium. (Vortex RNAifectin™ reagent before use)


3. Combine the solutions, mix thoroughly and incubate at room temperature for 20 mins to
allow DNA-lipsome complexes to form.


4. Remove growth medium from the cells and add 800μl of serum-free medium to the cells.


5. Add the RNAifectin™-oligo complexes to thecells, mix gently to ensure uniform distribution
and incubate at 37°C for 2-24 hours. We recommend starting with 5 hours.


6. Remove the transfection solution and add 2.0ml of the appropriate complete growth medium(with serum) to each well. Incubate cells at 37°Cfor a total of 24-72 hours.


7. Assay cell extracts for gene activity 24-72 hours a􀄞er the start of transfection depending on the cell types and promoter activity.


8. A similar procedure can be used to transfect an RNAi vector for stable expression. At 72 hours a􀄞er transfection, split the cells at a ratio of 1:10 into the selective medium for the marker gene transfected.


【太鼎生物科技有限公司02-86609496abmgood台灣總代理



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