Team:NJU China/Protocol
From 2013.igem.org
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Scaling Up or Down Transfections | Scaling Up or Down Transfections | ||
To transfect cells in different tissue culture formats, vary the amount of Lipofectamine TM 2000, nucleic acid, cells, and medium used in proportion to the relative surface area, as shown in the table. With automated, high-throughput systems a complexing volume of 50μl is recommended for transfections in96-well plates. Note: You may perform rapid 96-well plate transfections by plating cells directly into the transfection mix. Prepare complexes in the plate and directly add cells at twice the cell density as in the basic protocol in a 100μl volume. Cells will adhere as usual in the presence of complexes. | To transfect cells in different tissue culture formats, vary the amount of Lipofectamine TM 2000, nucleic acid, cells, and medium used in proportion to the relative surface area, as shown in the table. With automated, high-throughput systems a complexing volume of 50μl is recommended for transfections in96-well plates. Note: You may perform rapid 96-well plate transfections by plating cells directly into the transfection mix. Prepare complexes in the plate and directly add cells at twice the cell density as in the basic protocol in a 100μl volume. Cells will adhere as usual in the presence of complexes. | ||
- | </br><img width="400" | + | </br><img width="400" height="400" src="https://static.igem.org/mediawiki/2013/2/2f/20130927_222700.jpg"> |
</br>1Surface areas may vary depending on the manufacturer. | </br>1Surface areas may vary depending on the manufacturer. | ||
</br>2Volumes of dilution medium in Step 2a&2b of DNA or RNAi transfection protocols. | </br>2Volumes of dilution medium in Step 2a&2b of DNA or RNAi transfection protocols. |
Revision as of 14:31, 27 September 2013