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Team:IIT Madras/Notebook/Protocols/Double restriction
From 2011.igem.org
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<li>Preparative Restrictions – 40 – 50 ul.</li> | <li>Preparative Restrictions – 40 – 50 ul.</li> | ||
<li>BSA should be added if recommended. 0.1 ul of BSA is usually added for 10 ul reactions.</li> | <li>BSA should be added if recommended. 0.1 ul of BSA is usually added for 10 ul reactions.</li> | ||
| + | <li>Run the products on a gel and check double digestion.</li> | ||
</ul> | </ul> | ||
</div> | </div> | ||
Latest revision as of 11:09, 2 October 2011
IIT Madras
And then the E.coli said, "Let there be light"
Double Restriction
Common Protocol
- Use NEB digest finder to find the buffer that is compatible for the digestion.
- The buffers are 10 X. Thus the volume of the buffer added to the digestion must be such that it is 1 X.
- Usually 0.3-0.5 ul of Enzymes can be used for every 1 ug of DNA – 1 unit of Enzyme is added.
- In case of sequential digestions, the following techniques can be used:
- Use enzyme 1 – restrict – purify DNA – Use Enzyme 2.
- Use enzyme which requires a more dilute buffer first, Then add the concentrated buffer for restricting DNA using 2nd Enzyme.
- Analytic Restrictions – final volume 10 ul.
- Preparative Restrictions – 40 – 50 ul.
- BSA should be added if recommended. 0.1 ul of BSA is usually added for 10 ul reactions.
- Run the products on a gel and check double digestion.
