Team:EPF-Lausanne/Notebook/October2011

From 2011.igem.org

(Difference between revisions)
(Sunday, October 16 2011)
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For the K1 backbone, the recipe was slightly different due to the higher concentration of blunted DNA we wanted to achieve:
For the K1 backbone, the recipe was slightly different due to the higher concentration of blunted DNA we wanted to achieve:
-
   
+
  * H20 - 4.4 uL
 +
* NEBuffer2 (10X, found in enzyme ice box) - 4 uL (needs to be at a final concentration of 1X)
 +
* dNTP (10 mM) - 0.4 (needs to be at a final concentration of 100 uM)
 +
* template - 30 uL (for 1.5 ug of DNA, assuming the T7 + Lysis was at a concentration of 100 ng/uL)
 +
* T4 Polymerase - 1.2 uL (it comes at a "concentration" of 3000 units/mL and we want 1.5 units)
 +
 
 +
for a total of 40 uL.
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Revision as of 09:32, 17 October 2011