Team:Harvard/Template:NotebookDataJuly3

From 2011.igem.org

(Difference between revisions)
(PCR on minipreps to check cross junction)
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**Placed colonies in 20 μL of water and used 1 μl for a 20 μL PCR reaction
**Placed colonies in 20 μL of water and used 1 μl for a 20 μL PCR reaction
**Then took 10 μL from 20 μL dilution and added to 100 μL of LB in 96 well plate and put in 30°C fridge, at 3:19 pm
**Then took 10 μL from 20 μL dilution and added to 100 μL of LB in 96 well plate and put in 30°C fridge, at 3:19 pm
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**Same protocol as [[Protocols#PCR|KAPA PCR]] with the following changes made
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**Same protocol as [https://2011.igem.org/Team:Harvard/Protocols#PCR KAPA PCR] with the following changes made
***Step 3, gradient for annealing, 55°C - 77°C, for a range of 55,57,59,61 and 63°C for the two rows of 5 PCR tubes each (placed leftmost)
***Step 3, gradient for annealing, 55°C - 77°C, for a range of 55,57,59,61 and 63°C for the two rows of 5 PCR tubes each (placed leftmost)
***Step 4, Extension, 1 min
***Step 4, Extension, 1 min
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**Name: TOLCGRAD, PCR5 machine.</div>
**Name: TOLCGRAD, PCR5 machine.</div>
<div id="719" style="display:none">
<div id="719" style="display:none">
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==July 19th==
==July 19th==
===Team ZF===
===Team ZF===

Revision as of 19:10, 3 August 2011