Team:EPF-Lausanne/Notebook/October2011

From 2011.igem.org

(Difference between revisions)
(Sunday, October 16 2011)
(Sunday, October 16 2011)
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for a total of 40 uL.  
for a total of 40 uL.  
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== Sunday, October 23 2011 ==
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Vincent ran a colony PCR on the 1 and 13 T7 promoter + Lysis + psB3K1 constructs, since they were the ones that yielded the highest colony count (compared to the negative control). He chose ten colonies from each plate. The protocol was as followed:
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* TPB 2.5 uL
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* EPFL Taq 0.25 uL
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* primer FW (10 uM) 0.5 uL (1289_F, originally 100 uM)
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* primer RV (10 uM) 0.5 uL (pSB-Pcon-TetR-r, originally 20 uM)
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* template 2 uL of DNA (boiled)
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* dNTP 0.5 uL
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* dH20 18.75 uL
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===========================
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25 uL total
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The cycle (now called EPFLCOP for EPFL Colony PCR) is as follows:
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* 94 °C, 2 minutes
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30 times:
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* 94 °C, 15 sec.
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* 58 °C, 15 sec.
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* 68 °C, 1 minute (1 min / kb, and we expect 629 bp)
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End of 30
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* 68 °C, 5 min
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* 10 °C, infinitely
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{{:Team:EPF-Lausanne/Templates/Footer}}

Revision as of 14:16, 23 October 2011