Team:UNITN-Trento/Notebook/Labposts/08/43

From 2013.igem.org

(Difference between revisions)
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{
{
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"date" : "2013-08-31",
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"date":"2013-08-31",
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"author" : "fabio",
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"author":"fabio",
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"title" : " <html> the blue circuit doesn’t always work!!</html> ",
+
"title":" <html> the blue circuit doesn’t always work!!</html> ",
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"content" : " <html> I repeated the experiment with light induction lots and lots of times, but unfortunately a few time cells behaved strangely: even the dark control produced amilCP... probably the circuit is not perfectly regulated!! Now I have to think about a new cloning: pedro will try out a ligation of the circuit with EFE, instead I will try to insert EFE at the end of the improved circuit without inverter. I will do a PCR of the improved part with Kapa polymesase and then inserting this sequence inside the plasmid containing EFE +terminators. Then we will have ethylene production upon illumination.</html> ",
+
"content":" <html> I repeated the experiment with light induction lots and lots of times, but unfortunately a few time cells behaved strangely: even the dark control produced amilCP... probably the circuit is not perfectly regulated!! Now I have to think about a new cloning: pedro will try out a ligation of the circuit with EFE, instead I will try to insert EFE at the end of the improved circuit without inverter. I will do a PCR of the improved part with Kapa polymesase and then inserting this sequence inside the plasmid containing EFE +terminators. Then we will have ethylene production upon illumination.</html> ",
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"tags" : "blue_light-EFE"
+
"tags":"blue_light-EFE"
}
}

Revision as of 08:03, 25 September 2013

{ "date":"2013-08-31", "author":"fabio", "title":" the blue circuit doesn’t always work!! ", "content":" I repeated the experiment with light induction lots and lots of times, but unfortunately a few time cells behaved strangely: even the dark control produced amilCP... probably the circuit is not perfectly regulated!! Now I have to think about a new cloning: pedro will try out a ligation of the circuit with EFE, instead I will try to insert EFE at the end of the improved circuit without inverter. I will do a PCR of the improved part with Kapa polymesase and then inserting this sequence inside the plasmid containing EFE +terminators. Then we will have ethylene production upon illumination. ", "tags":"blue_light-EFE" }