Team:LCG-UNAM-Mexico:Journals:Uriel
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with a restriction assay was done and also ogr+ter+18 was purified and opened digested with EcoRI/PstI to be prepared | with a restriction assay was done and also ogr+ter+18 was purified and opened digested with EcoRI/PstI to be prepared | ||
in case last ligation don't work. | in case last ligation don't work. | ||
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+ | == September 15, 2009 == | ||
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+ | The ligation didn't work, I planned to follow a different strategy first purify the cox fragment using Low melt point Agarose, we are using this procedure because the plasmido that contain cox is the samen as the one that has ogr+ter and | ||
+ | as a consequence the same antibiotic resistance gene, so by separating the DNA by electrophoresis we can take apart cox gene and the ligated in to the dephoshorylated plasmid ogr+ter that was digested EcoRI/XbaI, the resultin plasmid will be cox+ogr+ter. | ||
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+ | == September 22, 2009 == | ||
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+ | Band purification: | ||
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+ | Quiagen gel exration kit was used for this. | ||
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+ | An 1% Low melt point agarose gel was loaded with the sample that contained cox+18, the gel was stained with ethdium bromaid and saw with a transluminator. Once we saw our band it was cut from the gel and transferred to an 1.5 mL tube | ||
+ | and weighted (0.13g) in the kit protocol they propose an equivalences of buffer 100mg~100µL so we have to add 3 volumes of each 130µL of buffer and follow the kit protocol. | ||
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+ | == September 23, 2009 == | ||
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+ | A ligation is going to be done with cox and ogr+ter, ogr+ter+18 was dephosphorylated and cox was purified via gel. As a control we will try to religate the dephosphorylated plasmid, the same plasmid not dephosphorylated and a uncut plasmid | ||
+ | which must transform because was not digested. | ||
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+ | Ligation Reaction: | ||
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Revision as of 12:52, 20 October 2009