"
Team:Freiburg/Content/Notebook/Methods
From 2014.igem.org
| Line 21: | Line 21: | ||
<section> | <section> | ||
<h3>Gibson Assembly</h3> | <h3>Gibson Assembly</h3> | ||
| + | <p>To purify plasmid DNA we used several kits that were provided by our sponsors. For Minipreps we used Peqlab, Roche, qiagen, bioRon, Genetics, Roth. For Midipreps we used Qiagen, Jetstar, Peqlab. Beforehand o/n cultures of transformed <em class="highlight-kursiv">E.coli</em> were prepared. No deviances from the manufacturer's guidelines were incorporated by performing the isolation steps. | ||
| + | </p> | ||
</section> | </section> | ||
<section> | <section> | ||
| Line 30: | Line 32: | ||
<section> | <section> | ||
<h3>Plasmid Isolation</h3> | <h3>Plasmid Isolation</h3> | ||
| + | <p>First step of Gibson Assemblies was the rigidly calculation of molar amounts of the fragments. We afterwards joined the fragments and filled them up to 5 µL. These 5 µL were added to 15 µL ice chilled Gibson-Mastermix (Gibson et al., 2009), containing 5x ISO-Buffer, Taq-Ligase and T5 Exonuclease. Except Phusion Polymerase (Gibson et al., 2009) we used the same amount of Q5 Polymerase for the Mastermix. The samples were immediately heated to 50°C for one hour. Afterwards, the samples were cooled for 3 minutes at room temperature and 3 minutes on ice, before they were transformed into competent <em class="highlight-kursiv">E.coli</em>. | ||
| + | </p> | ||
</section> | </section> | ||
<section> | <section> | ||
Revision as of 15:55, 16 October 2014
Methods
Cloning
Agarose Gel Electrophoresis
Gel Extraction
Gibson Assembly
To purify plasmid DNA we used several kits that were provided by our sponsors. For Minipreps we used Peqlab, Roche, qiagen, bioRon, Genetics, Roth. For Midipreps we used Qiagen, Jetstar, Peqlab. Beforehand o/n cultures of transformed E.coli were prepared. No deviances from the manufacturer's guidelines were incorporated by performing the isolation steps.
Ligation
Oligo Annealing
Plasmid Isolation
First step of Gibson Assemblies was the rigidly calculation of molar amounts of the fragments. We afterwards joined the fragments and filled them up to 5 µL. These 5 µL were added to 15 µL ice chilled Gibson-Mastermix (Gibson et al., 2009), containing 5x ISO-Buffer, Taq-Ligase and T5 Exonuclease. Except Phusion Polymerase (Gibson et al., 2009) we used the same amount of Q5 Polymerase for the Mastermix. The samples were immediately heated to 50°C for one hour. Afterwards, the samples were cooled for 3 minutes at room temperature and 3 minutes on ice, before they were transformed into competent E.coli.
