Team:Colombia Uniandes/ChimiJournal
From 2013.igem.org
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+ | =='''Hands at work!'''== | ||
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+ | Here you will find the overall progression of our work at the laboratory designing Chimi. | ||
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+ | ===='''18-Jun-2013'''==== | ||
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+ | Hello! Hello! Hola! Hola! | ||
+ | After we went over the project, we proceed to design our primers so we could place our order, taking into account that we are going to use Fusion PCR as our main protocol. If you want to check our primers, go to [[https://2013.igem.org/Team:Colombia_Uniandes/How_to_parts| How to: Parts]]. Our primers take around 2 weeks to arrive… sooo meanwhilee all the team started making our ''E.coli'' babies electrocompetent, so we can work with them later on. | ||
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=='''Dear Journal! :)'''== | =='''Dear Journal! :)'''== | ||
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===='''13th June 2013'''==== | ===='''13th June 2013'''==== |
Revision as of 16:20, 25 September 2013
Hands at work!
Here you will find the overall progression of our work at the laboratory designing Chimi.
18-Jun-2013
Hello! Hello! Hola! Hola! After we went over the project, we proceed to design our primers so we could place our order, taking into account that we are going to use Fusion PCR as our main protocol. If you want to check our primers, go to [How to: Parts]. Our primers take around 2 weeks to arrive… sooo meanwhilee all the team started making our E.coli babies electrocompetent, so we can work with them later on.
=='''Dear Journal! :)'''== ===='''13th June 2013'''====The first thing we did was to extract the plasmids from the iGEM plaque.
- From the 2013 kit, Plate 1, Well 19 – o
- From the 2013 kit, Plate 1, Well 2 – i
- From the 2013 kit, Plate 3, Well 17 – c
- 20 µ of miliQ water (ultra pure). Find the plate and stick the tip with water into the well, perforating the aluminum.
- Resuspend the well’s content by gentle pipetting.
- When the water has a dark red color, transfer it to a PCR eppendorf and put on ice.
We performed miniprep procedures with the GenElute HP Plasmid Miniprep kit.
This are the overall steps:
- Harvest cells.
- Resuspend cells.
- Cell lysis.
- Neutralization. Spin method:
- Prepare column.
- Load cleared lysate.
- Wash column with wash solution 1.
- Was column with wash solution 2.
- Centrifuge.
- Elute DNA.
- 5 mL of overnight culture of S. cerevisiae (in BHI medium) were centrifuged at 8500 rpm for 5 min. Discard de supernatant.
- 500 µL of Harja lysis buffer were added to each tube.
- Place 2 min at -20 °C, 1 min in water bath at 90 °C and repeat.
- Vortex 30 s.
- Add 500 µL of chloroform, vortex 2 min and centrifuge 3 min at 8500 rpm.
- Transfer the upper aqueous phase to a tube with 800 µL of chilled 100% ethanol and mix by inversion.
- Incubate for 5 min at room temperature or at 30 °C.
- Centrifuge for 5 min, 8500 rpm, and discard supernatant.
- Wash the pellet with 500 µL of ethanol (100%) by vortex. Repeat step 9.
- Dry pellets at room temperature or at 60 °C.
- Resuspend in 40 µL miliQ water.
- Competent yeast were made following the procedure mentioned before.
- We also made our first PCRs! We used primers 6 & 1 (A) and 34 & 9 (B) to extract VP16 from the Nal1 plasmid and GCR.
- Confirmation gel (2013-06-26 19 hr 16 min.jpg & 2013-06-26 19hr 15 min.jpg) with wells:
- Ladder
- PCR A
- PCR B
- Miniprep for Nal. 1