Team:Colombia Uniandes/ChimiJournal

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{{Http://2013.igem.org/Team:Colombia Uniandes/Bootstrap}}
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<div class="tabbable"> <!-- Only required for left/right tabs -->
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  <ul class="nav nav-tabs">
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    <li class="active"><a href="#tab1" data-toggle="tab">Chimi's Journal</a></li>
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    <li><a href="#tab2" data-toggle="tab">Nicko's Journal</a></li>
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=='''Hands at work!'''==
=='''Hands at work!'''==
<p align="justify">
<p align="justify">
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Today we ran PCRs for pGAL1 and mCherry. Now that we have several parts, we must have a clear understanding of our notation!
Today we ran PCRs for pGAL1 and mCherry. Now that we have several parts, we must have a clear understanding of our notation!
<ul>
<ul>
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<il>pBap2 = C</li>
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<li>pBap2 = C</li>
<li>GAL4 = D</li>
<li>GAL4 = D</li>
<li>VP16 = A</li>
<li>VP16 = A</li>
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In our quest to obtain again all our parts, we performed the following fusion PCRs: ABF1 (primers 1 & 31), GF2 (primers 17 & 31), E1GF2 (primers 15 & 31), E2G (primers 15 & 13), E3G (primers 15 & 13), E4G (primers 15 & 13).
In our quest to obtain again all our parts, we performed the following fusion PCRs: ABF1 (primers 1 & 31), GF2 (primers 17 & 31), E1GF2 (primers 15 & 31), E2G (primers 15 & 13), E3G (primers 15 & 13), E4G (primers 15 & 13).
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We also performed the transformation by TOPO cloning.<html></p>
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We also performed the transformation by TOPO cloning.
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=='''Dear Journal! :)'''==
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<html>
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<p align="justify">
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Here we will place all the information about the work we have been doing during this time, it will be named by date.
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We hope you enjoy our work and thoughts as much as we do!
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</p>
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[[File:La_foto.JPG|300px|thumb|center|Our Notebook]]
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===='''18-Jun-2013'''====
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<html>
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<p align="justify">
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Hello! Hello! Hola! Hola!
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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 </html>[https://2013.igem.org/Team:Colombia_Uniandes/How_to_parts How to: Parts].<html> 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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===='''25-Jun-2013'''====
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<html>
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So today we took our bacterial cells (Top 10) onto an LB medium (no antibiotics). We let it ON at 37 °C on the shaker. Also we prepared all the material we need for tomorrow: ddwater, 10 % glycerol, LB medium and microfuge tubes.
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</p></html>
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===='''26-Jun-2013'''====
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<html>
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<p align="justify">
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Today we are going to start preparing our cells, we inoculated in the morning and placed all our material that needs to be cold in the fridge 4 °C(ddWater and glycerol), also the centifuge rotor needs to be chilled.
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Then we just waited for the perfect OD and made our cells around 4:00pm. We made a lot!
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</p>
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We placed them in the -80, ready to start our work!!!
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</html>
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===='''2-Jul-2013'''====
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Our primers are FINALLY here and we are anxious to start working!!!
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So we made our plan(in theory)on big steps for the next weeks!:
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'''1.''' '''DNA extraction''' from ''E.coli'' and ''Cupriavidus metallidurans CH34''
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===='''September 4th, 2013'''====
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'''2. PCR'''
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  2.1 PrcnR, RBS, rcnR, stop (Amplified as one piece)
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  2.2 PrcnA,RBS
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  2.3 hoxN, stop
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'''3.''' '''Fusion PCR'''
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  3.1 PrcnA/''hoxN''
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  3.2 PrcnR,RBS,''rcnR''/PrcnA/''hoxN''
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On each PCR add 30 steps more of making gels for confirmation, again and again and again.
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===='''3-Jul-2013'''====
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<p align="justify">
<p align="justify">
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Fortunately our team member Silvia Cañas already had a DNA extraction from ''E.coli'' so she donated it to us so we could start working! Thank you Silvia! :)
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We inoculated cells with dexamethasone. The original syringe had an initial concentration of 8mg/2mL. We obtained an initial volume of 3.189*10^-2 µL, so we had to dilute first the dexamethasone: 9900 µL water + 100 µL dexametasona.</p>
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We asked for ''Cupriavidus metallidurans'' to our teacher Jenny Dussan at her lab here in the university. She is giving us the strain tomorrow morning! Thank you Jenny!
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<p align="justify">Induction experiment ON: 5 mL LB + 20 µL ampicillin + 20 µL kanamycin + 10 µL inoculum + 32 µL dexamethasone (1:1000) (inoculate ON).</p>
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This done, did the extraction of ''C.metallidurans'' and store it in the -30 °C.
 
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</p>
 
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</html>
 
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===='''4-Jul-2013'''====
 
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<html>
 
<p align="justify">
<p align="justify">
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Today we started with the 2-step PCR of PrcnR, RBS, ''rcnR'', stop (Fragment that will be called "R" from now on).
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Gel PCR: F-H-P-E1GF2-MP-E2GF-E3GF1-E3GF2-E4GF- Everything was succesful except E1GF2.</p>
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Results were negative :(
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</p>
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===='''5-Jul-2013'''====
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<html>
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<p align="justify">
<p align="justify">
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Today we repeated "R" PCR and also did ''hoxN'' with the ''Cupriavidus metallidurans'' genome. The quantities used for the reaction of ''hoxN'' are shown in the table below.  
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We digested the obtained PCRs with 5 µL Buffer CutSmart + 15 µL PCR +1 µL XbaI + 1 µL SpeI + 28 µL water (for each PCR).</p>
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Results were negative :( as we could see in our sad, SAD gel.
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</p>
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{| border="1" align="center"
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|+'''PCR reagents and amounts for one 50 ul reaction'''
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| style="text-align: center;" |Reagent
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-
| style="text-align: center;" |Amount
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|-
 
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| style="text-align: center;" |''C.metallidurans'' DNA
 
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| style="text-align: center;" |3,0 ul
 
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|-
 
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| style="text-align: center;" |Primer FW
 
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| style="text-align: center;" |2,5 ul
 
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-
|-
 
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| style="text-align: center;" |Primer RV
 
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| style="text-align: center;" |2,5 ul
 
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|-
 
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| style="text-align: center;" |DMSO
 
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| style="text-align: center;" |2,0 ul
 
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|-
 
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| style="text-align: center;" |Master Mix
 
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| style="text-align: center;" |25 ul
 
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|-
 
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| style="text-align: center;" |dH2O
 
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| style="text-align: center;" |15 ul
 
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|-
 
-
|}
 
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-
 
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===='''9-Jul-2013'''====
 
<html>
<html>
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<p align="justify">
 
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So, our PCRs are NOT working....We think our problem is the length of the primers and their constitution that could form secondary structures very VERY easily.
 
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That's why we tried a new procotol of PCR for "R" with a temperature gradient, and we tried new buffers for ''hoxN''.  Reagents and quantities are shown in the table below.
 
-
</p>
 
-
</html>
 
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{| border="1" align="center"
 
-
|+'''PCR reagents and amounts for one 50 ul reaction'''
 
-
| style="text-align: center;" |Reagent
 
-
| style="text-align: center;" |Amount
 
-
 
-
|-
 
-
| style="text-align: center;" |''Escherichia coli'' DNA
 
-
| style="text-align: center;" |2,0 ul
 
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-
|-
 
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| style="text-align: center;" |Primer FW
 
-
| style="text-align: center;" |2,5 ul
 
-
 
-
|-
 
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| style="text-align: center;" |Primer RV
 
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| style="text-align: center;" |2,5 ul
 
-
 
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|-
 
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| style="text-align: center;" |DMSO
 
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| style="text-align: center;" |2,0 ul
 
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|-
 
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| style="text-align: center;" |Master Mix
 
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| style="text-align: center;" |25 ul
 
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|-
 
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| style="text-align: center;" |dH2O
 
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| style="text-align: center;" |16 ul
 
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|-
 
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|}
 
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-
 
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We got a POSITIVE result on ''hoxN'', and POSITIVE with "R" at "low" temperatures of annealing. Here is our BEAUTIFULLL gel.
 
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{|align="center"
 
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|[[File:Gel1.jpg|300px|thumb|'''GoodNewsGEL''']]
 
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|[[File:star.jpg|100px|thumb]]
 
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|}
 
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On 5,7,8,9 we can see "R" fragment of 359bp.
 
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On 12 we can see ''hoxN'' fragment of 837bp.
 
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===='''11-Jul-2013'''====
 
-
 
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Today we did the PrcnA PCR and it didn't work out.
 
-
 
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===='''15-Jul-2013'''====
 
-
 
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We started ''hoxN'' PCR with the phusion primers, over the ''C. metallidurans'' genome, using 2-step PCR protocol.
 
-
 
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Results are negative.
 
-
 
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===='''17-Jul-2013'''====
 
-
 
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We repeated hoxN PCR with the fusion primers over the genome and PrcnA PCR with ''E.coli'' genome.
 
-
 
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Nothing worked OUT :( !!!
 
-
 
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We are going to try to do the PCR of hoxN with the phusion primers over the fragment already amplified and see, as fas as PrcnA goes...we will try a temperature ramp with a 3-step PCR protocol.
 
-
End for today :(
 
-
 
-
===='''18-Jul-2013'''====
 
-
 
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Today we did ''E. coli'' chimiocompetent cells to mRFP transformation using TransforrmAid Bacterial Transformation Kit (Thermo Scientific). We did mRFP transformation from iGEM plate.
 
-
 
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===='''19-Jul-2013'''====
 
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We have transformants!!!! Beautiful, aren´t they?
 
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[[File:IMG-20130909-00382.jpg|400px|thumb|center|Transformants]]
 
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===='''24-Jul-2013'''====
 
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<html>
 
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<p align="justify">
 
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Today we are going to do pRcnA PCR. Besides iGEM kit, we used Phusion High Fidelity PCR kit and tested  its two buffers: Phusion HF reaction Buffer and Phusion GC Reaction Buffer. We used a 2-step PCR protocol. Reagents and quantities of iGEM kit are the same we have been using until now, but reagents and quantities used for Phusion High Fidelity PCR kit are shown in the table below.
 
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</p>
 
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</html>
 
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{| border="1" align="center"
 
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|+'''PCR reagents and amounts for one 50 ul reaction'''
 
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| style="text-align: center;" |Reagent
 
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| style="text-align: center;" |Amount
 
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-
|-
 
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| style="text-align: center;" |''Escherichia coli'' DNA
 
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| style="text-align: center;" |4,0 ul
 
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|-
 
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| style="text-align: center;" |Primer FW
 
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| style="text-align: center;" |2,5 ul
 
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|-
 
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| style="text-align: center;" |Primer RV
 
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| style="text-align: center;" |2,5 ul
 
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|-
 
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| style="text-align: center;" |Buffer
 
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| style="text-align: center;" |10 ul
 
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|-
 
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| style="text-align: center;" |dNTPs
 
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| style="text-align: center;" |1,0 ul
 
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| style="text-align: center;" |DMSO
 
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| style="text-align: center;" |1,5 ul
 
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|-
 
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| style="text-align: center;" |Pol
 
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| style="text-align: center;" |0,5 ul
 
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|-
 
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| style="text-align: center;" |dH2O
 
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| style="text-align: center;" |28,3 ul
 
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|-
 
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|}
 
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===='''25-Jul-2013'''====
 
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We did ''hoxN'' PCR by using the same kits than yesterday and 2-steps protocol. However, results are negative :'(.
 
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===='''26-Jul-2013'''====
 
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<html>
 
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<p align="justify">
 
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Since we have been having troubles with PCRs, we decided to do genome extraction of our bacteria again. For this purpose we used Easy DNA Isolation Kit, Invitrogen. We followed manufacturer's instructions. We confirmed the extraction by gel electrophoresis. Genomes of ''C. metallidurans'' and new ''E.coli'' Extracted :D 
 
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</html>
 
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[[File:GelGenoma.jpg|400px|thumb|center|GenomeNewExtractionWithOUTRnase]]
 
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<html>
 
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</p>
 
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</html>
 
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*Remember you can review protocols in the section named [https://2013.igem.org/Team:Colombia_Uniandes/Protocols Protocols]
 
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===='''29-Jul-2013'''====
 
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Today we did PCR of ''hoxN'' from the new ''C. metallidurans'' genome exracted and guess what? We got ''hoxN'' a beatiful band around 600 pb :D :D. Blue arrow shows HoxN and yellow arrow shows rcnR...FAIL
 
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[[File:GelHoxN.jpg|400px|thumb|center|GelHoxN]]
 
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===='''30-Jul-2013'''====
 
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We did PCR of ''rcnR'' using the ''E. coli'' genome extracted last Friday and Phusion High Fidelity PCR kit. On the gel we got a diffuse band around 400 pb, so we could not conclude anything.
 
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===='''31-Jul-2013'''====
 
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<html>
 
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<p align="justify">
 
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We did PCR of ''pRcnA'' and ''rcnR'' again using a annealing temperature gradient between 45°C and 60° and using the two buffers: Phusion HF reaction Buffer and Phusion GC Reaction Buffer. On the gel we saw a band that corresponded to ''pRcnA'' when the annealing temperature had been around 53°C and GC buffer had been used. On the other hand, in ''rcnR'' reactions we got a band when buffer HF had been used and when annealing temperature was around 58°C.
 
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So...u CAN BARELY see them BUT THEY ARE THERE!
 
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</html>
 
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[[File:PrcnA.jpg|400px|thumb|center|Prcna,rcnR]]
 
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<html>
 
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</p>
 
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</html>
 
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===='''01-Aug-2013'''====
 
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<html>
 
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<p align="justify">
 
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Today we did ''hoxN''-''rfp'' phusion. We used Phusion High Fidelity PCR kit, Phusion HF reaction Buffer and the amounts of other reagents described below. We got our first phusion!!! What a great day :)
 
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</p>
 
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</html>
 
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{| border="1" align="center"
 
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|+'''Phusion PCR'''
 
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| style="text-align: center;" |Reagent
 
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| style="text-align: center;" |Amount
 
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| style="text-align: center;" |''rfp''  DNA     
 
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| style="text-align: center;" |2,0 ul
 
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| style="text-align: center;" |''hoxN''  DNA
 
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| style="text-align: center;" |2,0 ul
 
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| style="text-align: center;" |Primer FW
 
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| style="text-align: center;" |1,0 ul
 
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| style="text-align: center;" |Primer RV
 
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| style="text-align: center;" |1,0 ul
 
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| style="text-align: center;" |Buffer
 
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| style="text-align: center;" |4 ul
 
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| style="text-align: center;" |dNTPs
 
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| style="text-align: center;" |0,4 ul
 
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| style="text-align: center;" |DMSO
 
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| style="text-align: center;" |1,0 ul
 
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| style="text-align: center;" |Pol
 
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| style="text-align: center;" |0,2 ul
 
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| style="text-align: center;" |dH2O
 
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| style="text-align: center;" |8,4 ul
 
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[[File:hoxNRFP.jpg|400px|thumb|center|hoxNRFP fusion!]]
 
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===='''02-Aug-2013'''====
 
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Another try of PrcnR-rcnR and then again...nothing.
 
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[[File:rcnR.jpg|400px|thumb|center|rcnR]]
 
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===='''05-Aug-2013'''====
 
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Since we obtained PrcnA and HoxN, we made a Prcna-HoxN fusion and we also amplified hoxN-RFP fusion. All was obtained and we can see that in our beautifull gel :)Go guys!! The fisrt column next to the DNA ladder is HoxN-RFP fusion on the first pink arrow, on the second pink arrow there is our fusion Prcna-HoxN.
 
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[[File:Prcna_hoxN.jpg|400px|thumb|center|Prcna-HoxN and HoxN-RFP]]
 
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===='''07-Aug-2013'''====
 
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Today we decided to digest our parts with EcoRI in order to insert our parts in the backbone. Thats why first we did the digestion with EcoRI on the Backbone and also the same process with the parts. We digested for 2 hours and then desactivated the ennzymes at 80°C for 20 min. For protocol see: https://www.neb.com/products/r0101-ecori#tabselect2
 
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We then used antarctic phosphatase for the backbone for 1h. For protocol see: https://www.neb.com/protocols/1/01/01/vector-dephosphorylation-protocol
 
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Finally we let the ligation all night at room temperature.
 
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===='''09-Aug-2013'''====
 
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Today we desactivated the ligase at 80°C for 15 min and started THE TRANSFORMATION!
 
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We transformated our cells and let them in  37°C. Lets see tomorrow :)
 
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===='''10-Aug-2013'''====
 
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They were NO colonies At ALL! not even halfffffff, not even a tiny oneee!!
 
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We are repeating process on monday.
 
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===='''13-Aug-2013'''====
 
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Today we did electrocompetent cells with E.coli DH10B and we tranformed and well...hopefully we will see something tomorrow!
 
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Hopes up!
 
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===='''14-Aug-2013'''====
 
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We have some colonies! but only on HoxN-RFP fusion! We are going to leave those on ON and we are transforming Prcna-HoxN again.
 
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===='''15-Aug-2013'''====
 
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Transformation not succesfull, do it one more time!
 
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===='''16-Aug-2013'''====
 
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Transformation not succesfull, do it one more time!
 
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===='''19-Aug-2013'''====
 
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Transformation not succesfull, do it one more time!
 
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===='''20-Aug-2013'''====
 
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Tranformation succesfull!!!! :) Growing on ON!
 
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===='''21-Aug-2013'''====
 
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Miniprep DAY! :)
 
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Parts Ready!
 
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===='''23-Aug-2013'''====
 
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We are sending Prcna-HoxN and HoxN-RFP :)
 
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We are still trying to get Prcnr-rcnR so lets go!
 
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===='''24-Aug-2013'''====
 
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We tried PCR Prcnr-rcnR and IS NOT THEREEEEEEEEEEEE!
 
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Latest revision as of 06:05, 27 September 2013


Contents

Hands at work!

Here you will find the overall progression of our work at the laboratory designing Chimi.

13th June 2013

The first thing we did was to extract the plasmids from the iGEM plaque.

  1. From the 2013 kit, Plate 1, Well 19 – o
  2. From the 2013 kit, Plate 1, Well 2 – i
  3. From the 2013 kit, Plate 3, Well 17 – c

The iGEM parts were taken in order to perform an electroporation. For this, we use:

  • 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.

15th June 2013

We picked the transformant colonies.

18th June 2013

We performed miniprep procedures with the GenElute HP Plasmid Miniprep kit.

This are the overall steps:

  1. Harvest cells.
  2. Resuspend cells.
  3. Cell lysis.
  4. Neutralization.
  5. Spin method:

  6. Prepare column.
  7. Load cleared lysate.
  8. Wash column with wash solution 1.
  9. Was column with wash solution 2.
  10. Centrifuge.
  11. Elute DNA.

We did a confirmation Gel 100 V x 30 min. -> It showed 1 bond in the first two wells corresponding to Nal1 and Nal2. We succesfully extracted the Nal plasmids!

June 21st, 2013

Harju et al., “Bust n’ Grab” Protocol for Yeast Genomic DNA Extraction

  1. 5 mL of overnight culture of S. cerevisiae (in BHI medium) were centrifuged at 8500 rpm for 5 min. Discard de supernatant.
  2. 500 µL of Harju lysis buffer were added to each tube.
  3. Place 2 min at -20 °C, 1 min in water bath at 90 °C and repeat.
  4. Vortex 30 s.
  5. Add 500 µL of chloroform, vortex 2 min and centrifuge 3 min at 8500 rpm.
  6. Transfer the upper aqueous phase to a tube with 800 µL of chilled 100% ethanol and mix by inversion.
  7. Incubate for 5 min at room temperature or at 30 °C.
  8. Centrifuge for 5 min, 8500 rpm, and discard supernatant.
  9. Wash the pellet with 500 µL of ethanol (100%) by vortex. Repeat step 9.
  10. Dry pellets at room temperature or at 60 °C.
  11. Resuspend in 40 µL miliQ water.

June 26, 2013

  • We made competent yeast following the procedure mentioned before.
  • We also made our first PCRs! We used primers 6 & 1 (A) and 34 & 9 (B) to extract VP16 and GCR from the Nal1 plasmid.
  • Confirmation gel (2013-06-26 19 hr 16 min.jpg & 2013-06-26 19hr 15 min.jpg) with wells:
    1. Ladder
    2. PCR A
    3. PCR B
    4. Miniprep for Nal. 1

A = VP16
B = GCR

Construct.jpg

June 27, 2013

We repeated the PCR for A and used lambda phage DNA for carrier DNA. We also tried extracting yeast genome using a modified Harju “Bust n’ Grab” protocol using three parallel methods:

  • Method “H” used the regular lysis buffer.
  • Method “C” used the following lysis buffer: 3% Triton, 100 mM LiCl, 10 mM Tris-HCl, 1 mM EDTA, 100 mM NaAc.
  • Method “O” used the following lysis buffer: 2% triton, 1& SDS, 10 mM tris-HCl, 1 mM EDTA, 100 mM LiCl.

Conformation gel was run with wells:

  1. Ladder
  2. PCR A (repeated)
  3. Carrier lambda PCR
  4. Method C
  5. Method H
  6. Method O

The genome extraction still isn't working! :(

We then ran a fusion PCR with GAL4 and VP16 (A and B). These were the PCR conditions:

  • 1st PCR --> 2-step PCR
    Cycle steps
    1. Initial denaturation (98 °C, 30 s)
    2. 15 cycles (98 °C, 10 s; 72 °C, 35 s)
    3. Final extension (72 °C, 5 min)
    4. Hold (4 °C, indefinite time)
  • 2nd PCR --> 2-step PCR (add primers)
    Cycle steps
    1. Initial denaturation (98 °C, 30 s)
    2. 35 cycles (98 °C, 10 s; 72 °C, 35 s)
    3. Final extension (72 °C, 10 min)
    4. Hold (4 °C, indefinite time)
  • July 2nd, 2013

    Still trying to successfully extract the yeast genome! This time we tried an alternate method where we used two different solutions to break the cell wall:

    • Solution I: Glucose 50 mM, EDTA pH 8 10 mM, Tris-HCl pH 8 25 mM (esterilized) + Zymolyase
    • Solution II: NaOH 0.2 N, SPS 1%
    • The rest of the protocol was taken from GenElute DNA Kit from Sigma-Aldrich.

    July 3rd, 2013

    The genome extraction was better, but it's mostly degraded DNA! We still have to improve the protocol.

    July 5th, 2013

    We're still improving our genome extraction protocol. This time we're trying 4 variations to break the cell wall
    We're varying the incubation of both solutions, the one that comes with the kit (Proteinase K + Lysis buffer) and the zymolyase solution we previously used. The four variations were as follows.

    • A: Zymolyase for ½ h at 37 °C
    • B: Zymolyase for ½ h at 37 °C, then protease K + lysis T ½ h at 55 °C
    • C: Zymolyase for ½ h at 37 °C, then protease K + lysis T ½ h at 37 °C
    • D: Regular GenElute Genome extraction protocol

    The rest of the steps were done following the instructions from the GenElute Genome extraction protocol.


    We ran a gel in this order: WM, A, B, C, D.
    Both B and C gave results, with C giving better yields! We're keeping the C protocol and we're happy we can start extracting parts from the yeast genome!

    We performed PCRs for BAP2, GAL4, yeast terminator and pGAL1. These were the conditions:
    PCR fusion 2 steps*, with process 3 at 72 °C for 45 s

      *
    1. 98 °C, 1 min
    2. 98 °C, 10 s
    3. 72 °C, 45 s
    4. Steps 2 and 3 x 35

    5. 72 °C, 10 min
    6. 4 °C

    July 9th, 2013

    Today we ran PCRs for pGAL1 and mCherry. Now that we have several parts, we must have a clear understanding of our notation!

    • pBap2 = C
    • GAL4 = D
    • VP16 = A
    • GCR = B
    • TER = F
    • VP16 + GCR = AB
    • pBAP2 + GAL4 = CD
    • AB + TER = ABF

    July 18th, 2013

    Today we ran PCRs for the following fusions: F1 = TER-GCR, with primers 31 & 35; F2 = TER – mCherry, with primers 31 & 33. We also amplified E = pGAL1, using primers 13 & 15.

    July 19th, 2013

    Today we amplified F2 that we obtained yesterday.

    July 22nd, 2013

    Today we tried to fuse C-D using primers 19 and 5, TER-GCR using primers 31 and 35 and TER-mCherry using primers 31 and 33. After 15 PCR cycles, we added the primers.

    July 24th, 2013

    Today we extracted the terminator from the yeast genome (F1 and F2) and pGAL1 from miniprep (E). We also did PCRs to fuse again our big parts: pBAP2 – GAL4 – VP16 – GCR (CD-AB) (primers 19 & 34) and pGAL1 – mCherry (E-G) (primers 32 & 15).
    At the moment, this is our progress!:

    Progress chart.jpg

    August 5th, 2013

    Things are advancing at a fast pace! Today we did miniprep to obtain PUC19!

    August 6th, 2013

    After doing a confirmation gel, C and CD are no longer with us! So we need to repeat them!

    August 16th, 2013

    Still no C nor D, so we did PCRs again with different methods to obtain C1, C2, D1 and D2.

    September 3rd, 2013

    Today we confirmed what we will be sending for the regional competition!
    qBlocks (200 ng):

    • Terminator (114486764) (F1 & F2)
    • 3X UAS-pGAL1 (114486765) (E2)
    • 6X UAS-pGAL1 (114486766) (E3)
    • 9X UAS-pGAL1 (114486767) (E4)

    Final volume: (40 µL)
    Final concentration: 5 ng/µL

    In our quest to obtain again all our parts, we performed the following fusion PCRs: ABF1 (primers 1 & 31), GF2 (primers 17 & 31), E1GF2 (primers 15 & 31), E2G (primers 15 & 13), E3G (primers 15 & 13), E4G (primers 15 & 13).

    We also performed the transformation by TOPO cloning.

    September 4th, 2013

    <p align="justify"> We inoculated cells with dexamethasone. The original syringe had an initial concentration of 8mg/2mL. We obtained an initial volume of 3.189*10^-2 µL, so we had to dilute first the dexamethasone: 9900 µL water + 100 µL dexametasona.</p>

    <p align="justify">Induction experiment ON: 5 mL LB + 20 µL ampicillin + 20 µL kanamycin + 10 µL inoculum + 32 µL dexamethasone (1:1000) (inoculate ON).</p>

    <p align="justify"> Gel PCR: F-H-P-E1GF2-MP-E2GF-E3GF1-E3GF2-E4GF- Everything was succesful except E1GF2.</p> <p align="justify"> We digested the obtained PCRs with 5 µL Buffer CutSmart + 15 µL PCR +1 µL XbaI + 1 µL SpeI + 28 µL water (for each PCR).</p>

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