Team:Poznan-BioInf/Book

From 2013.igem.org

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<h4>July.</h4>
<h4>July.</h4>
<h5>5th-6th week</h5>
<h5>5th-6th week</h5>
-
 
+
<p>
-
We shake off from the shock.
+
We're shaking off from the shock.
We are still trying to make an order at the biotechnological companies, so.. we are  
We are still trying to make an order at the biotechnological companies, so.. we are  
waiting for the reply from distributors.
waiting for the reply from distributors.
-
+
</p>
<h5>7th week</h5>
<h5>7th week</h5>
 +
<p>
We are still trying to make an order at the biotechnological companies, so.. we are
We are still trying to make an order at the biotechnological companies, so.. we are
gathering the signatures and forcing the offices of administration.
gathering the signatures and forcing the offices of administration.
-
+
</p>
<h5>8th week</h5>
<h5>8th week</h5>
 +
<p>
We are still waiting...
We are still waiting...
-
 
+
</p>
<h4>August.</h5>
<h4>August.</h5>
<h5>9th-10th week</h5>
<h5>9th-10th week</h5>
 +
<p>
We're done with waiting.
We're done with waiting.
Just kidding.
Just kidding.
-
We feel more like administrative labours than scientists.. - not kidding.
+
We feel more like office workers and lawyers than scientists.. - not kidding.
 +
</p>
<h5>11th-12th week</h5>
<h5>11th-12th week</h5>
-
We've receive the first part (one third) of our order of lab equipments.
+
<p>
-
We are seeing the light in the end of the tunnel, yay!
+
We've received the first part (one third) of our order of lab equipments.
-
+
We are seeing the light in the end of the tunnel, yay!<br>
Now, we could calmly put everything into designing our oligos and synthetic genes.
Now, we could calmly put everything into designing our oligos and synthetic genes.
-
We could start to planning the oligos not until we were certain, that we will get the second tranche of government funds.
+
We could not start to planning the oligos until we'd been certain we would get the second tranche of the government funds.
-
+
<p>
<h4>Semptember.</h5>
<h4>Semptember.</h5>
<h5>11 week</h5>
<h5>11 week</h5>
-
 
+
<p>
This week we've isolated the chromosome E. coli strain DH5alpha. From bacterial chromosome we want to pull out:
This week we've isolated the chromosome E. coli strain DH5alpha. From bacterial chromosome we want to pull out:
-
1. arabinose promoter
+
<br> 1. arabinose promoter
-
2. rhamnose promoter
+
<br> 2. rhamnose promoter
-
3. melibiose promoter
+
<br> 3. melibiose promoter
-
4. xylose promoter
+
<br> 4. xylose promoter
Continously we are designing of our constructs. (redirection)
Continously we are designing of our constructs. (redirection)
-
+
</p>
<h5>12 week</h5>
<h5>12 week</h5>
-
We received the first part of our oligos.
+
<p> We've received the first part of our oligos.
-
We were ably to make the PCR of our promoters, backbones with proper resistances.
+
We are able to make the PCR of our promoters & backbones with proper resistances.
-
Okey, a lot of PCR reaction with various primers. We wanted to be sure that reaction will go well, because
+
Okay, a lot of PCRs with various primers. We want to be sure that reactions go well.
-
A lot of agarose gel, as well. And photos, a lot of agarose gel photos.
+
A lot of agarose gel. And photos, a lot of agarose gel photos.
-
We are making the PCR form the AddGene plasmid, which we've ordered. On this plasmids we have:
+
We are making the PCR form the AddGene's plasmids, we've prevoiusly ordered. On this plasmids we have:
-
1. phiC31 integrase
+
<br> 1. phiC31 integrase
-
2. TP901 integrase
+
<br> 2. TP901 integrase
-
3. Bxb1 integrase
+
<br> 3. Bxb1 integrase
-
4. arabinose promoter
+
<br> 4. arabinose promoter
-
+
</p>
<h5>13 week</h5>
<h5>13 week</h5>
-
We've received the second part of oligos and synthetic genes.
+
 
 +
<p> We've received the second part of oligos and synthetic genes.
We are able to make the PCR reaction of fluorescent proteins: BFP, GFP and mRFP of our design, optimize for E. coli bacterium with three
We are able to make the PCR reaction of fluorescent proteins: BFP, GFP and mRFP of our design, optimize for E. coli bacterium with three
different tags, which should speed up the degradation of the proteins.
different tags, which should speed up the degradation of the proteins.
-
+
</p>
<h5>14 week</h5>
<h5>14 week</h5>
-
Let's start the Gibson assembly!
+
<p> Let's start the Gibson assembly!
Protocol you can find here.
Protocol you can find here.
In the beginning we use the Gibson assembly kit and the Gibson assembly master mix. We've achieved nothing.  
In the beginning we use the Gibson assembly kit and the Gibson assembly master mix. We've achieved nothing.  
-
+
</p>

Revision as of 01:10, 5 October 2013

Poznan-BioInf
Poznan-BioInf
iGEM

Home

Lab book.

Prologue.

October 2012. Weronika came back from the iGEM 2012 Regional Jamborees. After a series of Poznan University of Technology Bioinformatics Students' Research Group meetings concerning synthetic biology Poznan-BioInf came into being.

Cold, cold November. We've participated in "Generation of the Future" programme organized by the Ministry of Science and Higher Education for students needing financial support to take up a challenge in an international contest. And we're waiting...
...and waiting...
and waaaaaiting...
and at the end of April 2013 we've received decision that we are granted 200 000 zlotys.

May. We've officially signed the funding agreement and we're waiting for approval. Unfortunately, two thirds of our team are working on end-of-term exams and Bachelor's theses so... we received BioBricks and we're waiting for decision that we can administer our funds. That month We are looking for wet lab instructor and place, where we could spend summer. We are going to have a meeting with one of our professor, who we are going to ask about help. Finally, we've been sent to PhD Przemyslaw Nuc, who has agreed to join our team.

And then came June. We are still waiting for the agreement's acceptation. We've started to transform E. coli with Biobricks form Parts Registry to test the efficiency of our strain and our protocols. Since now we are working on borrowed laboratory equipments. During the tests we're looking for a suitable GFP. From now on we start to working with BBa_E0040, which exhibits bright green fluorescence.

June.

1st-4th week

We've started to trying to equip our lab. Because we study on two universities: Poznan University of Technology (where we officially belong) and Adam Mickiewicz University, we had some problems with the administration. On Poznan University of Technology there is no wet laboratory specialized at microbiological research. That's why we are forced to work on Adam Mickiewicz University.

Problems have started to rise. Due to Polish law we can't make any order as fast as we think and as we would like to. Every single one of our orders needs to be signed by four various officials. What is more, we are obliged to contact three various manufacturers or distributors of every product/service to get pricings of their products. Unfortunately to us, the holidays begin so we're going to encounter some serious trouble with making appointments.

July.

5th-6th week

We're shaking off from the shock. We are still trying to make an order at the biotechnological companies, so.. we are waiting for the reply from distributors.

7th week

We are still trying to make an order at the biotechnological companies, so.. we are gathering the signatures and forcing the offices of administration.

8th week

We are still waiting...

August.

9th-10th week

We're done with waiting. Just kidding. We feel more like office workers and lawyers than scientists.. - not kidding.

11th-12th week

We've received the first part (one third) of our order of lab equipments. We are seeing the light in the end of the tunnel, yay!
Now, we could calmly put everything into designing our oligos and synthetic genes. We could not start to planning the oligos until we'd been certain we would get the second tranche of the government funds.

Semptember.

11 week

This week we've isolated the chromosome E. coli strain DH5alpha. From bacterial chromosome we want to pull out:
1. arabinose promoter
2. rhamnose promoter
3. melibiose promoter
4. xylose promoter Continously we are designing of our constructs. (redirection)

12 week

We've received the first part of our oligos. We are able to make the PCR of our promoters & backbones with proper resistances. Okay, a lot of PCRs with various primers. We want to be sure that reactions go well. A lot of agarose gel. And photos, a lot of agarose gel photos. We are making the PCR form the AddGene's plasmids, we've prevoiusly ordered. On this plasmids we have:
1. phiC31 integrase
2. TP901 integrase
3. Bxb1 integrase
4. arabinose promoter

13 week

We've received the second part of oligos and synthetic genes. We are able to make the PCR reaction of fluorescent proteins: BFP, GFP and mRFP of our design, optimize for E. coli bacterium with three different tags, which should speed up the degradation of the proteins.

14 week

Let's start the Gibson assembly! Protocol you can find here. In the beginning we use the Gibson assembly kit and the Gibson assembly master mix. We've achieved nothing.

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