Team:Bielefeld-Germany/Labjournal
From 2012.igem.org
Contents |
Prologue
Starting the team
Beginning in january and february members of the former iGEM team from Bielefeld started seminars to inform interested students about synthetic biology, iGEM and the past Bielefeld projects. In March the final 2012 iGEM Bielefeld team was formed of 15 students and weekly meetings began. Our team was established and it was time to find a suitable project.
Find a project
The first weekly meeting were more like big group brainstorming and we discussed idea, which in some cases were totally different from each other. Everyone had to inform about ideas of others so that, in the end, we all could discuss together.
First project ideas were:
- the detection of multiresistent pathogens
- communication between bacteria and fungi using quorum sensing
- a bacterial hand warmer
- a possibility to detect and destroy mold fungus
- something about spontaneous combustion of hay bale
- an enzyme dispenser
For most of the ideas little information was available. For example spontaneous combustion of hay bales is probably a combination of the metabolisms of different microorganisms and fungus. After some reports in media and press about the environmental effects of steroid hormones, we decided to go for hormones. From the beginning our aim was not to detect but to degrade hormones. We found several possible ways for degradation as there are the hydrolysis of estradiol-derivates with sufatases and glucoronidases. But we thought the best way to degrade steroid hormones would be with the use of laccases. Laccases have the ability to radicalize aromatic rings and can therefore be used to degrade or polymerize a broad range of substances, such as steroid hormones, special insecticides, polycyclic aromatic carbohydrates and aromatic acids. In nature laccases are often used for degradation or polymerisation of lignin or pigments.
Molding together to a team
After we found our project idea we decided to have a get-to-know-weekend with some presentations about iGEM, important methods and ideas for human practices. We also held presentations about other possible iGEM projects to extend our horizon, as there were: e.g. RNA aptamers and magnetotactic bacteria. But the most important part of this weekend was the growing as a team. We realized that we all had one summer to work together, have fun together and most important to stand up together as a team.
Find the right
Now it was time to organize the work and find a suitable task for everyone. In a developing team a lot of different jobs have to be done, e.g.:
- finding sponsors
- communication with the public
- human practices
- wiki- and homepage-design
- modelling
- a forum for exchange of information
- a joker, who entertains the team and lifts the mood
And finally lab work began, feel free to follow us in our weekly labjournal and have a look how our labwork, results and of course problems and their solutions, evolved.
Labjournal
Woche 1
Start of our WET LAB time.
We began our Lab-time with the cultivation of Xanthomonas campestris B100 and E. coli BL21(DE3) to isolate the genomic DNA to do PCRs and purify the desired laccase ORFs. Therefore we designed forward and revers primers. The forward primers included the prefix, the T7 promotor, the RBS and the first 20 bases of the gene of interest. The reverse primers included the last 20 bases of the gene of interest, a His-tag, followed by two stop codons and the suffix. Furthermore we started making praparations for the Student Academy. The "Student Academy" is a week-lasting summer school (9th to 13th of July) with several presentations and experiments for pupils and we got the chance to take part in organizing it. The general idea for our experimental part was to give the students an understanding of the principle methods in biotechnology and synthetic biology by using fluorescent proteins, therefore we searched the partsregistry for two plasmids with different fluorescent proteins and antibiotic resistances, respectively. read more55px |