Difference between revisions of "Team:Humboldt Berlin/Attributions"

Line 207: Line 207:
 
                                                     <tr>
 
                                                     <tr>
 
                                                       <td>ptxD</td>
 
                                                       <td>ptxD</td>
                                                         <td> <a href="https://www.ncbi.nlm.nih.gov/nuccore/AF061070">AF061070.1>Sequence</a></br>Ordered by GeneCust
+
                                                         <td> Sequence: <a href="https://www.ncbi.nlm.nih.gov/nuccore/AF061070">AF061070.1</a></br>Ordered by GeneCust
 
                                                     </tr>
 
                                                     </tr>
 
                                                     <tr>
 
                                                     <tr>

Revision as of 13:11, 15 October 2019

notebook

Attributions

Supporters

Our team accomplished great things in the project Chlamylicious over the course of this year’s iGEM competition: We adapted a toolkit for the green algae C. reinhardtii with parts for successful and easy cloning of any transcription unit, which we implemented for the expression of the PET-degrading enzyme PETase by the algae and designed a bioreactor for its cultivation under constant monitoring of all parameters. These were our greatest supporters:

  • our host laboratories Experimental Biophysics and Molecular Genetics from the Humboldt University of Berlin, who shared their infrastructure with us
  • our supervisors Prof. Dr. Schmitz-Linneweber and Prof. Dr. Hegemann
  • the principal investigator Simon Kelterborn, who guided us with his expertise in transformations of Chlamydomonas and CRISPR-aided genetic engineering
  • the biological technical assistants Heide (Biophysics lab), Conny, Thea and Irina (all Genetics lab), who enabled us to launch the wet-lab
  • computer scientist Vincent Will, who implemented the design for our website
  • Prof. Dr. Ringrose, who coached us on how to create a good scientific poster
  • electrical engineer Markus Schulz, who helped designing and wiring the electronics for our bioreactor
  • technical engineering student Alejandro Gómez Jimenez from the Technical University of Berlin, who wrote the CAD-models for all parts of our bioreactor
  • the Interdisciplinary Workshop „Matters of Activity“ of Humboldt University, who laser-cut our hardware
  • the Mechanical Workshop of the Physics Department of our university



Re-used parts from different sources

Part name source
AR Plasmid p114 (AG Hegemann)
ARS Ordered Oligos from IDT
Sequence:https://www.uniprot.org/blast/?about=A8ISJ6[1-26]&key=Signal%20peptide
AmpOri Amplified from MoClo plasmid pICH47732
Ble/Scp: Ordered Oligos from IDT
GLE Uniprot Q93WN9[1 - 28]
3xHA-Tag Ordered Oligos from IDT
His-Tag Ordered Oligos from IDT
Hyg Amplified p360 AG Hegemann
MHETase (wildtype) Kaiserslautern (C.reinhardtii)
MHETase (wildtype II) Weber,A. (E. coli)
MHETase (Mutant W397A) Weber,A. (E. coli)
Paro Amplified from p114 AG Hegemann
PETase Ordered Oligos from IDT, Codon usgae is C.reinhadtii Ordered Oligos from IDT
PETase (E. coli) Adgene's plasmid: Plasmid #112203
ptxD Sequence: AF061070.1
Ordered by GeneCust
PsaD plasmid 51 (from AG Hegemann)
PsadIntron self designed, intron designed after AR-Promoter
Rbc52 amplified from p141 pCrP2-SaCas9 (RBCS2, G), p016
RFP p42 AG Hegemann
Spec Amplificated from mplifikation from Addgene MoClo Plasmid pAGM9121
YFP Amplificated fromYFP Sequenz vom p135 pCr3-Ble2-YFP-Sp-APH Plasmid >pAGM9121
Overhang PCR: Amplification

Timeline and responsibilities

As the first team from the Humboldt University ever to form and participate in the iGEM competition we had to organize the following to establish C. reinhardtii as a chassis for synthetic biology in the iGEM community:

  • Find a professor and department able to supervise the iGEM project. As there is no course of synthetic biology taught at our university we referred to the Molecular Genetics and Biophysics lab groups.
  • Found a team of students, who were able to conduct the project research during their studies without earning credits for it. Our university so far does not offer any courses for the participation of students as an iGEM team. By June 2018 the main core of our iGEM team was brought together.
  • Brainstorm for interesting and viable SynBio projects, which took place in July 2018. Most of us had little or no prior knowledge in synthetic biology.
  • Research more on the possibilities of C. reinhardtii as a SynBio tool and familiarize ourselves with project management conducts from July-October 2018
  • Start fundraising initiatives in July 2018
  • Get part of the team started with working in the wet lab in November 2018.
  • Organize Human Practice events and possibilities of outreach to the broader public from November 2018 - October 2019.
  • Get a second lab team to finish the wet lab work from April-October 2019.