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- | <title>IGEM Panama Team</title>
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- | <li class="item3"><a
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- | href="https://2010.igem.org/Team:Panama"><span>Home</span></a></li>
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- | <li class="item4"><a
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- | href="https://2010.igem.org/Team:Panama/Team"><span>Team</span></a></li>
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- | <li class="item5"><a
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- | href="https://2010.igem.org/Team:Panama/Project"><span>Project</span></a></li>
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- | <li class="item6"><a
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- | href="https://igem.org/Team.cgi?year=2010&team_name=Panama"><span>Official
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- | Team Profile</span></a></li>
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- | <li class="item7"><a
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- | href="https://2010.igem.org/Team:Panama/Parts"><span>Parts
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- | Submitted to the Registry</span></a></li>
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- | <li class="item8"><a
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- | href="https://2010.igem.org/Team:Panama/Modeling"><span>Modeling</span></a></li>
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- | <li class="item9"><a
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- | href="https://2010.igem.org/Team:Panama/Donors"><span>Donors</span></a></li>
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- | <li class="item11"><a
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- | href="https://2010.igem.org/Team:Panama/how_to_become_a_sponsor"><span>How to become a Donors</span></a></li>
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- | </ul>
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- | </div>
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- | <img style="width: 960px; height: 259px;" alt="Team_Panama"
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- | </html>
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- | ==Notebook==
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- | ===DNA 101: Information store, replication. 26 May===
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- | * Instructor: Dr. Abby Guerra
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- | * Date: 26 May 17h00-20h00
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- | * Venue: UTP
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- | A basic refresher course on how DNA stores information in the cell, and how it is involved in cellular replication.
| + | |
- | ===DNA 102: Protein creation relationship to cellular function. 26 May===
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- | Instructor: Dr. Abby Guerra
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- | Date: 26 May 17h00-20h00
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- | Venue: UTP
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- | Introduction to how DNA drives cellular functions by creating proteins
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- | ===DNA 103: DNA modification, plasmids===
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- | Instructor: Dr. Abby Guerra
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- | Date: 26 May 17h00-20h00
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- | Venue: UTP
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- | Introduction to long tested combinant DNA techniques, the role of plasmids in bacteria, and their use as a vector for DNA modification.
| + | |
- | ===INDICASAT lecture: Drug discovery in nature===
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- | Instructor: Dr. Sergio Martinez
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- | Date: (17h00-20h00 Thursday 3rd June)
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- | Venue: INDICASAT
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- | Would be a brainstorming session as students start thinking about projects. It would be GREAT if we could take a molecule discovered by INDICASAT in coral/frogs/nature and put it in E. coli!...
| + | |
- | ===INDICASAT lecture: Innovation===
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- | Instructor: Dr. Jagannatha Rao, Director of INDICASAT
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- | Date: (17h30-20h00 Friday 4th June)
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- | Venue: INDICASAT
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- | Dr. Rao's lecture on how to innovate.
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- | ===DNA 104: BioBricks Protocol===
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- | Instructor: Sara/Patrick
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- | Date: (17h30-20h00 Monday 7th June)
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- | Venue: INDICASAT
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- | Introduction to the BrioBricks protocol
| + | |
- | ===iGEM workshop follow up: Software tools===
| + | |
- | Instructor: Patrick / Sara
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- | Date: (17h30-20h00 Monday 7th June)
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- | Venue: INDICASAT
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- | Software tools available from the workshop.
| + | |
- | ===iGEM workshop follow up: Safety, ethics===
| + | |
- | Instructor: Dr. Ricardo Lleonart
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- | Date: (17h00-20h00 9th of June)
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- | Venue: INDICASAT
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- | There is definetly a "safety considerations" requirement and we should address it early.
| + | |
- | ===Wetlab 101: Tools of the lab and their use===
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- | Instructor: Dr. Patricia Llanes
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- | Date: (17h00-20h00 9th June)
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- | Venue: INDICASAT
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- | How to handle pipettes, clean test tubes, etc.
| + | |
- | ===Wetlab 102: Let's raise a few E. coli===
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- | Instructor: Lorena Coronado and and Dr. Carmenza Spadafora
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- | Date: (17h00-20h00 11th of June)
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- | Venue: INDICASAT
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- | How does one handle E. coli?
| + | |
- | ===Wetlab 103: Let's make an E. coli that fluoresce (or some simple BioBrick project)===
| + | |
- | Instructor: INDICASAT, Dr. Carmenza Spadafora
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- | Date: (17h00-20h00 11th of June)
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- | Venue: INDICASAT
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- | We identify a simple project based on past iGEM work and do our first BioBrick protocol project. Nothing innovative, but an opportunity to practice the protocols.
| + | |
- | ===Meeting June 26===
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- | At this moment we have two ideas for develop. We are debating which idea is more feasible.
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- | Idea #1: Carlos´s team idea
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- | We want to produce Rhamnolipid in bacteria (e.coli) to use it as a biosurfactant.
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- | First we have to be sure that our idea is not the same that the idea published in the reference paper.
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- | We want to make a biobrick to produce Rh1.
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- | We have to see how we can isolate the rhamnolipid, and be sure that the translation is functional.
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- | | + | |
- | Steps to follow:
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- | 1.Amplified the Rhamnosyltransferase 1 complex from Pseudomona Auruginosa to clone the fragment. Size aprox 2.2 Kb.
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- | 2.Ligation / Transformation
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- | 3.Expression with reporter gen.
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- | 4.Isolation
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- | 5.Is the protein functional?
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- | 6.Make sure that the rhamnolipid is produced in prescence of rhamnose and fatty acid.
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- | | + | |
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- | Notes:
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- | We can see the reaction ( enzymatic measure) by spectrometry.
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- | See kind of ligation.
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- | Decided if we are going to use sticky or blond ends. (Depend on the plasmid).
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- | | + | |
- | | + | |
- | | + | |
- | But first, before the amplification we need to design our primers.
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- | | + | |
- | Primers design:
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- | | + | |
- | 1.Check the gene sequence (In GenBank, FASTA format)
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- | 2.Check the primer sequence.
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- | 3.See kind of cloning.
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- | 4.M13 tail for cleavage site.
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- | 5.Look for cleavage site inside the rhamnosyltransferase 1 gene for our restriction enzymes. We can´t cut our gene in the process.
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- | In summary the steps that we need to follow are:
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- | | + | |
- | I.Primer design
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- | II.PCR or amplification
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- | III.Cloning
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- | IV.Expression
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- | V.Sequencing
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- | | + | |
- | The most important steps are I and II. We need a good primers design and PCR if we want to have successful.
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- | Idea #2
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- | Ernesto team´s idea
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- | | + | |
- | Production of Cecropin compound. We want to produce the antibacterial cecropin compound. Naturally is produced by insects and plants.
| + | |
- | | + | |
- | We want to use Anopheles gambiae cecropin precursor. The gene is about 550 pb.
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- | | + | |
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- | The steps to follow are the same in both groups.
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- | Both groups have to design the primers, and have all the experimental design for this week.
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- | | + | |
- | 1.The sequence of the interested gene.
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- | 2.Design the primers. (50-100pb more at the begging and end of the sequence).
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- | 3.Check for cloning sites. Which plasmid we are going to use, identify the restriction enzymes.
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- | 4.Assemble the blocks. In paper assemble all the system. Promoter + Ribosomal binding site + interest gene + reporter gene + translation end site.
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- | | + | |
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- | All the design has to be on paper to analyze them and decided which idea is going to be the elected one.
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