Meetings
From 2008.igem.org
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'''Controls for the DNA origamis'''<br> | '''Controls for the DNA origamis'''<br> | ||
* We should produce a DNA origami without NIP-coupled Oligos to check if there also a cell binding occurs (negative control)<br> | * We should produce a DNA origami without NIP-coupled Oligos to check if there also a cell binding occurs (negative control)<br> | ||
- | * To check the calculated distances between the NIP's on the origami | + | * To check the calculated distances between the NIP's on the origami, DNA-origami with fluorophores could be made. By using FRET the distance between the oligo's can be estimated.<br> |
<br> | <br> | ||
;May 23th 2008 | ;May 23th 2008 | ||
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* Integration of the TCR in the model to achieve a comparison of the sizes | * Integration of the TCR in the model to achieve a comparison of the sizes | ||
* Searching a suitable transmembraneregion for the artificial receptor | * Searching a suitable transmembraneregion for the artificial receptor | ||
- | * Calculation of costs for 10 Oligos wirh NIP coupled to the 5' or 3'-end: 3000,-US$ | + | * Calculation of costs for 10 Oligos wirh NIP coupled to the 5' or 3'-end: 3000,-US$ at uncertain coupling efficiency |
- | * => | + | * => Order presumably from PURIMEX |
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'''Ordering of NIPs'''<br> | '''Ordering of NIPs'''<br> | ||
- | Assembly of the DNA origami | + | Assembly of the DNA origami with coupled NIPs was discussed and decided: |
[[image:Freiburg08_NIP_13_06_08.jpg]] | [[image:Freiburg08_NIP_13_06_08.jpg]] | ||
- | Question: What are the exact distances between the DNA-helices? --> Rothemund <br> | + | Question: What are the exact distances between the DNA-helices/nod-points? --> Rothemund <br> |
'''The next steps'''<br> | '''The next steps'''<br> | ||
- | - searching for literature | + | - searching for literature on TCR-Clustering<br> |
- | - searching for literature | + | - searching for literature on transmembrane-helices, signal sequences<br> |
- | - planning the artificial system with antibodyfragment, transmembraneregion, splitenzymes, enzyme assay<br> | + | - planning of the artificial system with antibodyfragment, transmembraneregion, splitenzymes, enzyme assay<br> |
- | - EGFR as further | + | - EGFR as further test-system<br> |
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;Jun 16th 2008 10.00h | ;Jun 16th 2008 10.00h | ||
- | Preparation | + | Preparation of intern presentation on Tuesday |
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'''We have talked about...'''<br> | '''We have talked about...'''<br> | ||
- | - Until Friday we will order the NIP-coupled-Oligos. Consultation | + | - Until Friday we will order the NIP-coupled-Oligos. Consultation of Mahima: Philipp<br> |
- | - We should organize to get the vectors for cloning ( | + | - We should organize to get the vectors for cloning (Dinah/Christina: Vector with CMV-Promoter) --> Kathrin <br> |
- Reproduce Schamels experiment with the TCR --> appointment with Mahima<br> | - Reproduce Schamels experiment with the TCR --> appointment with Mahima<br> | ||
- Think about a cloning strategy using the BioBrick pre- and suffix <br> | - Think about a cloning strategy using the BioBrick pre- and suffix <br> | ||
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All of the sequences from Mahima arrived by now and they can be checked. A vector wiith CMV-promotor could be also saerched on the wiki 2007.<br> | All of the sequences from Mahima arrived by now and they can be checked. A vector wiith CMV-promotor could be also saerched on the wiki 2007.<br> | ||
- | '''2. | + | '''2. concentration of DNA structure'''<br> |
theoretically possible: 20 nM, maybe even 200 nM; according we need at least 2 µM to distinct between 2, 3 or 4 NIPs<br> | theoretically possible: 20 nM, maybe even 200 nM; according we need at least 2 µM to distinct between 2, 3 or 4 NIPs<br> | ||
- | '''3. DNA | + | '''3. DNA-Origami'''<br> |
* binding measurement: Origami with 4 NIP molecules and 2 fluorophores<br> | * binding measurement: Origami with 4 NIP molecules and 2 fluorophores<br> | ||
* negative control: DNA-Origami without NIP but with fluorophores<br> | * negative control: DNA-Origami without NIP but with fluorophores<br> | ||
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*wavelength 488nm and 568nm might be measured at another lab<br> | *wavelength 488nm and 568nm might be measured at another lab<br> | ||
- | '''6. in general'''<br> | + | '''6. "in general"'''<br> |
* upload more data onto the intern wiki<br> | * upload more data onto the intern wiki<br> | ||
* meet more frequently | * meet more frequently | ||
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<ul> | <ul> | ||
<li><font face="Arial">M13mp18 phage DNA was preped</font></li> | <li><font face="Arial">M13mp18 phage DNA was preped</font></li> | ||
- | <li><font face="Arial">The Oligios we ordered arrived --> A poll was made, the pool contains all the Oligos except the 10 which | + | <li><font face="Arial">The Oligios we ordered arrived --> A poll was made, the pool contains all the Oligos except of the 10 which are to be marked with NIP or fluorophor </font></li> |
<li><font face="Arial">Ca<sup>2+</sup> - Daniels experiment (making DNA-Origami 1:20 has been reproduced, but we have to check on the AFM if the Origami formed right -> AFM measurement is tomorrow.</font></li> | <li><font face="Arial">Ca<sup>2+</sup> - Daniels experiment (making DNA-Origami 1:20 has been reproduced, but we have to check on the AFM if the Origami formed right -> AFM measurement is tomorrow.</font></li> | ||
<li><font face="Arial">We have to reorder some of the Oligo</font></li> | <li><font face="Arial">We have to reorder some of the Oligo</font></li> | ||
</ul> | </ul> | ||
- | <p><font face="Arial"><b>3. We need to | + | <p><font face="Arial"><b>3. We need to solve the Origami-concentration problem</b></font></p> |
<ul> | <ul> | ||
- | <li><font face="Arial">Ca<sup>2+</sup>We could measure the calcium influx with a flourescence microscope. Therefore we have to find out which dye | + | <li><font face="Arial">Ca<sup>2+</sup>We could measure the calcium influx with a flourescence microscope. Therefore we have to find out which dye to use</font></li> |
</ul> | </ul> | ||
<p><font face="Arial"><b>4. Think about the synthetic receptor system</b></font></p> | <p><font face="Arial"><b>4. Think about the synthetic receptor system</b></font></p> | ||
<ul> | <ul> | ||
- | <li><font face="Arial">we could use a vector which already has the beta chain of the TCR coupled to the NIP fab fragment and fuse half of β-Lactamase to each of it</font></li> | + | <li><font face="Arial">we could use a vector which already has the beta-chain of the TCR coupled to the NIP fab fragment and fuse half of β-Lactamase to each of it</font></li> |
<li><font face="Arial">if the receptors get clustered by the NIP the β-Lactamase would be functional </font></li> | <li><font face="Arial">if the receptors get clustered by the NIP the β-Lactamase would be functional </font></li> | ||
</ul> | </ul> | ||
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<p> </p> | <p> </p> | ||
<br> | <br> | ||
- | <p><font face="Arial"><b> | + | <p><font face="Arial"><b> July 16th 2008 12.00h</b></font></p> |
'''Attendees:''' <br> | '''Attendees:''' <br> | ||
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<br> | <br> | ||
<br> | <br> | ||
- | ''' | + | '''July 23rd 2008 12.00h'''<br> |
<br> | <br> | ||
<span style="font-weight: bold;">Attendees</span> <br> | <span style="font-weight: bold;">Attendees</span> <br> | ||
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'''Aug. 7th 2008 ''' | '''Aug. 7th 2008 ''' | ||
- | <span style="font-weight: bold;"> | + | <span style="font-weight: bold;">Attendees:</span> <br> |
Robert Gawlik, Philipp Mappes, Normann Kilb, Sabine Jägle, | Robert Gawlik, Philipp Mappes, Normann Kilb, Sabine Jägle, | ||
Kristian Müller, Moritz Busacker.<br> | Kristian Müller, Moritz Busacker.<br> | ||
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'''Sept. 24th. 2008'''<br> | '''Sept. 24th. 2008'''<br> | ||
<br> | <br> | ||
- | -Modeling<br | + | -Modeling<br> |
-measurement of fura-stained T-and B-cells (ZBSA)<br> | -measurement of fura-stained T-and B-cells (ZBSA)<br> | ||
-AFM-measurement at IMTEK?<br> | -AFM-measurement at IMTEK?<br> | ||
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construcs: <br> | construcs: <br> | ||
<br> | <br> | ||
- | pMA - signal peptide – scFv-anti-NIP – gggs-Linker – | + | pMA - signal peptide – scFv-anti-NIP – gggs-Linker – transmembrane region(BCR/EGFR) - '''X''' – pMA<br><br> |
'''X :''' | '''X :''' | ||
* bla1(1/2 beta-Lactamase)-<br> | * bla1(1/2 beta-Lactamase)-<br> | ||
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<br> | <br> | ||
'''Next steps:''' <br> | '''Next steps:''' <br> | ||
- | 1) We want to test | + | 1) We want to test wheather the transmembrane region really is located in the membrane<br> |
- | Therefore we want to clone a | + | Therefore we want to clone a construct expressing YFP on the cytoplasmic side of the receptor.<br> |
Construct:<br> | Construct:<br> | ||
- | - | + | - singal peptide – scFv-anti-NIP – gggs-Linker – transmembrane region - split-linker - bla1 - YFP -<br> |
<br> | <br> | ||
- | 2) We also want to test | + | 2) We also want to test if we able to bring the receptors together using a NIP coupled peptide.<br> |
Therefore we need the peptides from Schamels group -> Norman will ask them.<br> | Therefore we need the peptides from Schamels group -> Norman will ask them.<br> | ||
<br> | <br> | ||
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Have to produce new Origami -> Michael and Norman<br> | Have to produce new Origami -> Michael and Norman<br> | ||
<br> | <br> | ||
- | Next meeting: Oct. 23th 2008<br> | + | <!--Next meeting: Oct. 23th 2008<br>--> |
<br> | <br> | ||
}} | }} |
Latest revision as of 01:30, 20 November 2008
_meetings
Recruitment of team
attendees How to organize the project?
attendees We have talked about...
attendees Ordering of NIPs Question: What are the exact distances between the DNA-helices/nod-points? --> Rothemund The next steps
Preparation of intern presentation on Tuesday
We have talked about... - Until Friday we will order the NIP-coupled-Oligos. Consultation of Mahima: Philipp
attendees Robert Gawlik, Philipp Mappes, Michael Kneib, Kathrin Pieper, Sabine Jägle, Kristina Brückner, Simone Weber
We have talked about... · Oligos are ordered. They should be delivered until the 10th of July. · Transmembraneregion: o Literature about the transmembraneregion o Which transmembraneregion can be used? For example EGF-R o Signalpeptide?! o Paper: Erythropoitetin Receptor Activation by a Ligand-Induced Conformation Change · synthetic transmembraneregion: o Which parts shall build the synthetic receptor?
· Vectors: o Genemaps for the Vectors o Available Vectors have to be compared to the iGEM-Systeme(Freiburg2007-WIKI) o possibly searching suitable vectors
jobs · Literature transmembraneregion/signalepeptide : Simone, Kristina, Sabine · Vectorsequences : Philipp, Kathrin, Michael · Registry on the official WIKI:Robert
attendees 1. Vectors 2. concentration of DNA structure 3. DNA-Origami
4. proof of principle: T-cell-receptor activation
5. confocal microscopy
6. "in general"
July 10th, 2008 Attendees: Simone Weber, Sabine Jägle, Kathrin Pieper, Phillip Mappes, Norman Kilb, Robert Gawlik, Daniel Hautzinger, Michael Kneib, Kristian Müller, Kristina Brückner
1. Security instruction > emergency call: 2000 2.actual state of affairs
3. We need to solve the Origami-concentration problem
4. Think about the synthetic receptor system
5. substrates for the β-Lactamase
6. Transfection Protocol
7. Positive control for the transfections
8. Searching other vectores
9. second system for multimerisation with different antibodieszweitesn
10. intracellular domain of EGF-R
July 16th 2008 12.00h Attendees: Vectors and synthetic receptor system:
1)EGFR + Single chain + one half of beta-Lactamase
2)EGFR + Single chain + second half of beta-Lactamase
3)The whole EGFR fused to the NIP fab fragment. With this construct it might be also possible to activate the receptor by adding EGF. Hence we would have a additionally positive control. But first we would have to find a readout for the activation with EGF.
Fura 2/ Indo-1:
Aug. 7th 2008 Attendees: Robert Gawlik, Philipp Mappes, Normann Kilb, Sabine Jägle, Kristian Müller, Moritz Busacker.
brochure for further information [http://tools.invitrogen.com/content/sfs/manuals/liveblazer_FRETBGLoadingKit_man.pdf brochure_liveblazer_FRETBGLoadingKit]
Aug. 28th 2008 Sept. 11th 2008
Themes: 1. CMV Promotor Sabine tried to amplificate the CMV Promotor (in the vector) -> it didn’t work! Improvements: 2. Antibodies Probably we could get some antibodies against NIP from Schamel and his group, so we could proof if our origamis have the NIP. Normally we could see the antibodies on the AFM. 3. FACS We measured the calcium influx on the FACS. 4. Fura-Loading Because the Fura stain didn´t work when we tried to measure the calcium influx at the microscope (ZBSA), we wanted to repeat the staining to see what we should change. o Again the staining didn´t work -> We have to ask Nitschke about the conditions. o We also have to order the Fura-2AM. 5. NIP binding to the cells We also repeated the binding measurement at the microscope. -> We can get the B-cells(2558Lδm/mb-1) from Schamel!
attendees organisatory Ca-measurement Wiki part-order control of DNA-Origami binding to cell-surface
Sept. 29th 2008
official wikipediasite iGEM parts
attendees:
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