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| <ul class="art-menu"> | | <ul class="art-menu"> |
- | <li><a href="https://2009.igem.org/Team:Freiburg_bioware" class="active"><span | + | <li><a class="active" |
| + | href="https://2009.igem.org/Team:Freiburg_bioware"><span |
| class="l"></span><span class="r"></span><span | | class="l"></span><span class="r"></span><span |
| class="t">Home</span></a></li> | | class="t">Home</span></a></li> |
- | <li><a href="#"><span class="l"></span><span | + | <li><a href="https://2009.igem.org/Team:Freiburg_bioware/Team"><span |
- | class="r"></span><span class="t">The Team</span></a>
| + | class="l"></span><span class="r"></span><span |
| + | class="t">The Team</span></a> |
| <ul> | | <ul> |
- | <li><a | + | <li><a href="a href="https://2009.igem.org/Team:Freiburg_bioware/Team">Overview</a></li> |
- | href="https://2009.igem.org/Team:Freiburg_bioware/Team">Overview</a></li>
| + | <li><a href="a href="https://2009.igem.org/Team:Freiburg_bioware/Team/Portraits">Photos</a></li> |
- | <li><a href="#">Fotos</a></li> | + | |
| </ul> | | </ul> |
| </li> | | </li> |
- | <li><a href="#"><span class="l"></span><span | + | <li><a href="https://2009.igem.org/Team:Freiburg_bioware/Project"><span class="l"></span><span |
| class="r"></span><span class="t">The | | class="r"></span><span class="t">The |
- | Project</span></a></li> | + | Project</span></a><ul> |
- | <li><a href="#"><span class="l"></span><span
| + | <li><a |
- | class="r"></span><span class="t">Parts</span></a>
| + | href="https://2009.igem.org/Team:Freiburg_bioware/Project#Summary">Summary</a> |
| + | </li> |
| + | <li><a |
| + | href="https://2009.igem.org/Team:Freiburg_bioware/Project#Subprojects">Subprojects</a></li> |
| + | <li><a |
| + | href="https://2009.igem.org/Team:Freiburg_bioware/Project#Highlights">Highlights</a></li> |
| + | </ul></li> |
| + | <li><a |
| + | href="https://2009.igem.org/Team:Freiburg_bioware/Human_Practice"><span |
| + | class="l"></span><span class="r"></span><span |
| + | class="t">Human |
| + | Practice</span></a> |
| <ul> | | <ul> |
- | <li><a href="#">1</a> | + | <li><a href="#">D'oh! Something's missing here.</a> |
| <ul> | | <ul> |
| + | <li><a href="#">1</a> </li> |
| <li><a href="#">2</a> </li> | | <li><a href="#">2</a> </li> |
| <li><a href="#">3</a> </li> | | <li><a href="#">3</a> </li> |
- | <li><a href="#">4</a> </li>
| |
| </ul> | | </ul> |
| </li> | | </li> |
| + | <li><a href="#">4</a></li> |
| <li><a href="#">5</a></li> | | <li><a href="#">5</a></li> |
- | <li><a href="#">6</a></li>
| |
| </ul> | | </ul> |
| </li> | | </li> |
| <li><a href="https://2009.igem.org/Team:Freiburg_bioware/Notebook"><span class="l"></span><span | | <li><a href="https://2009.igem.org/Team:Freiburg_bioware/Notebook"><span class="l"></span><span |
| class="r"></span><span class="t">Notebook</span></a></li> | | class="r"></span><span class="t">Notebook</span></a></li> |
| + | <li><a |
| + | href="https://2009.igem.org/Team:Freiburg_bioware/Collaboration"><span |
| + | class="l"></span><span class="r"></span><span |
| + | class="t">Collaboration</span></a></li> |
| </ul> | | </ul> |
| </div> | | </div> |
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| <div class="art-Post-inner"> | | <div class="art-Post-inner"> |
| <div class="art-PostMetadataHeader"> | | <div class="art-PostMetadataHeader"> |
- | <h2 class="art-PostHeaderIcon-wrapper">May<span | + | <h2 style="border-bottom: none;" class="art-PostHeaderIcon-wrapper"> <img |
- | class="art-PostHeader"></span> </h2> | + | src="https://static.igem.org/mediawiki/2009/2/2a/Freiburg09_Post_tanne_2.png" |
| + | alt="" style="width: 28px; height: 25px;" /> May |
| + | <span class="art-PostHeader"></span> </h2> |
| </div> | | </div> |
- | <div style="text-align: center;" class="art-PostContent"> | + | <div class="art-PostContent"> |
| + | <div style="text-align: center;"></div> |
| <br /> | | <br /> |
| + | <h3>02.05 13-20.30o'clock, Rüdiger</h3> |
| + | <br /> |
| + | datamining and investigation about DNA und FOKI. Paper Miller07, |
| + | Wah1998.<br /> |
| + | 3d analysis and pictures taken from pymol.<br /> |
| + | Alignment of 2BamHI and 2FOKI to get DNA in proper position. However it |
| + | is still not perfekt, <br /> |
| + | but gives a reasonable insight into distances we need for the linker |
| + | and where we can position the oligo |
| <div style="text-align: left;"> | | <div style="text-align: left;"> |
- | | + | <table style="text-align: left; width: 633px; height: 76px;" |
- | <b>UNDER CONSTRUCTION</b><br><br> | + | border="0" cellpadding="0" cellspacing="2"> |
- | | + | <tbody> |
- | <h3>02.05 13-20.30o'clock, Rüdiger</h3>
| + | <tr> |
- | <br>
| + | <td><img |
- | datamining and investigation about DNA und FOKI. Paper Miller07, Wah1998.<br>
| + | src="https://static.igem.org/mediawiki/2009/3/3a/Freiburg09_truncated_2fokI%2BBamHIdna.JPG" |
- | 3d analysis and pictures taken from pymol.<br>
| + | name="Figure 1: this is the truncated catalytically active fokI(dimer) bound to DNA. Pink residues are the catalytic ones." |
- | Alignment of 2BamHI and 2FOKI to get DNA in proper position. However it is still not perfekt, <br>
| + | height="250" width="370" /><br /> |
- | but gives a reasonable insight into distances we need for the linker and where we can position the oligos.<br>
| + | Figure 1: this is the truncated catalytically active fokI(dimer) bound |
- | | + | to DNA. Pink residues are the catalytic ones.</td> |
- | <table>
| + | <td><img |
- | | + | src="https://static.igem.org/mediawiki/2009/e/e3/Freiburg09_gesamtkonstrukt.jpg" |
- | | + | name="Figure 2: Like this could be the completed construct. You see the FOKIdomains as in fig.1 combined with 2streptavidin proteins that bind to biotin." |
- | <tr> | + | height="300" width="300" /><br /> |
- | <td align="center"><img src="https://static.igem.org/mediawiki/2009/3/3a/Freiburg09_truncated_2fokI%2BBamHIdna.JPG" name="Figure 1: this is the truncated catalytically active fokI(dimer) bound to DNA. Pink residues are the catalytic ones." width="370" height="250" /> | + | Figure 2: Like this could be the completed construct. You see the |
- | <br> | + | FOKIdomains as in fig.1 combined with 2streptavidin proteins that bind |
- | Figure 1: this is the truncated catalytically active fokI(dimer) bound to DNA. Pink residues are the catalytic ones.</td> | + | to biotin.</td> |
- | | + | </tr> |
- | <td align="center"><img src="https://static.igem.org/mediawiki/2009/e/e3/Freiburg09_gesamtkonstrukt.jpg" name="Figure 2: Like this could be the completed construct. You see the FOKIdomains as in fig.1 combined with 2streptavidin proteins that bind to biotin." width="300" height="300" /> | + | <tr> |
- | <br> | + | <td><img |
- | Figure 2: Like this could be the completed construct. You see the FOKIdomains as in fig.1 combined with 2streptavidin proteins that bind to biotin.</td> | + | src="https://static.igem.org/mediawiki/2009/e/ed/Freiburg09_truncated_2fokIBamHIdna_insight3.JPG" |
- | </tr> | + | name="Scheme 1: cut through from the side to make dna accessibility visible. If we add a linker from below(in this picture it is the top) the indicated base would be a good place." |
- | | + | height="240" width="400" /><br /> |
- | <tr> | + | Scheme 3: cut through from the side to make dna accessibility visible. |
- | <td align="center"><img src="https://static.igem.org/mediawiki/2009/e/ed/Freiburg09_truncated_2fokIBamHIdna_insight3.JPG" name="Scheme 1: cut through from the side to make dna accessibility visible. If we add a linker from below(in this picture it is the top) the indicated base would be a good place." width="400" height="240" /> | + | If we add a linker from below(in this picture it is the top) the |
- | <br> | + | indicated base would be a good place.</td> |
- | Scheme 3: cut through from the side to make dna accessibility visible. If we add a linker from below(in this picture it is the top) the indicated base would be a good place.</td> | + | <td><img |
- | | + | src="https://static.igem.org/mediawiki/2009/e/ef/Freiburg09_truncated_2fokIBamHIdna_insight2.JPG" |
- | <td align="center"><img src="https://static.igem.org/mediawiki/2009/e/ef/Freiburg09_truncated_2fokIBamHIdna_insight2.JPG" name="Scheme 4: cut through from below to make dna accessibility visible. If we add a linker from below the indicated base would be a good place." width="370" height="215" /> | + | name="Scheme 4: cut through from below to make dna accessibility visible. If we add a linker from below the indicated base would be a good place." |
- | <br> | + | height="215" width="370" /><br /> |
- | Scheme 4: cut through from below to make dna accessibility visible. If we add a linker from below the indicated base would be a good place.</td> | + | Scheme 4: cut through from below to make dna accessibility visible. If |
- | </tr> | + | we add a linker from below the indicated base would be a good place.</td> |
- | | + | </tr> |
- | <tr>
| + | </tbody> |
- | <td align="center"><img src="Image:Freiburg09_truncated_2fokIBamHIdna_insight1.JPG|none|thumb|Schema 5: Here the sites where FokI dimer cuts the DNA(white lines)|400x400px]]</td>
| + | |
- | | + | |
- | <td align="center"><img src="Image:Freiburg09_schema_oligos.JPG|none|thumb|Schema 6: Scheme that shows the bases of blue and red DNA strands counted down from the cutting site. Red strand would be the "oligo-strand". Yellow spot are suggested places to add a linker(biotin) - in case we add one from below|400x400px]]</td>
| + | |
- | </tr>
| + | |
| </table> | | </table> |
- | | + | </div> |
- | <h3> 05th may, 11-13o'clock Rüdiger</h3> | + | <br /> |
- | Sponsoringmeeting with Timo, Anika, Rüdiger<br> | + | <h3>05th may, 11-13o'clock Rüdiger</h3> |
- | <br> | + | Sponsoringmeeting with Timo, Anika, Rüdiger<br /> |
- | to lazy to translate already taken notes....<br> | + | <br /> |
- | <br> | + | to lazy to translate already taken notes....<br /> |
- | Uni-interne zeitschriften zuspammen<br> | + | <br /> |
- | -nachwuchsförderung<br> | + | Uni-interne zeitschriften zuspammen<br /> |
- | -lernen in der praxis<br> | + | -nachwuchsförderung<br /> |
- | -kooperatives lernen<br> | + | -lernen in der praxis<br /> |
- | -gruppenmanagement<br> | + | -kooperatives lernen<br /> |
- | firmenzeitschriften finden und zuspammen<br> | + | -gruppenmanagement<br /> |
- | Sponsoren tour<br> | + | firmenzeitschriften finden und zuspammen<br /> |
- | fernsehen??!<br> | + | Sponsoren tour<br /> |
- | radio<br> | + | fernsehen??!<br /> |
- | Mentorenprogramm<br> | + | radio<br /> |
- | <br> | + | Mentorenprogramm<br /> |
- | to do:<br> | + | <br /> |
- | argumentenliste (schleimig)<br> | + | to do:<br /> |
- | -ziele<br> | + | argumentenliste (schleimig)<br /> |
- | -selbstständig arbeiten<br> | + | -ziele<br /> |
- | -eigenes projekt von planung bis zur vollendung, sowas gibt es sonst nirgends. Einblick in zukunft unseres <br>Forscherlebens.<br> | + | -selbstständig arbeiten<br /> |
- | neues universelles werkzeug für synthetische biologen: soll laboralltag revolutionieren.<br> | + | -eigenes projekt von planung bis zur vollendung, sowas gibt es sonst |
- | 2Projekte: <br> | + | nirgends. Einblick in zukunft unseres <br /> |
- | Entwicklung eines universellen Schneidewerkzeuges: Man könnte es mit einem Schraubenzieher vergleichen, <br> | + | Forscherlebens.<br /> |
- | auf den man alle arten von Bits aufsetzen kann. Jede Art von Schraube ist mit einem einzigen ,statt, <br> | + | neues universelles werkzeug für synthetische biologen: soll |
- | wie bisher mit hunderten verschiedenen Schraubenziehern herausdrehbar.<br> | + | laboralltag revolutionieren.<br /> |
- | Es soll neue opensource Software für iGEM entwickelt werden, das die komplete Arbeit mit den BiobrickTM <br>Standard Parts in einer einzigen Anwendung zusammenführt. Dies beinhaltet das Suchen und runterladen der <br> | + | 2Projekte: <br /> |
- | Sequenzen, sowie die Zusammenstellung und Bearbeitung, bis hin zur Veröffentlichung der Sequenzen in Form eines<br> neuen Biobrick Parts.<br> | + | Entwicklung eines universellen Schneidewerkzeuges: Man könnte |
- | Man kann sich das wie Lego basteln vorstellen: Beispielsweise man möchte ein Haus aus Lego bauen. <br>Dazu sucht man sich alle benötigten Steine zusammen. Aber bevor man anfängt wild drauf los zu basteln, <br>zieht man das Programm zu Rate und spielt alle Varianten am Computer vorher durch. Das Programm zeigt einem <br>dabei mittels verständlicher Grafiken, was machbar und sinnvoll ist und druckt am Ende eine fertige Bauanleitung aus.<br> Und da das Programm der Open-source Idee verpflichtet ist, kommen alle Anleitung für alle zur freien<br> Verfügung ins WWW.<br> | + | es mit einem Schraubenzieher vergleichen, <br /> |
- | -programm<br><br> | + | auf den man alle arten von Bits aufsetzen kann. Jede Art von Schraube |
- | | + | ist mit einem einzigen ,statt, <br /> |
- | <h3> 05th may, 17o'clock Rüdiger</h3> | + | wie bisher mit hunderten verschiedenen Schraubenziehern herausdrehbar.<br /> |
- | 17o'clock, Meeting the Captain(Igloi) with Dieter and Rüdiger. | + | Es soll neue opensource Software für iGEM entwickelt werden, |
- | Captain tells us about how to link PNA with Protein via Ni/Co and His tag. | + | das die komplete Arbeit mit den BiobrickTM <br /> |
| + | Standard Parts in einer einzigen Anwendung zusammenführt. Dies |
| + | beinhaltet das Suchen und runterladen der <br /> |
| + | Sequenzen, sowie die Zusammenstellung und Bearbeitung, bis hin zur |
| + | Veröffentlichung der Sequenzen in Form eines<br /> |
| + | neuen Biobrick Parts.<br /> |
| + | Man kann sich das wie Lego basteln vorstellen: Beispielsweise man |
| + | möchte ein Haus aus Lego bauen. <br /> |
| + | Dazu sucht man sich alle benötigten Steine zusammen. Aber |
| + | bevor man anfängt wild drauf los zu basteln, <br /> |
| + | zieht man das Programm zu Rate und spielt alle Varianten am Computer |
| + | vorher durch. Das Programm zeigt einem <br /> |
| + | dabei mittels verständlicher Grafiken, was machbar und |
| + | sinnvoll ist und druckt am Ende eine fertige Bauanleitung aus.<br /> |
| + | Und da das Programm der Open-source Idee verpflichtet ist, kommen alle |
| + | Anleitung für alle zur freien<br /> |
| + | Verfügung ins WWW.<br /> |
| + | -programm<br /> |
| + | <br /> |
| + | <h3> 05th may, 17o'clock Rüdiger</h3> |
| + | 17o'clock, Meeting the Captain(Igloi) with Dieter and Rüdiger. |
| + | Captain tells us about how to link PNA with Protein via Ni/Co and His |
| + | tag. |
| same could be applied to link ologo and protein. | | same could be applied to link ologo and protein. |
- | dna needs to hybridize with around 30 bases oligo to properly build up double helix. | + | dna needs to hybridize with around 30 bases oligo to properly build up |
- | | + | double helix. |
- | <h3>07th may, 14-18o'clock Rüdiger</h3> | + | <h3>07th may, 14-18o'clock Rüdiger</h3> |
- | Dicussing FokI Sequence and further strategy with Laura, Gerrit Dieter and Kristian.<br> | + | Dicussing FokI Sequence and further strategy with Laura, Gerrit Dieter |
- | <br> | + | and Kristian.<br /> |
- | Companys to buy Genes from:<br> | + | <br /> |
- | -Geneart<br> | + | Companys to buy Genes from:<br /> |
- | -Mr.gene(low budget version without support)<br> | + | -Geneart<br /> |
- | -itelichon or sth like that<br> | + | -Mr.gene(low budget version without support)<br /> |
- | -DNA 2.0 (expensive but can demand adequate features of vector) <br> | + | -itelichon or sth like that<br /> |
- | <br> | + | -DNA 2.0 (expensive but can demand adequate features of vector) <br /> |
- | Glenn research Bioscience offers modified nucleotides for our oligos<br> | + | <br /> |
- | <br> | + | Glenn research Bioscience offers modified nucleotides for our oligos<br /> |
- | <br> | + | <br /> |
- | Vektor we should create/order now:<br> | + | <br /> |
- | *must not contain IGEM restriction sites<br> | + | Vektor we should create/order now:<br /> |
- | *1FokI, active cleavage sitewe need to check literature about that. <br> | + | *must not contain IGEM restriction sites<br /> |
- | Possible experiment with original cys containg fokI: <br> | + | *1FokI, active cleavage sitewe need to check literature about that. <br /> |
- | add iodoacetamide to it and look if it gets acetylated and if it still cleaves.<br> | + | Possible experiment with original cys containg fokI: <br /> |
- | *1FokI without cleavage Aminoacids<br> | + | add iodoacetamide to it and look if it gets acetylated and if it still |
- | *replacing cys by ser (first <br> | + | cleaves.<br /> |
- | <br> | + | *1FokI without cleavage Aminoacids<br /> |
- | <br> | + | *replacing cys by ser (first <br /> |
- | Possible Tags (will be investigated later in more detail):<br> | + | <br /> |
- | *Fluoreszin & Digoxigenin ? coupled to oligo<br> | + | <br /> |
- | *Lipocalin can bind to these specufically<br> | + | Possible Tags (will be investigated later in more detail):<br /> |
- | *does the Captain have Ni/Co for Oligo synthesis?<br> | + | *Fluoreszin & Digoxigenin ? coupled to oligo<br /> |
- | *or maybe Bannwarth ? ?<br> | + | *Lipocalin can bind to these specufically<br /> |
- | <br> | + | *does the Captain have Ni/Co for Oligo synthesis?<br /> |
- | Program for Vector handling: Gentle<br> | + | *or maybe Bannwarth ? ?<br /> |
- | | + | <br /> |
| + | Program for Vector handling: Gentle<br /> |
| <h3>08th may, 17.15-18.30o'clock Caro</h3> | | <h3>08th may, 17.15-18.30o'clock Caro</h3> |
- | Dicussing RAG1/RAG2 DNA cleavage mechanism with Caro, Manu, Gerrit, Hannes, Kristian, Cristoph.<br> | + | Dicussing RAG1/RAG2 DNA cleavage mechanism with Caro, Manu, Gerrit, |
- | <br> | + | Hannes, Kristian, Cristoph.<br /> |
- | | + | <br /> |
- | Question discussed:<br> | + | Question discussed:<br /> |
- | * Which kind and how many domains have RAG1/2?<br> | + | * Which kind and how many domains have RAG1/2?<br /> |
- | * What are the cleavage mechanims and the interaction of theese domains?<br> | + | * What are the cleavage mechanims and the interaction of theese domains?<br /> |
- | *What is the essential part of theese proteins and what can be eliminated?<br> | + | *What is the essential part of theese proteins and what can be |
- | | + | eliminated?<br /> |
- | <b>Next meeting for RAG1/RAG2 and Recommbineering group: Monday, 11.may, 17.30 at kristians lab</b><br> | + | <b>Next meeting for RAG1/RAG2 and Recommbineering group: Monday, |
- | | + | 11.may, 17.30 at kristians lab</b><br /> |
| <h3>08th may, 13:30-19:30o'clock Laura</h3> | | <h3>08th may, 13:30-19:30o'clock Laura</h3> |
- | Planning the design for two vectors including one different FokI-heterodimer each with Rüdiger, Dieter and Laura<br> | + | Planning the design for two vectors including one different |
- | <br> | + | FokI-heterodimer each with Rüdiger, Dieter and Laura<br /> |
- | Procedures for both vectors:<br> | + | <br /> |
- | *extract coding region of Fok from the restriction-modification genes of the chromosomal DNA of Flavobacterium okeanokoites [http://www.ncbi.nlm.nih.gov/nuccore/148723?ordinalpos=1&itool=EntrezSystem2.PEntrez.Sequence.Sequence_ResultsPanel.Sequence_RVDocSum F.okeanokoites fokIR and fokIM genes]<br> | + | Procedures for both vectors:<br /> |
- | *delete the first 1158 nucleotides/386 aa (recognition domain) <br> | + | *extract coding region of Fok from the restriction-modification genes |
- | *switch Cystein 541/463-465 to Ser (TGT->TCT)<br><br> | + | of the chromosomal DNA of Flavobacterium okeanokoites |
- | Modifications of the single vectors to introduce heterodimeric modifications according to [[Media:Miller_J,_Rebar_E_Nature_biotech_2007_25_778.pdf]]:<br><br> | + | [http://www.ncbi.nlm.nih.gov/nuccore/148723?ordinalpos=1&itool=EntrezSystem2.PEntrez.Sequence.Sequence_ResultsPanel.Sequence_RVDocSum |
- | Modifications of the first vector (catalytic active heterodimer) <br> | + | F.okeanokoites fokIR and fokIM genes]<br /> |
| + | *delete the first 1158 nucleotides/386 aa (recognition domain) <br /> |
| + | *switch Cystein 541/463-465 to Ser (TGT->TCT)<br /> |
| + | <br /> |
| + | Modifications of the single vectors to introduce heterodimeric |
| + | modifications according to |
| + | [[Media:Miller_J,_Rebar_E_Nature_biotech_2007_25_778.pdf‎]]:<br /> |
| + | <br /> |
| + | Modifications of the first vector (catalytic active heterodimer) <br /> |
| -heterodimeric aminio acids | | -heterodimeric aminio acids |
- | *switch Glutamate 490/310-312 to Lysin (GAA->AAA)<br> | + | *switch Glutamate 490/310-312 to Lysin (GAA->AAA)<br /> |
- | *switch isoleucin 538/454-456 to Lysin (ATC->AAA)<br> | + | *switch isoleucin 538/454-456 to Lysin (ATC->AAA)<br /> |
- | <br> | + | <br /> |
- | Modifications of the second vector (catalytic inactive heterodimer) <br> | + | Modifications of the second vector (catalytic inactive heterodimer) <br /> |
| -heterodimeric amino acids | | -heterodimeric amino acids |
- | *switch Glutamin 486/298-300 to Glutamate (CAA->GAA)<br> | + | *switch Glutamin 486/298-300 to Glutamate (CAA->GAA)<br /> |
- | *switch Isoleucin 499/337-339 to Leucin (ATC->CTG)<br> | + | *switch Isoleucin 499/337-339 to Leucin (ATC->CTG)<br /> |
| -catalytic amino acids | | -catalytic amino acids |
- | *switch Aspartate 450/190-192 to Alanin (GAC->GCG)<br> | + | *switch Aspartate 450/190-192 to Alanin (GAC->GCG)<br /> |
- | *switch Aspartate 467/243-245 to Alanin (GAT->GCG)<br> | + | *switch Aspartate 467/243-245 to Alanin (GAT->GCG)<br /> |
- | <br> | + | <br /> |
| Annotations: | | Annotations: |
- | *The notation e.g. for Cystein 541/463-465 means the amino acid 541 in literature which correspond to the codons 463-465 in our vector. <br> | + | *The notation e.g. for Cystein 541/463-465 means the amino acid 541 in |
- | *For exchanging the amino acids we used the Codon usage table in E.coli from Hénaut and Danchin. [http://www.faculty.ucr.edu/~mmaduro/codonusage/codontable.htm E.coli Codon Usage]<br><br> | + | literature which correspond to the codons 463-465 in our vector. <br /> |
- | <b>Next meeting: Monday, 11th may, 16pm at kristians lab</b><br> | + | *For exchanging the amino acids we used the Codon usage table in E.coli |
- | | + | from Hénaut and Danchin. |
| + | [http://www.faculty.ucr.edu/~mmaduro/codonusage/codontable.htm E.coli |
| + | Codon Usage]<br /> |
| + | <br /> |
| + | <b>Next meeting: Monday, 11th may, 16pm at kristians lab</b><br /> |
| <h3>11th may, 17.30-19.30o'clock Max</h3> | | <h3>11th may, 17.30-19.30o'clock Max</h3> |
- | Attendees: Hannes, Caro, Manuel, Gerrit, Christoph, Max<br> | + | Attendees: Hannes, Caro, Manuel, Gerrit, Christoph, Max<br /> |
- | <b>RAG:</b> | + | <b>RAG:</b> * <b>Discussion about different domains.</b> |
- | * <b>Discussion about different domains.</b> | + | **If in RAG1 R855 and K856 are exchanged there is no hairpin but still |
- | **If in RAG1 R855 and K856 are exchanged there is no hairpin but still nicking.<br> | + | nicking.<br /> |
- | * RAG1: - cleavage active sites: D600,D708,E962 provides metalbinding function and ion -induced hydroxy-cleavage.<br> | + | * RAG1: - cleavage active sites: D600,D708,E962 provides metalbinding |
- | *RAG2: -The core is characterised by a six repeats of a kelch motif(50 residues each) <br> | + | function and ion -induced hydroxy-cleavage.<br /> |
- | - each repead forms a four-stranded twisted antiparallel beta-sheet(six bladed propeller). This structure takes part in protein protein binding.<br> | + | *RAG2: -The core is characterised by a six repeats of a kelch motif(50 |
- | - T490 phosphorylation site<br> | + | residues each) <br /> |
- | - aa 352-410 acidic portion<br> | + | - each repead forms a four-stranded twisted antiparallel beta-sheet(six |
- | -aa 420-480 is a Cys-His rich reagion similar to homodomains of zink fingers <br> | + | bladed propeller). This structure takes part in protein protein binding.<br /> |
- | -R73A, K118A/K119A Hairpin-opening <br> | + | - T490 phosphorylation site<br /> |
- | - RAG2 binds RAG1 and DNA <br> | + | - aa 352-410 acidic portion<br /> |
- | | + | -aa 420-480 is a Cys-His rich reagion similar to homodomains of zink |
- | | + | fingers <br /> |
- | * <b>What can be taken away from the protein so that it still works?</b> | + | -R73A, K118A/K119A Hairpin-opening <br /> |
- | Large parts can be deleted without loosing recombination activity. | + | - RAG2 binds RAG1 and DNA <br /> |
- | The full length of mouse RAG1 is 1040 amino acids. Aminoacids 384-1008 are required. | + | * <b>What can be taken away from the protein so that it still |
- | Mouse RAG2 has about 527 aa. Only the first 383(387)are required. | + | works?</b> |
- | In presence of Mn2+ RAG1/2 efficiently cuts an RSS(recombination signal sequence) in a DNA fragment to yield blunt 5´ phosphorylated signal ends and hairpin coding ends that retain the full coding sequence. | + | Large parts can be deleted without loosing recombination activity. The |
- | * RAG may be quite difficult to be made suitable for our purpose. | + | full length of mouse RAG1 is 1040 amino acids. Aminoacids 384-1008 are |
- | * We decided to look for another suiting enzyme just in case RAG turns out as not realizable. | + | required. |
- | <br> | + | Mouse RAG2 has about 527 aa. Only the first 383(387)are required. In |
- | <b> Next meeting: Thursday, 05/14/09, 12.30 @ Zoo-Café</b><br> | + | presence of Mn2+ RAG1/2 efficiently cuts an RSS(recombination signal |
- | | + | sequence) in a DNA fragment to yield blunt 5´ phosphorylated |
| + | signal |
| + | ends and hairpin coding ends that retain the full coding sequence. * |
| + | RAG may be quite difficult to be made suitable for our purpose. |
| + | * We decided to look for another suiting enzyme just in case RAG turns |
| + | out as not realizable. |
| + | <br /> |
| + | <b> Next meeting: Thursday, 05/14/09, 12.30 @ Zoo-Café</b><br /> |
| <h3>11th may, 16:00-20:30o'clock Laura</h3> | | <h3>11th may, 16:00-20:30o'clock Laura</h3> |
- | Planning the design for two vectors with Rüdiger, Dieter and Laura<br> | + | Planning the design for two vectors with Rüdiger, Dieter and |
- | <br> | + | Laura<br /> |
- | Execution of the planned modifications with the program Gentle<br> | + | <br /> |
- | To avoid restriction sites of the restriction enzymes used by iGEM:<br> | + | Execution of the planned modifications with the program Gentle<br /> |
- | *switch Isoleucin 109-111 to Isoleucin (ATT->ATC)<br> | + | To avoid restriction sites of the restriction enzymes used by iGEM:<br /> |
- | *switch Alanine 520-522 to Alanine (GCC->GCG)<br><br> | + | *switch Isoleucin 109-111 to Isoleucin (ATT->ATC)<br /> |
- | sequences of the completely edited active FOKI heterodimer:<br> | + | *switch Alanine 520-522 to Alanine (GCC->GCG)<br /> |
- | -amino acid sequence: | + | <br /> |
- | KSELEEKKSELRHKLKYVPHEYIELIEIARNSTQDRILEMKVMEFFMKVYGYRGKHLGGSRKPDGAIYTVGSPIDYGVIVDTKAYSGGYNLPIGQADEMQRYVKENQTRNKHINPNEWWKVYPSSVTEFKFLFVSGHFKGNYKAQLTRLNHKTNSNGAVLSVEELLIGGEMIKAGTLTLEEVRRKFNNGEINF<br> | + | sequences of the completely edited active FOKI heterodimer:<br /> |
| + | -amino |
| + | acid sequence: |
| + | KSELEEKKSELRHKLKYVPHEYIELIEIARNSTQDRILEMKVMEFFMKVYGYRGKHLGGSRKPDGAIYTVGSPIDYGVIVDTKAYSGGYNLPIGQADEMQRYVKENQTRNKHINPNEWWKVYPSSVTEFKFLFVSGHFKGNYKAQLTRLNHKTNSNGAVLSVEELLIGGEMIKAGTLTLEEVRRKFNNGEINF<br /> |
| -nucleotide sequence: | | -nucleotide sequence: |
- | AAAAGTGAACTGGAGGAGAAGAAATCTGAACTTCGTCATAAATTGAAATATGTGCCTCATGAATATATTGAATTAATTGAAATTGCCAGAAATTCCACTCAGGATAGAATCCTTGAAATGAAGGTAATGGAATTTTTTATGAAAGTTTATGGATATAGAGGTAAACATTTGGGTGGATCAAGGAAACCGGACGGAGCAATTTATACTGTCGGATCTCCTATTGATTACGGTGTGATCGTGGATACTAAAGCTTATAGCGGAGGTTATAATCTGCCAATTGGCCAAGCAGATGAAATGCAACGATATGTCAAAGAAAATCAAACACGAAACAAACATATCAACCCTAATGAATGGTGGAAAGTCTATCCATCTTCTGTAACGGAATTTAAGTTTTTATTTGTGAGTGGTCACTTTAAAGGAAACTACAAAGCTCAGCTTACACGATTAAATCATAAAACTAATTCTAATGGAGCTGTTCTTAGTGTAGAAGAGCTTTTAATTGGTGGAGAAATGATTAAAGCGGGCACATTAACCTTAGAGGAAGTGAGACGGAAATTTAATAACGGCGAGATAAACTTT<br> | + | AAAAGTGAACTGGAGGAGAAGAAATCTGAACTTCGTCATAAATTGAAATATGTGCCTCATGAATATATTGAATTAATTGAAATTGCCAGAAATTCCACTCAGGATAGAATCCTTGAAATGAAGGTAATGGAATTTTTTATGAAAGTTTATGGATATAGAGGTAAACATTTGGGTGGATCAAGGAAACCGGACGGAGCAATTTATACTGTCGGATCTCCTATTGATTACGGTGTGATCGTGGATACTAAAGCTTATAGCGGAGGTTATAATCTGCCAATTGGCCAAGCAGATGAAATGCAACGATATGTCAAAGAAAATCAAACACGAAACAAACATATCAACCCTAATGAATGGTGGAAAGTCTATCCATCTTCTGTAACGGAATTTAAGTTTTTATTTGTGAGTGGTCACTTTAAAGGAAACTACAAAGCTCAGCTTACACGATTAAATCATAAAACTAATTCTAATGGAGCTGTTCTTAGTGTAGAAGAGCTTTTAATTGGTGGAGAAATGATTAAAGCGGGCACATTAACCTTAGAGGAAGTGAGACGGAAATTTAATAACGGCGAGATAAACTTT<br /> |
- | | + | |
| sequences ot the completely edited inactive FOKI heterodimer: | | sequences ot the completely edited inactive FOKI heterodimer: |
- | -amino acid sequence:<br> | + | -amino acid sequence:<br /> |
- | KSELEEKKSELRHKLKYVPHEYIELIEIARNSTQDRILEMKVMEFFMKVYGYRGKHLGGSRKPDGAIYTVGSPIDYGVIVDTKAYSGGYNLPIGQADEMQRYVKENQTRNKHINPNEWWKVYPSSVTEFKFLFVSGHFKGNYKAQLTRLNHKTNSNGAVLSVEELLIGGEMIKAGTLTLEEVRRKFNNGEINF<br> | + | KSELEEKKSELRHKLKYVPHEYIELIEIARNSTQDRILEMKVMEFFMKVYGYRGKHLGGSRKPDGAIYTVGSPIDYGVIVDTKAYSGGYNLPIGQADEMQRYVKENQTRNKHINPNEWWKVYPSSVTEFKFLFVSGHFKGNYKAQLTRLNHKTNSNGAVLSVEELLIGGEMIKAGTLTLEEVRRKFNNGEINF<br /> |
| -nucleotide sequence: | | -nucleotide sequence: |
- | AAAAGTGAACTGGAGGAGAAGAAATCTGAACTTCGTCATAAATTGAAATATGTGCCTCATGAATATATTGAATTAATTGAAATTGCCAGAAATTCCACTCAGGATAGAATCCTTGAAATGAAGGTAATGGAATTTTTTATGAAAGTTTATGGATATAGAGGTAAACATTTGGGTGGATCAAGGAAACCGGCGGGAGCAATTTATACTGTCGGATCTCCTATTGATTACGGTGTGATCGTGGCGACTAAAGCTTATAGCGGAGGTTATAATCTGCCAATTGGCCAAGCAGATGAAATGGAACGATATGTCGAAGAAAATCAAACACGAAACAAACATCTGAACCCTAATGAATGGTGGAAAGTCTATCCATCTTCTGTAACGGAATTTAAGTTTTTATTTGTGAGTGGTCACTTTAAAGGAAACTACAAAGCTCAGCTTACACGATTAAATCATATCACTAATTCTAATGGAGCTGTTCTTAGTGTAGAAGAGCTTTTAATTGGTGGAGAAATGATTAAAGCGGGCACATTAACCTTAGAGGAAGTGAGACGGAAATTTAATAACGGCGAGATAAACTTT<br><br> | + | AAAAGTGAACTGGAGGAGAAGAAATCTGAACTTCGTCATAAATTGAAATATGTGCCTCATGAATATATTGAATTAATTGAAATTGCCAGAAATTCCACTCAGGATAGAATCCTTGAAATGAAGGTAATGGAATTTTTTATGAAAGTTTATGGATATAGAGGTAAACATTTGGGTGGATCAAGGAAACCGGCGGGAGCAATTTATACTGTCGGATCTCCTATTGATTACGGTGTGATCGTGGCGACTAAAGCTTATAGCGGAGGTTATAATCTGCCAATTGGCCAAGCAGATGAAATGGAACGATATGTCGAAGAAAATCAAACACGAAACAAACATCTGAACCCTAATGAATGGTGGAAAGTCTATCCATCTTCTGTAACGGAATTTAAGTTTTTATTTGTGAGTGGTCACTTTAAAGGAAACTACAAAGCTCAGCTTACACGATTAAATCATATCACTAATTCTAATGGAGCTGTTCTTAGTGTAGAAGAGCTTTTAATTGGTGGAGAAATGATTAAAGCGGGCACATTAACCTTAGAGGAAGTGAGACGGAAATTTAATAACGGCGAGATAAACTTT<br /> |
- | Introduction of prefix and suffix according to the Fusion Protein (Freiburg)Biobrick assembly standard<br> | + | <br /> |
| + | Introduction of prefix and suffix according to the Fusion Protein |
| + | (Freiburg)Biobrick assembly standard<br /> |
| [[Image:Fusion part.JPG|none|thumb|400x400px]] | | [[Image:Fusion part.JPG|none|thumb|400x400px]] |
- | <br> | + | <br /> |
- | Ask for an offer for our two vectors from "Biomatik Corporation" <br> | + | Ask for an offer for our two vectors from "Biomatik Corporation" <br /> |
- | <br> | + | <br /> |
- | | + | |
| <h3>14th May 12:30-15:00 o'clock, Hannes</h3> | | <h3>14th May 12:30-15:00 o'clock, Hannes</h3> |
- | Attendees: Hannes, Caro, Gerrit<br> | + | Attendees: Hannes, Caro, Gerrit<br /> |
- | <b>RAG</b><br> | + | <b>RAG</b><br /> |
- | - preparation of RAG-presentation for the meeting on friday <br> | + | - preparation of RAG-presentation for the meeting on friday <br /> |
- | - discussion of new ideas (AloI)<br><br> | + | - discussion of new ideas (AloI)<br /> |
- | | + | <br /> |
- | | + | |
| <h3>15th may 2009, 13:00- 16:00 o'clock Anika</h3> | | <h3>15th may 2009, 13:00- 16:00 o'clock Anika</h3> |
- | Attendees: Max, Sascha, Timo, Hannes, Dieter, Rüdiger, Laura, Julia, Caro, Paul, Gerrit, Manuel, Kristian, Anika | + | Attendees: Max, Sascha, Timo, Hannes, Dieter, Rüdiger, Laura, |
- | <br><br> | + | Julia, Caro, Paul, Gerrit, Manuel, Kristian, Anika |
- | Presentation of different subprojects<br><br> | + | <br /> |
- | - <b>FOKI</b><br> | + | <br /> |
- | genes are ordered, each vector costs approx. 344 USD, we ordered two vectors for the beginning <br><br> | + | Presentation of different subprojects<br /> |
- | - <b>homepage</b><br> | + | <br /> |
- | basis is written in html so that everybody can contribute to complete the page, everything in english, except the 'Vereinssatzung'in german<br> | + | - <b>FOKI</b><br /> |
- | authors of the subitems: <br> | + | genes are ordered, each vector costs approx. 344 USD, we ordered two |
- | Team: Caro<br> | + | vectors for the beginning <br /> |
- | Project: Rüdiger<br> | + | <br /> |
- | Publicity: Manu<br> | + | - <b>homepage</b><br /> |
- | iGEM Contest: Anika, Timo<br> | + | basis is written in html so that everybody can contribute to complete |
- | iGEM e.V.: Laura<br> | + | the page, everything in english, except the 'Vereinssatzung'in german<br /> |
- | -> send everything to Sascha<br><br> | + | authors of the subitems: <br /> |
- | - <b>software</b><br> | + | Team: Caro<br /> |
- | still looking for ideas, Java seems to be a good idea, program should run without an internt connnection, a Plug-In based, we will need some biologist testing this program<br><br> | + | Project: Rüdiger<br /> |
- | - <b>sponsoring/marketing</b><br> | + | Publicity: Manu<br /> |
- | discussion about different possibilities to find donators<br><br> | + | iGEM Contest: Anika, Timo<br /> |
- | - <b>RAG1+2</b><br> | + | iGEM e.V.: Laura<br /> |
- | group presented their plans, for the moment it seems that FOKI has the better prospect<br><br> | + | -> send everything to Sascha<br /> |
| + | <br /> |
| + | - <b>software</b><br /> |
| + | still looking for ideas, Java seems to be a good idea, program should |
| + | run without an internt connnection, a Plug-In based, we will need some |
| + | biologist testing this program<br /> |
| + | <br /> |
| + | - <b>sponsoring/marketing</b><br /> |
| + | discussion about different possibilities to find donators<br /> |
| + | <br /> |
| + | - <b>RAG1+2</b><br /> |
| + | group presented their plans, for the moment it seems that FOKI has the |
| + | better prospect<br /> |
| + | <br /> |
| <b>next meeting: Wednesday, 20th May 2009</b> | | <b>next meeting: Wednesday, 20th May 2009</b> |
- | <br><br><br><br> | + | <br /> |
| + | <br /> |
| + | <br /> |
| + | <br /> |
| <h3>20th may 2009, 11:00 o'clock ct. Anika</h3> | | <h3>20th may 2009, 11:00 o'clock ct. Anika</h3> |
- | Attendees: Imi, Laura, Caro, Christoph, Rüdiger, Sascha, Kristian, Anika<br> | + | Attendees: Imi, Laura, Caro, Christoph, Rüdiger, Sascha, |
- | Topics: <br> | + | Kristian, Anika<br /> |
- | <b>1. Vereinsbelangen</b><br> | + | Topics: <br /> |
- | Problem: If we are going to be an 'allgemeinnütziger Verein' it is prohibited to make advertising for our sponsors. On our website as well as on our T- shirts.<br> | + | <b>1. Vereinsbelangen</b><br /> |
- | Caro and Laura will go to the tax and legal advice of the u-Asta.<br> | + | Problem: If we are going to be an 'allgemeinnütziger Verein' |
- | | + | it is |
- | <b>2. Sponsoring</b><br> | + | prohibited to make advertising for our sponsors. On our website as well |
- | We are going to start posting the letters to the companies beginning of next week. There will be an extra meeting for the sponsoring group which is not arranged yet.<br> | + | as on our T- shirts.<br /> |
- | | + | Caro and Laura will go to the tax and legal advice of the u-Asta.<br /> |
- | <b>3. Plasmidconstruction</b><br> | + | <b>2. Sponsoring</b><br /> |
- | The ordered things arrivedwhich means that the laboratory work can start. The FokI group is looking for people who have time to work in the lab for cloning.<br><br> | + | We are going to start posting the letters to the companies beginning of |
| + | next week. There will be an extra meeting for the sponsoring group |
| + | which is not arranged yet.<br /> |
| + | <b>3. Plasmidconstruction</b><br /> |
| + | The ordered things arrivedwhich means that the laboratory work can |
| + | start. The FokI group is looking for people who have time to work in |
| + | the lab for cloning.<br /> |
| + | <br /> |
| One more thing: the website is going to put online on Sunday this week. | | One more thing: the website is going to put online on Sunday this week. |
- |
| |
| <h3>25th may 2009, 10:00- 17:00 o'clock Laura and Caro</h3> | | <h3>25th may 2009, 10:00- 17:00 o'clock Laura and Caro</h3> |
- | Attendees: Max, Sascha, Hannes, Gerrit, Anika, Christoph, Imi, Sonja, Caro, Laura | + | Attendees: Max, Sascha, Hannes, Gerrit, Anika, Christoph, Imi, Sonja, |
- | <br><br> | + | Caro, Laura |
- | Introduction into the lab work:<br><br> | + | <br /> |
- | Hier die Einführung auf deutsch (muss ja nicht ins richtige Wiki übernommen werden):<br> | + | <br /> |
- | Unser Laborraum: <br> | + | Introduction into the lab work:<br /> |
- | *UV-Gerät auf Kühlschrank zum Reinigen der Pipetten bei Handhabung mit elektrokompetenten Zellen<br> | + | <br /> |
- | * fertig gegossene SDS-Gele in Kühlschrank hinter unserer bench (evtl. selber gießen) <br> | + | Hier die Einführung auf deutsch (muss ja nicht ins richtige |
- | * Kopierkarte auf Annas Platz hinter unserem Laborplatz<br> | + | Wiki übernommen werden):<br /> |
- | *Zellkulturschrank (neben Zellkultur): Zellkulturflaschen zum Sterilfiltrieren (für Puffer etc.) und große Kolben<br> | + | Unser Laborraum: <br /> |
- | Messraum (EKTA-Raum?): Viva spins (Zentrifugeneinsätze bei Proteinaufzentrifugation) im oberen Schrank; Spitzen (verschiedene Größen) im unteren Schrank<br> | + | *UV-Gerät auf Kühlschrank zum Reinigen der Pipetten |
- | PCR/Gelraum (von der Tür zw. PRC-Raum und unserem Labor gesehen): <br> | + | bei Handhabung mit elektrokompetenten Zellen<br /> |
- | * Ethidiumbromidverschmutzter Bereich auf der bench <br> | + | * fertig gegossene SDS-Gele in Kühlschrank hinter unserer |
- | * Ethidiumbromid und normaler Abfall auf der bench getrennt; auch beim Ausgang an der zweiten Tür größere Abfalltonnen für EthBr (Achtung: keine Handschuhe!) und Glasbruchabfall<br> | + | bench (evtl. selber gießen) <br /> |
- | * Proteinpuffer und Comassiefärbelösungen in Regal über Tonnen<br> | + | * Kopierkarte auf Annas Platz hinter unserem Laborplatz<br /> |
- | * eigenes Fach im -80°C Kühlschrank oben; Fach für Klone und Proteine im unteren Teil 3. Spalte, 1. Zeile <br> | + | *Zellkulturschrank (neben Zellkultur): Zellkulturflaschen zum |
- | * Waage hinten rechts in der Ecke<br> | + | Sterilfiltrieren (für Puffer etc.) und große Kolben<br /> |
- | * nichtexplosive und nichtgiftige Chemikalien im Schrank auf der rechten Seite<br> | + | Messraum (EKTA-Raum?): Viva spins (Zentrifugeneinsätze bei |
- | * brennbare und explosive Substanzen im gelben Schrank an hinterer Wand<br> | + | Proteinaufzentrifugation) im oberen Schrank; Spitzen (verschiedene |
- | * häufig benutzte Chemikalien im Regal rechts daneben<br> | + | Größen) im unteren Schrank<br /> |
- | * im Abzug bestimmte Abfälle wie für Silber etc. <br> | + | PCR/Gelraum (von der Tür zw. PRC-Raum und unserem Labor |
- | * gefährliche Chemikalien in Metallschränken unter dem Abzug<br> | + | gesehen): <br /> |
- | * für pH-Einstellungen pH-Meter unter Abzug (in Liste daneben mit Datum, Name und Kalibrierwert eintragen; Elektrode wird in 3M KCl-Lösung gelagert) <br> | + | * Ethidiumbromidverschmutzter Bereich auf der bench <br /> |
- | * Zentrifugen in der Mitte des Raumes; Zentrifugengefäße im Schrank darunter<br> | + | * Ethidiumbromid und normaler Abfall auf der bench getrennt; auch beim |
- | * Laufpuffer für Gele im Schrank oberhalb der bench<br> | + | Ausgang an der zweiten Tür größere |
- | Verschiedene Gänge von Kristians Labor aus gesehen: <br> | + | Abfalltonnen für EthBr (Achtung: |
- | Links: <br> | + | keine Handschuhe!) und Glasbruchabfall<br /> |
- | * Kopierraum<br> | + | * Proteinpuffer und Comassiefärbelösungen in Regal |
- | Geradeaus: <br> | + | über Tonnen<br /> |
- | * noch links vor Laboreingang: 37°C Raum (großen Schüttler immer wieder anstellen!) <br> | + | * eigenes Fach im -80°C Kühlschrank oben; Fach |
- | *Platten zum Inkubieren ins Regal; Blotting-Papier und Schneidemaschine vor 37°C Raum<br> | + | für Klone und Proteine im unteren Teil 3. Spalte, 1. Zeile <br /> |
- | * im Labor: im Zentrifugenraum Eismaschine und große Zentrifugen; UV-Lichtraum zum Geldokumentieren und -schneiden weiter hinten, UV-Lichtkamera rechts von Raum nicht benutzen<br> | + | * Waage hinten rechts in der Ecke<br /> |
- | Rechts: <br> | + | * nichtexplosive und nichtgiftige Chemikalien im Schrank auf der |
- | *Schrank rechts mit Handschuhen, Eppis, Pipettenspitze (bei Gebrauch auf Liste bei Müller AG Strich) <br> | + | rechten Seite<br /> |
- | * Geräteraum links mit temperierbaren Shakern (Alternative zu 37°C Raum; bei Gebrauch mit post-it über Dauer der Benutzung informieren) <br> | + | * brennbare und explosive Substanzen im gelben Schrank an hinterer Wand<br /> |
- | * Biorad-Geldock auch zum Gel fotografieren (aber EthBr frei) <br> | + | * häufig benutzte Chemikalien im Regal rechts daneben<br /> |
- | Spülküche (noch links vor Laboreingang): <br>
| + | * im Abzug bestimmte Abfälle wie für Silber etc. <br /> |
- | * alle mögliche Glaswaren (Messbecher, Glaskolben etc) <br> | + | * gefährliche Chemikalien in Metallschränken unter |
- | * beim Platten Gießen Flasche mit Wasserbad beschriften; Flasche wird dann ins Wasserbad gestellt und kann nach zwei Stunden abgeholt werden<br> | + | dem Abzug<br /> |
- | *Gießraum: UV-Licht vorm Betreten ausschalten!; Petrischalen vorhanden; an der Tür verbrauchte Materialien in die Liste eintragen; nach Verlassen UV-Licht wieder anschalten<br> | + | * für pH-Einstellungen pH-Meter unter Abzug (in Liste daneben |
- | *Spezialbecken für Restagar neben Waschbecken im hinteren Bereich (mit Heißwasser auspülen und wegschütten) <br> | + | mit |
- | * daneben Feinwaagen <br> | + | Datum, Name und Kalibrierwert eintragen; Elektrode wird in 3M |
- | * Wagen für Spitzen, Eppis etc. und Wagen für Flüssigkeitsabfall zum Totautoklavieren<br> | + | KCl-Lösung gelagert) <br /> |
- | * Millipore Wasser-Anlage im mittleren Bereich: Process, ca. 1 min warten bis über mind. 18,1 MOhm, mit oberem Drehschalter Wasser einlassen<br> | + | * Zentrifugen in der Mitte des Raumes; |
- | Goßes Labor: <br>
| + | Zentrifugengefäße im Schrank darunter<br /> |
- | * SDS-Gel Scanner; oberhalb befinden sich multipler SDS Plattengießer (mighty small), Spritzfilter und Tris-Puffer<br> | + | * Laufpuffer für Gele im Schrank oberhalb der bench<br /> |
- | *Eppis, Spitzen, PCR tubes und DNA Präparations Kits etc. in großem Schrank vor Waschbecken; Falcons obendrauf<br> | + | Verschiedene Gänge von Kristians Labor aus gesehen: <br /> |
- | * Rührfische nebenWaschbecken, Zylinder unter Waschbecken<br> | + | Links: <br /> |
- | *neben Waschbecken auch Gefäßsammelstelle für Gefäße und Flüssigkeitsabfall (falls zu voll oder Gefäße zu groß, selbst Sachen in die Spülküche bringen) <br> | + | * Kopierraum<br /> |
- | * zum Sequenzieren an Christina wenden (über GATC Service; Eppis iun organgenen Boxen, im EG in den Briefkasten) <br> | + | Geradeaus: <br /> |
- | * im Kühlschrank gekühlte Feststoffe wie Antibiotika<br> | + | * noch links vor Laboreingang: 37°C Raum (großen |
- | *Autoklaviertape, Alufolie etc. auf dem Kühlschrank<br> | + | Schüttler immer wieder anstellen!) <br /> |
- | | + | *Platten zum Inkubieren ins Regal; Blotting-Papier und Schneidemaschine |
- | Further Topics: <br> | + | vor 37°C Raum<br /> |
- | | + | * im Labor: im Zentrifugenraum Eismaschine und große |
| + | Zentrifugen; |
| + | UV-Lichtraum zum Geldokumentieren und -schneiden weiter hinten, |
| + | UV-Lichtkamera rechts von Raum nicht benutzen<br /> |
| + | Rechts: <br /> |
| + | *Schrank rechts mit Handschuhen, Eppis, Pipettenspitze (bei Gebrauch |
| + | auf Liste bei Müller AG Strich) <br /> |
| + | * Geräteraum links mit temperierbaren Shakern (Alternative zu |
| + | 37°C |
| + | Raum; bei Gebrauch mit post-it über Dauer der Benutzung |
| + | informieren) <br /> |
| + | * Biorad-Geldock auch zum Gel fotografieren (aber EthBr frei) <br /> |
| + | Spülküche (noch links vor Laboreingang): <br /> |
| + | * alle mögliche Glaswaren (Messbecher, Glaskolben etc) <br /> |
| + | * beim Platten Gießen Flasche mit Wasserbad beschriften; |
| + | Flasche wird |
| + | dann ins Wasserbad gestellt und kann nach zwei Stunden abgeholt werden<br /> |
| + | *Gießraum: UV-Licht vorm Betreten ausschalten!; Petrischalen |
| + | vorhanden; |
| + | an der Tür verbrauchte Materialien in die Liste eintragen; |
| + | nach |
| + | Verlassen UV-Licht wieder anschalten<br /> |
| + | *Spezialbecken für Restagar neben Waschbecken im hinteren |
| + | Bereich (mit Heißwasser auspülen und |
| + | wegschütten) <br /> |
| + | * daneben Feinwaagen <br /> |
| + | * Wagen für Spitzen, Eppis etc. und Wagen für |
| + | Flüssigkeitsabfall zum Totautoklavieren<br /> |
| + | * Millipore Wasser-Anlage im mittleren Bereich: Process, ca. 1 min |
| + | warten bis über mind. 18,1 MOhm, mit oberem Drehschalter |
| + | Wasser |
| + | einlassen<br /> |
| + | Goßes Labor: <br /> |
| + | * SDS-Gel Scanner; oberhalb befinden sich multipler SDS |
| + | Plattengießer (mighty small), Spritzfilter und Tris-Puffer<br /> |
| + | *Eppis, Spitzen, PCR tubes und DNA Präparations Kits etc. in |
| + | großem Schrank vor Waschbecken; Falcons obendrauf<br /> |
| + | * Rührfische nebenWaschbecken, Zylinder unter Waschbecken<br /> |
| + | *neben Waschbecken auch Gefäßsammelstelle |
| + | für Gefäße und |
| + | Flüssigkeitsabfall (falls zu voll oder |
| + | Gefäße zu groß, selbst Sachen in |
| + | die Spülküche bringen) <br /> |
| + | * zum Sequenzieren an Christina wenden (über GATC Service; |
| + | Eppis iun organgenen Boxen, im EG in den Briefkasten) <br /> |
| + | * im Kühlschrank gekühlte Feststoffe wie Antibiotika<br /> |
| + | *Autoklaviertape, Alufolie etc. auf dem Kühlschrank<br /> |
| + | Further Topics: <br /> |
| * First steps: Preparation of mediums, agarplates,.... | | * First steps: Preparation of mediums, agarplates,.... |
| * Work-Plan of the week: | | * Work-Plan of the week: |
- | Tuesday: Competent cells (Sascha, Christophe)<br> | + | Tuesday: Competent cells (Sascha, Christophe)<br /> |
- | Wednesday: Inoculation (Imi)<br> | + | Wednesday: Inoculation (Imi)<br /> |
- | Thursday: VectorPrep (Laura, Caro) and Transformation (Hannes)<br> | + | Thursday: VectorPrep (Laura, Caro) and Transformation (Hannes)<br /> |
- | Friday:<br> | + | Friday:<br /> |
- | Next Week: Individual workings(Proteinexpression) of the Argonaute team and all people that want to help<br> | + | Next Week: Individual workings(Proteinexpression) of the Argonaute team |
- | --> For this please write a message to christoph<br><br> | + | and all people that want to help<br /> |
| + | --> For this please write a message to christoph<br /> |
| + | <br /> |
| Next Meeting: Monday 8th june, 11:00 in the Seminar room | | Next Meeting: Monday 8th june, 11:00 in the Seminar room |
- |
| |
| <h3>26th may 2009, 09:00- 15:00 o'clock; Christoph</h3> | | <h3>26th may 2009, 09:00- 15:00 o'clock; Christoph</h3> |
| Attendees: Max, Gerrit, Christoph, Sarah | | Attendees: Max, Gerrit, Christoph, Sarah |
- | <br><br> | + | <br /> |
- | We made about 200 aliquods of competent cells from the strands RV 308 and X blue (not so sure about which strands we exactly took... I will lock it up in the labbock!). Those can be used by all groups. | + | <br /> |
- | <br> | + | We made about 200 aliquods of competent cells from the strands RV 308 |
- | <br> | + | and X blue (not so sure about which strands we exactly took... I will |
- | | + | lock it up in the labbock!). Those can be used by all groups. |
| + | <br /> |
| + | <br /> |
| <h3>27th may 2009, 12:00- 15:00 o'clock; Hannes</h3> | | <h3>27th may 2009, 12:00- 15:00 o'clock; Hannes</h3> |
- | Attendees: Imi, Hannes<br><br> | + | Attendees: Imi, Hannes<br /> |
- | <b>Transformation</b> was done with XL1 blue and the two vectors (exact name?--> pET SUMO/ pET28a). We made a control plate with XL1 (without the plasmid) as well. Plates are grown over night at 37°C. Inoculation in LB+antibiotic has to be done tomorrow (Thursday)(growth not more than 16h) and the plasmid prep on Friday. | + | <br /> |
- | | + | <b>Transformation</b> was done with XL1 blue and the two |
| + | vectors (exact |
| + | name?--> pET SUMO/ pET28a). We made a control plate with XL1 |
| + | (without the plasmid) as well. Plates are grown over night at |
| + | 37°C. |
| + | Inoculation in LB+antibiotic has to be done tomorrow (Thursday)(growth |
| + | not more than 16h) and the plasmid prep on Friday. |
| <h3>28th may 2009, 11:00- 12:30 o'clock; Caro, Laura</h3> | | <h3>28th may 2009, 11:00- 12:30 o'clock; Caro, Laura</h3> |
- | *check of the three plates: Control is negative, plates with vectors are grown very well.<br> | + | *check of the three plates: Control is negative, plates with vectors |
- | *discussion of the expression vector of Raik Grünberg. We emailed further questions concerning the vector.<br><br> | + | are grown very well.<br /> |
- | | + | *discussion of the expression vector of Raik Grünberg. We |
| + | emailed further questions concerning the vector.<br /> |
| + | <br /> |
| <h3>28th may 2009, 18:30 - 19:00 o'clock; Hannes</h3> | | <h3>28th may 2009, 18:30 - 19:00 o'clock; Hannes</h3> |
- | *Inoculation of 2x3ml LB+Kan with a single colony of the two transformed strains (XL1+Tt and XL1+Aa). 12-16 hours growth over night.<br><br> | + | *Inoculation of |
- | | + | 2x3ml LB+Kan with a single colony of the two transformed strains |
| + | (XL1+Tt and XL1+Aa). 12-16 hours growth over night.<br /> |
| + | <br /> |
| <h3>29th may 2009, 10:30- 12:30 o'clock; Max</h3> | | <h3>29th may 2009, 10:30- 12:30 o'clock; Max</h3> |
- | Attendees: Caro, Gerrit, Hannes, Max<br> | + | Attendees: Caro, Gerrit, Hannes, Max<br /> |
- | <br>
| + | |
- | Plasmid purification of Tt and Aa with QIAprep Spin Miniprep Kit <br>
| + | |
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- | </div> | + | Plasmid purification of Tt and Aa with QIAprep Spin Miniprep Kit <br /> |
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| + | <div class="art-Footer-text"> |
| + | <p>contact: <a |
| + | href="mailto:freigem09@googlemail.com">freigem09@googlemail.com</a><br /> |
| + | </p> |
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