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− | <h4>Transforming E. Coli Rosetta and MG1655 for pRED/ET | + | <h4>Transforming E. Coli Rosetta and MG1655 for pRED/ET Engineering</h4> |
<em>2018/08/28</em> | <em>2018/08/28</em> | ||
<table class="table table-borderless"> | <table class="table table-borderless"> | ||
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</table> | </table> | ||
− | <h4>pRED/ET | + | <h4>pRED/ET Genome Engineering of Delta msb-B and Delta recBCD Strains</h4> |
<em>2018/08/29</em> | <em>2018/08/29</em> | ||
<table class="table table-borderless"> | <table class="table table-borderless"> | ||
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<tr> | <tr> | ||
<td>Protocol:</td> | <td>Protocol:</td> | ||
− | <td>pRED/ET engineering | + | <td> |
+ | <a href="https://static.igem.org/mediawiki/2018/b/bf/T--Munich--pRED_ET-Ecoli_Gene_Deletion_Kit.pdf.pdf" target="_blank">pRED/ET engineering</a> | ||
+ | |||
+ | </td> | ||
</tr> | </tr> | ||
<tr> | <tr> | ||
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</table> | </table> | ||
− | <h4>Transforming E. Coli DH5a to | + | <h4>Transforming E. Coli DH5a to Find a Reason for the Contamination</h4> |
<em>2018/08/30</em> | <em>2018/08/30</em> | ||
<table class="table table-borderless"> | <table class="table table-borderless"> | ||
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</table> | </table> | ||
− | <h4>Creating a | + | <h4>Creating a Selection Cassette from pSB1C3</h4> |
<em>2018/08/30</em> | <em>2018/08/30</em> | ||
<table class="table table-borderless"> | <table class="table table-borderless"> | ||
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</table> | </table> | ||
− | <h4>pRED/ET | + | <h4>pRED/ET Genome Engineering of Delta msb-B and Delta recBCD Strains</h4> |
<em>2018/09/01</em> | <em>2018/09/01</em> | ||
<table class="table table-borderless"> | <table class="table table-borderless"> | ||
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<tr> | <tr> | ||
<td>Protocol:</td> | <td>Protocol:</td> | ||
− | <td>pRED/ET engineering | + | <td><a href="https://static.igem.org/mediawiki/2018/b/bf/T--Munich--pRED_ET-Ecoli_Gene_Deletion_Kit.pdf.pdf" target="_blank">pRED/ET engineering</a></td> |
</tr> | </tr> | ||
<tr> | <tr> | ||
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</table> | </table> | ||
− | <h4>Verifying | + | <h4>Verifying Deletion Strains of E. Coli MG1655</h4> |
<em>2018/09/05</em> | <em>2018/09/05</em> | ||
<table class="table table-borderless"> | <table class="table table-borderless"> |
Latest revision as of 00:25, 18 October 2018
Transforming E. Coli Rosetta and MG1655 for pRED/ET Engineering
2018/08/28Participants: | Dominic Schwarz |
Protocol: | Electrocompetent transformation |
Notes: | Genetic engineering is planned in E. Coli Rosetta, MG1655 is E.Coli WT as backup. |
Results: | Colonies only on E. Coli MG1655 plate; No colonies on E. Coli Rosetta |
pRED/ET Genome Engineering of Delta msb-B and Delta recBCD Strains
2018/08/29Participants: | Dominic Schwarz |
Protocol: | pRED/ET engineering |
Notes: | The template for the resistance cassette for deletions was taken from a plasmid containing mRFP |
Results: | Red colonies. Elena (Advisor) and Dominic decided to repeat the experiment but to do a dpnI digest before to get rid of the template DNA. |
Transforming E. Coli DH5a to Find a Reason for the Contamination
2018/08/30Participants: | Dominic Schwarz |
Protocol: | Electrocompetent transformation |
Notes: | CAP_recBCD, CAP_msbb, psb1c3_mrfp in Dh5a |
Results: | Red colonies on all plates -> mRFP contamination |
Creating a Selection Cassette from pSB1C3
2018/08/30Participants: | Dominic Schwarz |
Protocol: | Restrition digest, PCR purification |
Notes: | DpnI |
Results: | CAP_recBCD 18ng/ul CAP_msbB 12ng/ul |
pRED/ET Genome Engineering of Delta msb-B and Delta recBCD Strains
2018/09/01Participants: | Dominic Schwarz |
Protocol: | pRED/ET engineering |
Notes: | The template for the resistance cassette for deletions was taken from a plasmid containing mRFP |
Results: | Colonies on both plates |
Verifying Deletion Strains of E. Coli MG1655
2018/09/05Participants: | Dominic Schwarz |
Protocol: | Colony PCR, Agarose gel |
Notes: | Primers: VF2, geno_msb-B_rv, geno_recBCD_rv;
Ta: 48°C
t= 1kb/min RecBCD: 1,2,3,4,5 msbB: 35,36,37,38,39 expected: RecBCD 443bp Expected: msb-B 574bp |
Results: | All 5 picked colonies were positive for the insertion of the selection cassette PIC |