Team:Goettingen/week18-1
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<b>V09_01_2: Separation assay</b><br> | <b>V09_01_2: Separation assay</b><br> | ||
<ul> | <ul> | ||
- | <li>Experiment: <br>One of our goals was to invent es protocol that allows the separation of two different fast strains using the antibiotics marker on an inserted plasmid. The plated prepared at the xx were used to test the separation assay. On these plated cultures of the strain Δ<i>tar</i> with J2006 expressing rfp (amp resistance) and the strain Δ<i>tar</i> with pSB1C3-<i>tar</i>-QC-18C were mixed 1:1 (according to the OD600) and dropped on 3% tryptone swimming agar plates containing no | + | <li>Experiment: <br>One of our goals was to invent es protocol that allows the separation of two different fast strains using the antibiotics marker on an inserted plasmid. The plated prepared at the xx were used to test the separation assay. On these plated cultures of the strain Δ<i>tar</i> with J2006 expressing rfp (amp resistance) and the strain Δ<i>tar</i> with pSB1C3-<i>tar</i>-QC-18C were mixed 1:1 (according to the OD600) and dropped on 0.3% tryptone swimming agar plates containing no antibiotic.</li> |
<li>Experimental procedure: <br> | <li>Experimental procedure: <br> | ||
- | - The agar was cut out at three different positions using a to the first mark shortened yellow Eppendorf tip respectively | + | - The agar was cut out at three different positions using a to the first mark shortened yellow Eppendorf tip respectively <br> |
- The first section was cut out at the swimming front (I), and the next two (II, III) in a line behind the first one<br> | - The first section was cut out at the swimming front (I), and the next two (II, III) in a line behind the first one<br> | ||
- The tips with the agar pieces were inserted into a glas tube filled with 1 ml LB media respectively<br> | - The tips with the agar pieces were inserted into a glas tube filled with 1 ml LB media respectively<br> |
Revision as of 18:39, 24 September 2012
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#1 Selection / Swimming - 18th WeekBack to overview
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