Difference between revisions of "Team:Vilnius-Lithuania/Methods"
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<section class="container-fluid" style="padding: 0px; padding-top: 20px;"> | <section class="container-fluid" style="padding: 0px; padding-top: 20px;"> | ||
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| + | <!-- MethodBox --> | ||
<div class="panel panel-default" style="position: relative"> | <div class="panel panel-default" style="position: relative"> | ||
<div class="panel-heading"> | <div class="panel-heading"> | ||
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</div> | </div> | ||
</div> | </div> | ||
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| + | <div class="panel panel-default" style="position: relative"> | ||
| + | <div class="panel-heading"> | ||
| + | <a class="accordion-toggle collapsed" data-toggle="collapse" data-parent="#accordion" href="#2"> | ||
| + | <h4 class="panel-title">2. DNA electrophoresis</h4> | ||
| + | </a> | ||
| + | </div> | ||
| + | <div id="2" class="panel-collapse collapse"> | ||
| + | <div class="panel-body"> | ||
| + | <div class="row"> | ||
| + | <div class="col-md-4"> | ||
| + | <strong>Materials:</strong><br /> | ||
| + | Agarose gel<br /> | ||
| + | DNA ladder<br /> | ||
| + | 6x Loading Dye<br /> | ||
| + | 1x TAE buffer<br /> | ||
| + | </div> | ||
| + | <div class="col-md-8"> | ||
| + | <strong>Process</strong>:<br /> | ||
| + | The agarose gel is loaded into electrophoresis sytem, filled with the buffer. The DNA ladder and DNA samples are then loaded into the wells. Run the gel at 130V for 30-40 minutes. | ||
| + | </div> | ||
| + | </div> | ||
| + | </div> | ||
| + | </div> | ||
| + | </div> | ||
| + | <!-- /MethodBox --> | ||
| + | |||
| + | <!-- MethodBox --> | ||
| + | <div class="panel panel-default" style="position: relative"> | ||
| + | <div class="panel-heading"> | ||
| + | <a class="accordion-toggle collapsed" data-toggle="collapse" data-parent="#accordion" href="#3"> | ||
| + | <h4 class="panel-title">3. Transformation</h4> | ||
| + | </a> | ||
| + | </div> | ||
| + | <div id="3" class="panel-collapse collapse"> | ||
| + | <div class="panel-body"> | ||
| + | <div class="row"> | ||
| + | <div class="col-md-4"> | ||
| + | <strong>Materials:</strong><br /> | ||
| + | Competent cells<br /> | ||
| + | Ligate/plasmid DNA<br /> | ||
| + | LB medium<br /> | ||
| + | Plates with LB medium and antibiotic<br /> | ||
| + | </div> | ||
| + | <div class="col-md-8"> | ||
| + | <strong>Process</strong>:<br /> | ||
| + | In order to perform transformation, the prepared competent cells are centrifuged (2 minutes, 6000 rpm, 4ºC) and most of the supernantant is discarded, leaving about 100 μL of solution, in which cells are suspended.<br /> | ||
| + | |||
| + | These cells are mixed with 10-20 ng of ligate or plasmid DNA. The mixture is incubated on ice for half an hour and right after the eppendorf tubes are placed in a thermostat in 42ºC for 1 minute. This is why it is called heat-schock transformation.<br /> | ||
| + | |||
| + | 1 mL of LB liquid medium (without antibiotic) is added to the eppendorf tube with the mixture and grown in a shaking thermostat for an hour at 37ºC. After the tubes are pelleted by centrifuging, supernantant is discarded, leaving about 100 μL, in which cells are suspended.<br /> | ||
| + | |||
| + | Transformants are placed onto a Petri dish with LB medium and specific antibiotic. Plates are incubated in a thermostat at 37ºC for a night. | ||
| + | </div> | ||
| + | </div> | ||
| + | </div> | ||
| + | </div> | ||
| + | </div> | ||
| + | <!-- /MethodBox --> | ||
</section> | </section> | ||
Revision as of 08:59, 3 September 2015
Materials:
4 mL of LB medium
Antibiotic
Transformed bacteria
4 mL of LB medium
Antibiotic
Transformed bacteria
Process:
Transformed bacteria, which contain a plasmid with a target DNA, is placed into laboratory tube with 4 ml of liquid LB medium and specific antibiotic. Bacteria are then placed into the shaker during the night at 37ºC. For the plasmid DNA extraction we used GeneJet Plasmid Miniprep Kit, according to manufacterer's instructions (pdf file).
Transformed bacteria, which contain a plasmid with a target DNA, is placed into laboratory tube with 4 ml of liquid LB medium and specific antibiotic. Bacteria are then placed into the shaker during the night at 37ºC. For the plasmid DNA extraction we used GeneJet Plasmid Miniprep Kit, according to manufacterer's instructions (pdf file).
Materials:
Agarose gel
DNA ladder
6x Loading Dye
1x TAE buffer
Agarose gel
DNA ladder
6x Loading Dye
1x TAE buffer
Process:
The agarose gel is loaded into electrophoresis sytem, filled with the buffer. The DNA ladder and DNA samples are then loaded into the wells. Run the gel at 130V for 30-40 minutes.
The agarose gel is loaded into electrophoresis sytem, filled with the buffer. The DNA ladder and DNA samples are then loaded into the wells. Run the gel at 130V for 30-40 minutes.
Materials:
Competent cells
Ligate/plasmid DNA
LB medium
Plates with LB medium and antibiotic
Competent cells
Ligate/plasmid DNA
LB medium
Plates with LB medium and antibiotic
Process:
In order to perform transformation, the prepared competent cells are centrifuged (2 minutes, 6000 rpm, 4ºC) and most of the supernantant is discarded, leaving about 100 μL of solution, in which cells are suspended.
These cells are mixed with 10-20 ng of ligate or plasmid DNA. The mixture is incubated on ice for half an hour and right after the eppendorf tubes are placed in a thermostat in 42ºC for 1 minute. This is why it is called heat-schock transformation.
1 mL of LB liquid medium (without antibiotic) is added to the eppendorf tube with the mixture and grown in a shaking thermostat for an hour at 37ºC. After the tubes are pelleted by centrifuging, supernantant is discarded, leaving about 100 μL, in which cells are suspended.
Transformants are placed onto a Petri dish with LB medium and specific antibiotic. Plates are incubated in a thermostat at 37ºC for a night.
In order to perform transformation, the prepared competent cells are centrifuged (2 minutes, 6000 rpm, 4ºC) and most of the supernantant is discarded, leaving about 100 μL of solution, in which cells are suspended.
These cells are mixed with 10-20 ng of ligate or plasmid DNA. The mixture is incubated on ice for half an hour and right after the eppendorf tubes are placed in a thermostat in 42ºC for 1 minute. This is why it is called heat-schock transformation.
1 mL of LB liquid medium (without antibiotic) is added to the eppendorf tube with the mixture and grown in a shaking thermostat for an hour at 37ºC. After the tubes are pelleted by centrifuging, supernantant is discarded, leaving about 100 μL, in which cells are suspended.
Transformants are placed onto a Petri dish with LB medium and specific antibiotic. Plates are incubated in a thermostat at 37ºC for a night.