Difference between revisions of "Team:CSU Fort Collins/Experiments"
Line 98: | Line 98: | ||
<div class="panel" id="panel1"> | <div class="panel" id="panel1"> | ||
<h3>Materials</h3> | <h3>Materials</h3> | ||
− | <ul> <li> | + | <ul> <li>Agarose</li> |
− | <li> | + | <li>1X TAE Buffer</li> |
− | <li> | + | <li>Parafilm</li> |
+ | <li>Electrophoresis chamber and power source</li> | ||
+ | <li>SYBR Green</li> | ||
+ | <li>Loading Dye</li> | ||
+ | <li>DNA Ladder</li> | ||
+ | <li>PCR Samples</li> | ||
</ul> | </ul> | ||
<h3 >Procedure</h3> | <h3 >Procedure</h3> |
Revision as of 00:19, 29 August 2015
Click the panels to slide down or up
Protocols
Plasmid Construction
Materials
Material | Amount |
---|---|
Something | ul |
Something | ul |
Something | ul |
Procedure
- First
- Second
- Third
Gel Electrophoresis
Materials
- Agarose
- 1X TAE Buffer
- Parafilm
- Electrophoresis chamber and power source
- SYBR Green
- Loading Dye
- DNA Ladder
- PCR Samples
Procedure
- Using a balance, mass out 0.5 gram of agarose (for 1% gel, for 2% mass out 1.0 gram). Mix this with 50 mL of TAE 1X Buffer.
- Microwave the mixture, mixing by swirling intermittently, until all the agarose is dissolved and the mixture is homogeneous and clear (about 2 minutes).
- Pour the mixture into a gel plate and insert a correctly-sized comb (8, 10, etc. lanes). Allow to cool and solidify on the benchtop.
- Mix your samples on a piece of parafilm. Use 10 μL of the appropriate DNA Ladder (1 kb, 100 bp, 2 log, etc.) combined with 1 μL SYBR Green/DMSO in the first lane. For all samples, mix 10 μl of sample and 2 μL of SYBR Green/Dye Mixture.
- Place gel in tray into the gel electrophoresis apparatus - wells should be close to the negative (conventionally black) end. Fill apparatus with 1X TAE until the gel is completely submerged. Do not overfill - there is a guide sticker on the apparatus which marks the max fill line.
- Load 10 μL of each sample into the appropriate wells.
- Connect wiring and run gel electrophoresis at 110 V for 1 hour.
- Analyze gel in UV light and see if samples match the expected size using the ladder as a guide.
Experiments
Growth on Fatty Acids
Materials
Material | Amount |
---|---|
Something | ul |
Something | ul |
Something | ul |
Procedure
- First
- Second
- Third
Terpenoid Production and Detection
Materials
- First
- Second
- Third
Procedure
- First
- Second
- Third
KillerRed Kill Curve
Materials
- First
- Second
- Third
Procedure
- First
- Second
- Third