Difference between revisions of "Team:CSU Fort Collins/Experiments"

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<div class="panel" id="panel1">
 
<div class="panel" id="panel1">
 
     <h3>Materials</h3>
 
     <h3>Materials</h3>
     <ul>    <li>First</li>
+
     <ul>    <li>Agarose</li>
             <li>Second</li>
+
             <li>1X TAE Buffer</li>
             <li>Third</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

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Protocols

Plasmid Construction

Materials

Material Amount
Something ul
Something ul
Something ul

Procedure

  1. First
  2. Second
  3. Third

Gel Electrophoresis

Materials

  • Agarose
  • 1X TAE Buffer
  • Parafilm
  • Electrophoresis chamber and power source
  • SYBR Green
  • Loading Dye
  • DNA Ladder
  • PCR Samples

Procedure

  1. 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.
  2. Microwave the mixture, mixing by swirling intermittently, until all the agarose is dissolved and the mixture is homogeneous and clear (about 2 minutes).
  3. 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.
  4. 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.
  5. 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.
  6. Load 10 μL of each sample into the appropriate wells.
  7. Connect wiring and run gel electrophoresis at 110 V for 1 hour.
  8. 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

  1. First
  2. Second
  3. Third

Terpenoid Production and Detection

Materials

  • First
  • Second
  • Third

Procedure

  1. First
  2. Second
  3. Third

KillerRed Kill Curve

Materials

  • First
  • Second
  • Third

Procedure

  1. First
  2. Second
  3. Third

Inspiration