Difference between revisions of "Team:NAIT Edmonton/Protocols"

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   <center><img src="http://www.bio-rad.com/webroot/web/images/lsr/products/electrophoresis/product_detail/global/lsr_silver_stain_plus_kit.jpg"></center>
 
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     <p>1) Once SDS-PAGE is complete, remove gels from the glass plates and remove the stacking gel layer
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     <ol type="1">
using a paper towel. <br> 2) Place gel in a glass container, wash with 200ml distilled water for 5 minutes. Repeat the wash
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step 4X. (shake gel back and forth in shaker) Decant water into waste container. <br> 3) Mix a solution with 90ml of 10% acetic acid and 90ml of 10% methanol in a clean beaker. Add
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<li>Once SDS-PAGE is complete, remove gels from the glass plates and remove the stacking gel layer using a paper towel. </li>
10ml of fixative enhancer solution into the beaker and pour over the gel. Let sit for 20 minutes  
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<li>Place gel in a glass container, wash with 200ml distilled water for 5 minutes. Repeat the wash step 4X. (shake gel back and forth in shaker) Decant water into waste container. </li>
on shaker, or up to a maximum of overnight, depending on the desired sensitivity of the gel. <br> 4) Decant solution into a proper waste container. <br> 5) Wash gel once again with 200ml of distilled water for 5 minutes on shaker. Repeat 4X. Decant
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<li>Mix a solution with 90ml of 10% acetic acid and 90ml of 10% methanol in a clean beaker. Add 10ml of fixative enhancer solution into the beaker and pour over the gel. Let sit for 20 minutes on shaker, or up to a maximum of overnight, depending on the desired sensitivity of the gel.</li>
water into waste container. <br> 6) Mix both parts of stain solution into two separate falcon tubes. <br><br></p>
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<li>Decant solution into a proper waste container.</li>
      <p><b><u>Mix 1</u></b></p>
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<li>Wash gel once again with 200ml of distilled water for 5 minutes on shaker. Repeat 4X. Decant water into waste container.</li>
      <p>- 2.5ml of Silver Complex Solution<br> - 2.5ml of Reduction Moderator Solution<br> - 2.5ml of Image Development Reagent<br> - 17.5ml of DH20 <br><br></p>
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<li>Mix both parts of stain solution into two separate falcon tubes.
      <p><b><u>Mix 2</u></b></p>
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<ul><b>Mix 1</b>
      <p>- 1.25g of Development Accelerator<br> - 25ml of DH20 <br><br> 7) Mix both solutions together until each are dissolved, pour over gel. Let sit for up to 20 minutes
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<li>2.5 mL of Silver Complex Solution</li>
or until desired bands show. <br> 8) Decant solution into proper waste container. <br> 9) Prepare a stop solution containing 90ml of 10% acetic acid and 90ml of 10% methanol. Pour
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<li>2.5 mL of Reduction Moderator Solution</li>
over gel and shake for 15-20 minutes. <br> 10) Decant solution into proper waste container. <br> 11) Wash gel with 200ml of DH20 for 5 minutes on shaker. Repeat 2X.<br> GELS ARE STAINED!</p>
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<li>2.5 mL of Image Development Reagent</li>
 +
<li>17.5 mL of DH20 </li>
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</ul>
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<ul><b>Mix 2</b>
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<li>1.25 g of Development Accelerator</li>
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<li>25mL of DH20 </li>
 +
 
 +
</ul>
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</li>
 +
 
 +
<li>Mix both solutions together until each are dissolved, pour over gel. Let sit for up to 20 minutes or until desired bands show. </li>
 +
<li>Decant solution into proper waste container. </li>
 +
<li>Prepare a stop solution containing 90ml of 10% acetic acid and 90ml of 10% methanol. Pour over gel and shake for 15-20 minutes.</li>
 +
<li>Decant solution into proper waste container. </li>
 +
<li>Wash gel with 200ml of DH20 for 5 minutes on shaker. Repeat 2X.</li>
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</ol> <br>
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GELS ARE STAINED!
  
  

Revision as of 22:05, 20 August 2015

Team NAIT 2015

Experimental Design

Go through our interactive experimental design flow chart! Many of our protocols are manufacturer specicfied; however, some are customized by us! Click on the flow chart boxes if the hand cursor appears to read more about our customized protocols.

PDFs of protocols can also be found

Theorizing our Sequences
Literature has shown certain proteins inherently stain in colour.
Looked up characteristics of said proteins
Isolated and identified the unique characteristics of said proteins so that we can manually write our own sequences and generate custom proteins.
Writing our Sequences
Went down to base pair level and wrote out our sequences with the defining characteristics identified in literature.
PCR
Digestion and Ligation
Transforming Bacteria
Validating the Transformation
Protein Isolation and Purification
SDS PAGE and Silver Staining