BME103:T130 Group 6 l2: Difference between revisions

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<ul>Here are two examples:<br>
<ul>Here are two examples:<br>
<li> <b>Single Nucleotide Polymorphism (SNP) - <font color="red">rs799917</font color></b><br>
<li> <b>Single Nucleotide Polymorphism (SNP) - <font color="red">rs799917</font color></b><br>
[http://www.ncbi.nlm.nih.gov/projects/SNP/snp_ref.cgi?rs=799917 NCBI database] <br>
[http://www.ncbi.nlm.nih.gov/projects/SNP/snp_ref.cgi?rs=799917 NCBI database rs799917] <br>
<u>Location:</u> <i>Chromosome 17 at position 41,244,936bp. </i><br>
<u>Location:</u> <i>Chromosome 17 at position 41,244,936bp. </i><br>
<u>Variation Type:</u> <i>Single Nucleotide Variation</i>; Missense Mutation<br>
<u>Variation Type:</u> <i>Single Nucleotide Variation</i>; Missense Mutation<br>
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<i>If Cytosine is replaced by Adenine or Thymine in this sequence the resulting amino acid would either be glutamine or leucine respectively instead of proline. This change in amino acids will result in an alteration to the overall protein. Something this small is what could cause a cancerous gene.</i>
<i>If Cytosine is replaced by Adenine or Thymine in this sequence the resulting amino acid would either be glutamine or leucine respectively instead of proline. This change in amino acids will result in an alteration to the overall protein. Something this small is what could cause a cancerous gene.</i>
<br><br>
<br><br>
<li> <b>Single Nucleotide Polymorphism - <font color="red">rs4986852</font color></b><br>
<li>
<b>Single Nucleotide Polymorphism - <font color="red">rs4986852</font color></b><br>
[http://www.ncbi.nlm.nih.gov/projects/SNP/snp_ref.cgi?rs=4986852 NCBI database rs4986852] <br>
<u>Location:</u> <i>Chromosome 17 at position 41,244,429bp. </i><br>
<u>Location:</u> <i>Chromosome 17 at position 41,244,429bp. </i><br>
<u>Variation Type:</u> <i>Single Nucleotide Variation</i>; Missense Mutation<br>
<u>Variation Type:</u> <i>Single Nucleotide Variation</i>; Missense Mutation<br>
<u>Reference strand (<i>41,244,455 bp-41,244,404 bp</i>):</u>  
<u>Reference strand (<i>41,244,455 bp-41,244,404 bp</i>): </u>  
<br><b>3'</b> TAGAGAAAATGTTTTTAAAGAAGCCA[<font color="red">A</font color>/G*]CTCAAGCAATATTAATGAAGTAGGT<b> 5'</b> <br>
<br><b>3'</b> TAGAGAAAATGTTTTTAAAGAAGCCA[<font color="red">A</font color>/G*]CTCAAGCAATATTAATGAAGTAGGT<b> 5'</b> <br>
* This represents G as the normal base and C as the possible mutation for this SNP.<br>
* This represents G as the normal base and C as the possible mutation for this SNP.<br>
<i>If Guanine is replaced with Cytosine then Asparagine will be produced instead of Serine which will also cause a change in the protein that has been connected to BRCA1.</i>
<i>If Guanine is replaced with Cytosine then Asparagine will be produced instead of Serine which will also cause a change in the protein that has been connected to BRCA1.</i>
<br>
<br></li>
</ul>
</ul>


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<br><br>
<br><br>
'''Primer Design'''
'''Primer Design'''
 
In order for the PCR to replicate only the DNA which contains the viral mutation we had to design specific primers for each SNP.<br>
<br><ul><li><b>SNP - rs799917</b><br>
<b><u>Forward Primer:</u>5'</b>GCTTATCTTTCTGACCAACC<b>3'</b><br>
<b><u>Forward Primer:</u>5'</b>GCTTATCTTTCTGACCAACC<b>3'</b><br>
<i>located at approximately 41,244,736 - 41,244,756; 200bp to the left of the mutation</i><br>
<i>located at approximately 41,244,736 - 41,244,756; 200bp to the left of the mutation</i><br>
<b><u>Reverse Primer:</u>3'</b>TCATTGCTC<font color="red">A/T</font color>GTTTTCAAA<b>5'</b><br>
<b><u>Reverse Primer:</u>3'</b>TCATTGCTC<font color="red">A/T</font color>GTTTTCAAA<b>5'</b><br><br></li>
<li><b>SNP - rs4986852</b><br>


<!--- Include the sequences of your forward and reverse primers. Explain why a disease allele will give a PCR product and the non-disease allele will not. --->
<!--- Include the sequences of your forward and reverse primers. Explain why a disease allele will give a PCR product and the non-disease allele will not. --->

Revision as of 05:38, 29 November 2012

BME 103 Fall 2012 Home
People
Lab Write-Up 1
Lab Write-Up 2
Lab Write-Up 3
Course Logistics For Instructors
Photos
Wiki Editing Help

OUR TEAM

Name: Jocelynn Christensen
Role: R & D Scientist
Name: Ryan Uchimura
Role: Experimental Protocol Planner/Coolest person ever
Name: Sam Zimmerman
Role: OpenPCR Machine Engineer)
Name: Adam Helland
Role:
Name: Dakota Styck
Role:

LAB 2 WRITE-UP


PCR Machine Improvements


Design Goals:
Expand Sample Size; which will increase efficiency
Add Tabs to the Bottom of the Lid; this will make it so that the user knows when the lid is on completely without crushing the samples.

Thermal Cycler Engineering

Our re-design is based upon the Open PCR system originally designed by Josh Perfetto and Tito Jankowski.


System Design


Key Features


Instructions





Protocols

Materials
Supplied in the Kit

PCR Flourimeter
gloves/labcoat - 1 flourimeter - 1
PCR machine - 1 Box - 1
Pipets - 8 Smartphone holder - 1
PCR reaction mix - 8 tubes, 50 μL each
PCR holding tray - 1


Supplied by User

PCR Flourimeter
Computer - 1 Smartphone/Camera - 1
DNA - 8 samples Image J Software - 1




PCR Protocol



DNA Measurement Protocol
1. Take the file box and place it upside down (after it's been emptied) so that there is now an area that will restrict as much light as possible from coming through in the pictures.
2. Place the hydrophobic slide in the center of the fluorimeter and align it so that the row of dots is directly in the middle of the blue lazer.
3. Using a pipet, place two droplets of water gently on the middle hole of the slide.
4. Next use the pipet to add two droplets of the PCR solution for the first sample with the two water droplets. This must be done cautiously so that the droplets will stay in the center and adhere to each other properly.
5. Turn on the light source on and place the fluorimeter as far back as possible inside the upside down box.
6. Turn the camera on a smart phone and adjust the settings accordingly. Inactivate the flash, set iso to 800 (or higher if possible), set white balance to auto, exposure to the highest setting, saturation to highest setting and contrast to the lowest setting.
7. Place a smartphone camera into the cradle and then move the cradle in front of the fluorimeter at the perfect distance for good resolution (may take some adjusting).
8. Take a picture of the mixture on the fluorimeter (best done if camera is on a timer so that you can fully close the box and avoid excess light exposure.
9. Repeat steps 2-8 for each sample.

1. Download the Image J software
2. Open Image J
3. To chose your pictures click 'file' and 'open' then select the image you wish to analyze
3. Once your image is opened highlight and click on "analyze", "set measurements", and check the boxes "area" "integrated density" and "mean gray value" in order to just analyze the pieces for this lab.
4. After this you have to highlight and click "image", "color", then click "split channels"
5. This splits the image you have into three new images. For this assignment just keep the image "green" and disregard the others.
6. Then analyze the droplet in the picture to get the info for integrated density, mean gray value, and area.
7. Repeat steps for one picture of each sample.
8. Save your data in an excel page for easy access at another time

Research and Development

Breast Cancer Markers

Without including skin cancer, breast cancer is the most frequently diagnosed cancer in women today. While there's not one specific "cause" of breast cancer many things like excessive weight gain after age 18, use of estrogen and progestin hormone therapy, physical inactivity, as well as alcohol consumption have all been identified as risk-factors for breast cancer. While those may be avoidable risks there are some risks that cannot be avoided because they're genetically encoded in our DNA. Breast cancer has been linked to certain genetic mutations in the BRCA1 gene as well as the BRCA2 gene. While having a mutation of either of these genes doesn't guarantee breast cancer, someone with a mutation on either gene is 5 times more likely to develop breast cancer during their life.
The BRCA1&2 genes have been identified as tumor suppressor genes on the 17th chromosome. Specifically looking at BRCA1, the gene encodes a nuclear phosphoprotein who's job is to maintain genomic stability and act as a tumor suppressor. This protein plays a huge role in transcription, DNA repair, and recombination. When this gene is mutated it's responsible for nearly 40% of inherited breast cancers.

Background on Disease Markers

There are thousands of mutations associated with the BRCA1 gene.

    Here are two examples:
  • Single Nucleotide Polymorphism (SNP) - rs799917
    NCBI database rs799917
    Location: Chromosome 17 at position 41,244,936bp.
    Variation Type: Single Nucleotide Variation; Missense Mutation
    Reference strand (41,244,962 bp-41,244,911 bp):
    3' GGTTTCAAAGCGCCAGTCATTTGCTC[A/C/T*]GTTTTCAAATCCAGGAAATGCAGAA 5'
    * This represents C as the normal base and A/T as the possible mutations for this SNP.
    If Cytosine is replaced by Adenine or Thymine in this sequence the resulting amino acid would either be glutamine or leucine respectively instead of proline. This change in amino acids will result in an alteration to the overall protein. Something this small is what could cause a cancerous gene.

  • Single Nucleotide Polymorphism - rs4986852
    NCBI database rs4986852
    Location: Chromosome 17 at position 41,244,429bp.
    Variation Type: Single Nucleotide Variation; Missense Mutation
    Reference strand (41,244,455 bp-41,244,404 bp):
    3' TAGAGAAAATGTTTTTAAAGAAGCCA[A/G*]CTCAAGCAATATTAATGAAGTAGGT 5'
    • This represents G as the normal base and C as the possible mutation for this SNP.
    If Guanine is replaced with Cytosine then Asparagine will be produced instead of Serine which will also cause a change in the protein that has been connected to BRCA1.




Primer Design In order for the PCR to replicate only the DNA which contains the viral mutation we had to design specific primers for each SNP.


  • SNP - rs799917
    Forward Primer:5'GCTTATCTTTCTGACCAACC3'
    located at approximately 41,244,736 - 41,244,756; 200bp to the left of the mutation
    Reverse Primer:3'TCATTGCTCA/TGTTTTCAAA5'

  • SNP - rs4986852


    Illustration
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