BME100 s2014:T Group9 L4

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BME 100 Spring 2014 Home
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Lab Write-Up 1 | Lab Write-Up 2 | Lab Write-Up 3
Lab Write-Up 4 | Lab Write-Up 5 | Lab Write-Up 6
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OUR TEAM

Name: Cassaundra Kinnear
Name: Katherine Underwood
Name: Kyle Queen
Name: Mohammed Binsheliail

LAB 1 WRITE-UP

Initial Machine Testing

The Original Design
(Add image of the full OpenPCR machine here, from the Week 9 exercise. Write a paragraph description for visitors who have no idea what this is)


Experimenting With the Connections

When we unplugged (part 3) from (part 6), the machine's LCD display turned off.

When we unplugged the white wire that connects (part 6) to (part 2), the machine the temperature reading showed as -40 degrees Celsius and showed a wrong reading.


Test Run

On March 10th, 2014 between the hours of 9am and 12pm, the test run was attempted. 12 runs were completed and the machine passed.




Protocols

Thermal Cycler Program


DNA Sample Set-up

Positive Control- a Negative Control- b Patient 1 Sample 1- c Patient 1 Sample 2- d
Patient 1 Sample 3- E Patient 2 Sample 1- F Patient 2 Sample 2- G Patient 2 Sample 3- H


DNA Sample Set-up Procedure

  1. 1. Collect the following items: 8 empty PCR tubes, 8 PCR tubes filled with PCR liquid, the negative control, the positive control, and the 6 PCR tubes filled with samples from the patients.
  2. Step 2
  3. Step 3...


PCR Reaction Mix

  • What is in the PCR reaction mix?


DNA/ primer mix

  • What is in the DNA/ primer mix?





Research and Development

PCR - The Underlying Technology


In this lab we learned how PCR is used to detect a disease-associated DNA sequence(SNP). To do this we had to know a nucleotide is an organic molecule that serves as the monomer of nucleic acids like DNA and RNA. We also had to know polymorphism is two or more different phenotypes within the same species.

Finding the Disease-Associated Sequence

For this experiment we were given the SNP sequence rs237025. We found the species for this variation is homo sapien. This variation is found on teh chromosome 6:149721690 and the clinical significance was listed as other. This SNP is associated with the genes SUMO4 and TAB2. SUMO4, small ubiquitin-like modifier 4, is located in the cytoplasm of cells and specifically modifies IRBA. The diseases linked to it are type 1 Diabetes, Type 2 Diabetes, nephropathy, and VKH syndrome.

Designing a Disease Sequence-Specific Primer Pair

An allele is and alternative form of a gene for a character producing different effects. The non-disease allele contains GTG, whereas the disease-associated allele contains the sequence ATG.
The numerical position of the SNP rs237025 is 149721690. The forward primer needed to design a diseased-allele-specific primer pair is CACCACTTAGTAAACTAATG. The numerical position 200 bases to the right of the disease SNP is 149721890, and the reverse primer for the SNP is CGTAAGAGTTAATCTTTTGA. If the template contains the non-disease allele PCR should not occur. This is due to the disease-specific primer and template not binding 1oo% to the non-disease allele because the non-disease allele had a sequence of GTG, when the disease-assocoated allele has a sequence of ATG.



(BONUS points: Use a program like Powerpoint, Word, Illustrator, Microsoft Paint, etc. to illustrate how primers bind to the cancer DNA template, and how Taq polymerases amplify the DNA. Screen-captures from the PCR video/ tutorial might be useful. Be sure to credit the sources if you borrow images.)





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