Description of samples:
Image 1: 3 drops of sybrgreen, 2 drops of calibrator solution. Dot was all blue not green. This implies the solution is negative for cancer.
Image 2: 4 drops of sybrgreen, 2 drops of water solution. Dot was all blue no green. This implies the solution is negative for cancer.
Image 3: 3 drops of sybrgreen, 2 drops of patient 1 solution A. Dot has some slight blurrs of gree. This implies the DNA solution is positive for cancer.
Image 4: 2 drops of sybrgreen, 2 drops patient 1 solution B. Dot was all blue with no sight of green. This implies the DNA solution is negative for cancer.
Image 5: 3 drops of sybrgreen, 2 drops of patient 1 solution C. Dot was all blue with no sight of green. This implies the DNA solution is negative for cancer.
Image 6: 3 drops of sybrgreen, 2 drops of patient 1 solution D. Dot was all blue with no sight of green. This implies the DNA solution is negative for cancer.
Image 7: 3 drops of sybrgreen, 2 drops of patient 2 solution A2. Dot was all blue with no sight of green. This implies the DNA solution is negative for cancer.
Image 8: 3 drops of sybrgreen, 2 drops of patient 2 solution B2. Dot has a spec of bright green. This implies the DNA solution is positive for cancer.
Image 9: 4 drops of sybrgreen, 2 drops of patient 2 solution C2. Dot had some spattered green. This implies the DNA solution is positive for cancer.
Image 10: 5 drops of sybrgreen, 2 drops of patient 2 solution D2. Dot had a really green center. This implies the DNA solution is positive for cancer.
Patient ID:
Patient 1: 74065, Male, Age:63
Patient 2: 64835, Male, Age:46
Flourimeter Measurements
1. Turn on the blue light in the Flourimeter using the switch for the Blue LED.
2. Place the smart phone accordingly so that the super-hydrophobic slide is in front of the smart phone.
3. Turn on the camera on the smart phone. **TURN OFF THE FLASH** Set the ISO to 800 or higher. Increase the exposure to maximum.
4. Set the distance between the smart phone and the machine so that the smart phone can take a clear picture of the droplet.
5. First label the blank pipettes according to the patients (A,B,C,D... all eight of them). The pipettes given by the instructor are
color coded. The white coded pipette is used for water. the red coded pipette is used for the calibrator (the tube with the red dot). The blue coded pipette is used for the sybrgreen (the tube with the blue dot). The black coded pipette is used to pick up the waste and put it in the cup that collects the waste droplets.
6. First calibrate the machine (to make sure the machine works). Put two droplets of the cyber green on the first two dots in the middle. If the droplets are not connected then add a third droplet that combines the two droplets.
7. Then put two drops of calibrator solution with the calibrator solution. Then set the smart phone accordingly to take a clear picture of the droplet. Then put the black box on top of the phone and the machine so that when the the light is completely blocked and the shade of blue of green is shown when the picture is taken.
8. Record observations.
9. Remove the solution from the glass dish using the black pipette and discard it in the plastic cup given for the waste droplets.
10.Repeat step 6-9, but instead of adding calibrator solution, add 2 droplets of water.
11.Repeat steps 6-9 for patient 1 solutions (A,B,C,D) and patient 2 solutions (A2.B2,C2,D2).
Research and Development
Specific Cancer Marker Detection - The Underlying Technology
The r17879961 sequence will produce a cancer mutation at Chromosomes 22 of the gene sequence. The normal sequence has a T ( thymine) nucleotide at chromosome 22 while the mutation sequence has an associated C (cytosine) nucleotide. The Open PCR machine is able to determine whether or not the r17879961 sample has cancer by replicating the desired mutation exponentially. Positive and negative strands are inserted into the PCR with a certain primer. The primer in the reaction is designed to attach to the C nucleotide that signifies cancer mutation. One strand has the primer, while the other strand does not. Open PCR will replicate the strand with the certain primer, causing an exponential growth. The negative strand will grow in a linear fashion. The PCR process goes through 30 cycles to complete this. After the PCR process, fluorescent dye is added to the solutions. The fluorescent dye will cause the DNA with double strands to glow. Since the PCR has grown the double stranded positive DNA exponentially the fluorescent dye glows brighter. Therefore the cancer DNA is in the sample with the glow.
The DNA double helix seperates, creating two single-stranded DNA molecules.
Primers attach and lock onto the targeted sequence before the strands can rejoin.
DNA polmerase locates the primerr and begins to add complimentary nucleotides onto the strands.
Cycle one is complete.
The steps are repeated, increasing the amount of DNA.
Primers attach to the targeted sequence
The desired fragments are segments of the targeted DNA (Cancer).
These fragments will continue to duplicate with each cycle.
Source: Genetic Science Learning Center (2012, August 6) PCR Virtual Lab. Learn.Genetics. Retrieved November 8, 2012, from http://learn.genetics.utah.edu/content/labs/pcr/
Results
Sample |
Integrated Density |
DNA μg/mL |
Conclusion
|
PCR: Negative Control |
2003444 |
0 |
negative
|
PCR: Positive Control |
9972359 |
2 |
positive
|
PCR: Patient 1 ID 74065, rep 1 |
7454123 |
1.495 |
positive
|
PCR: Patient 1 ID 74065, rep 2 |
5846771 |
1.1726 |
positive
|
PCR: Patient 1 ID 74065, rep 3 |
3886745 |
0.7795 |
negative
|
PCR: Patient 2 ID 64835, rep 1 |
26052159 |
5.2249 |
positive
|
PCR: Patient 2 ID 64835, rep 2 |
33652771 |
6.7492 |
positive
|
PCR: Patient 2 ID 64835, rep 3 |
48574317 |
9.7418 |
positive
|
KEY
- Sample =
- Integrated Density =
- DNA μg/mL =
- Conclusion =
|