BME103:W930 Group7

From OpenWetWare
Revision as of 19:58, 13 November 2012 by Seong Song (talk | contribs) (→‎Results)
Jump to navigationJump to search
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: Jake Turner
PCR Machine Engineer
Name: Tyler Allen
PCR Machine Engineer
Name: Khalil Pathan
Experimental Protocol Planner
Name: Pahul Singh
Experimental Protocol Planner
Name: Frea Mehta
Research and Development Specialist
Name: Paul Song
Research and Development Specialist

<iframe width="560" height="315" src="http://www.youtube.com/embed/x5yPkxCLads?rel=0" frameborder="0" allowfullscreen></iframe>

LAB 1 WRITE-UP

Initial Machine Testing

The Original Design
Open PCR Machine

This is a solidworks rendering of the OpenPCR machine. The OpenPCR is an affordable alternative to costly clinical machines used to amplify particular DNA sequences. This interfaces with any computer with the proper software downloaded and the process of thermal cycling to conduct a variety of tests. This could be anything from paternity tests to test for genetic marks of cancer.


Experimenting With the Connections

When we unplugged part (part 3) from (part 6), the machine did not have power. The blue display screen did not turn on and appeared completely black.

When we unplugged the white wire that connects (part 6) to (part 2), the machine temperature on the display screen appeared incorrectly. Part 6 is responsible for recording the the internal temperature of the machine throughout the test.


Test Run

While running our open PCR test, we experienced nothing but problems. We set the cycles to the appropriate temperatures and time intervals; the Initial cycle on 95°C for 30 seconds, the Denaturing cycle on 95°C for 30 seconds, the Annealing cycle on 55°C for 30 seconds, the Extending cycle on 72°C for 30 seconds, the final cycle on 72°C for 180 seconds, and the final hold at 20°C. Initially, our open PCR appeared to be running correctly for the desired two hour time interval. However, due to a cycling error, our timer extended to nearly three hours. Not only did our test exceed the desired time interval, but our time would not wind down. Our test constantly moved up and down between the times of two hours thirty minutes and two hours and fifty minutes. When our time got close to two thirty, more time would be added to our test. Also, our laptop was experiencing errors. Our laptop received an application error notice multiple times, each time disrupting our process. As a result of these complications, when the two hours elapsed we only reached step seventeen of thirty. We were forced to prematurely end our test. Therefore, we could not receive sufficient results.





Protocols

Polymerase Chain Reaction

(

1. Within a polymerase chain reaction everything is controlled by temperature. The high temperature(95 C) causes melting of DNA templates and primers by disrupting the hydrogen bonds. Next is annealing. The temperature is dropped down to 65 temporarily(20 seconds) to allow a piece of DNA to bind to your product from the initial step. The polymerase binds to the DNA template and DNA synthesis begins. Next is elongation, the DNA polymerase synthesizes a new DNA strand. This process is repeated to replicate numerous strands of DNA.

2. 

     1. Heat denaturation-
               a. Heat the reactant , which causes melting of the DNA
               b. A DNA molecule sequence is targeted which is then separated into two strands
               c. Separation is because of hydrogen bonds breaking
     2. Primer annealing 
               a. Then you lower the temperature to 65 which allows a piece of the DNA to bind to the initial step product. 
               b. Each strand of DNA molecule becomes annealed with an oligonucleotide primer complementary to either end of the target sequence.
     3. Primers extension
               a. DNA polymerase is added and complementary strands are synthesized at 65-75 C
               b. Causes synthesis of a new strand in the direction of 5 to 3 direction

4. 

    Reagent	                       Volume
    Template DNA (20ng)	               .2 µL 
    10 µM forward primer	       1.0 µL
    10 µM reverse primer	       1.0 µL
    GoTaq master mix	               50.0 µL
    dH20	                       47.8 µL
    Total volume	               100.0 µL

)


Flourimeter Measurements

(Add your work from Week 3, Part 2 here)




Research and Development

Specific Cancer Marker Detection - The Underlying Technology

The NCBI database is used to isolate the sequence used and determine specific primers.

(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 OpenPCR tutorial might be useful. Be sure to credit the source if you borrow images.)




Results

Sample Integrated Density DNA μg/mL Conclusion
PCR: Negative Control 267793 0 G6
PCR: Positive Control 27409968 2 G7
PCR: Patient 1 ID 91562, rep 1 3511064 0.238984 G8
PCR: Patient 1 ID 91562, rep 2 15099598 1.09290 G9
PCR: Patient 1 ID 91562, rep 3 8451848 0.603051 G10
PCR: Patient 2 ID 25235, rep 1 17311845 1.25591 G11
PCR: Patient 2 ID 25235, rep 2 9289657 0.200563 G12
PCR: Patient 2 ID 25235, rep 3 28825322 2.10429 G13


KEY

  • Sample =
  • Integrated Density =
  • DNA μg/mL =
  • Conclusion =
Retrieved from "https://openwetware.org/mediawiki/index.php?title=BME103:W930_Group7&oldid=653964"