Team:Cornell/Protocol

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Results | Protocol | Notebook | Parts Submitted

Protocols

Below, please find the steps that we followed to carry out molecular cloning, create recombinant DNA parts, and construct microfluidic channels.

Molecular Cloning Protocols

PCR Reaction
Note: Keep everything on ice and add all volumes in a PCR tube.
37.5μL ddH2O
5.0μL 10x buffer
2.5μL dNTPs
1.0μL MgSO4
1.0μL forward primer
1.0μL reverse primer
1.0μL template
1.0μL Vent DNA polymerase
50.0μL Total
Based on primers, set an appropriate annealing temperature
Agarose Gel Electrophoresis
  1. Prepare a 1% weight-to-volume agarose gel and add SYBR dye or ethidium bromide to stain DNA
  2. Place the gel in the apparatus rig with the wells facing the negative end (black-colored)
  3. Fill the rig with 1x TAE buffer
  4. Load 2µL of 1kb ladder
  5. Add 2µL of 6x loading dye to each PCR reaction tube. Load 20µL in wells
  6. Run at 120V
Gel Purification of DNA (Qiagen QIAquick Gel Extraction Kit)
  1. Cut out the DNA fragment from the agarose gel with a razor blade, while minimizing the size of the gel slice
  2. Weigh the gel slice and add 3 volumes of Buffer QG to every 1 volume of gel (100mg = 100µL)
  3. Dissolve the gel slice using a 60°C heat block
  4. Apply the dissolved gel to the QIAquick column and centrifuge at 13,000rpm for 1 minute
  5. Discard the flow-through and repeat Step 4 until all sample has passed through the column
  6. Add 500µL of Buffer QG to the QIAquick column and centrifuge at 13,000rpm for 1 minute
  7. Wash the column with 750µL of Buffer PE and centrifuge at 13,000rpm for 1 minute
  8. Discard the flow-through and centrifuge at 13,000rpm for 1 minute
  9. Transfer the QIAquick column to a new Eppendorf
  10. Add 35µL elution buffer to the center of the column and wait at least 2 minutes
  11. Centrifuge at 13,000rpm for 1 minute
DNA Quantification using NanoDrop Spectrophotometry
  1. Select Nucleic Acids measurement
  2. Initialize the NanoDrop spectrophotometer with 2µL of autoclaved H2O and wipe off
  3. Blank (calibrate) the NanoDrop spectrophotometer with 2µL of the same elution buffer used during DNA purification and wipe off
  4. Measure 1.5µL of DNA sample and record the concentration in ng/µL
Digestion Reaction
Note: Keep everything on ice
? µL ddH2O (? = whatever volume needed to bring the total volume up to 50µL)
5µL 10x NEBuffer
? µL DNA sample (? = whatever volume corresponds with 1µg)
0.5µL 100x BSA
1µL first restriction enzyme
1µL second restriction enzyme
50µL Total
Note: Consult www.neb.com to determine the buffer compatibility of the restriction enzymes used
  • Incubate the digestion reaction tube in a 37°C water bath for 3 hours
Dephosphorylation of 5' Ends of Vector Backbone

Microfluidics Protocols

Biosafety Rules and Procedures
We complied with Weill hall’s safety requirements in gaining access to lab space, as well as in use of the lab. All safety information and procedures are linked on the main Weill safety page [http://blogs.cornell.edu/whfs/weill-hall-safety-links-and-information/ here].

Weill Hall Safety Personnel
Scott D. Emr is the director of Weill Hall which is the building our lab is located. There is also a Weill Hall Safety Committee. While we did not personally meet as a group with either groups, we talked Dr. Archer who is in charge of our particular lab space. She approved of our project and helped us with the safe construction of our microfluidic mask.

Safety Training We received safety training from two online courses that all members were required to pass in order to gain access to the building. These were Lab Safety and Chemical Waste Disposal. Also we received training from our lab instructor on basic safety issues such as waste disposal, use of the fuse hood, etc.

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