"

 

From 2008.igem.org

• Home
  • Welcome
  • Announcements
• The Team
  • Who We Are
    • Advisors
    • Undergrads
  • What We've Done
  • Where We're From
  • Contact Us
• The Project
  • Overview
  • Expression
  • Communication
  • Oscillation
  • Application
  • Journal Club
• BioBricks
• Modeling
• Wet Lab
  • Lab Protocols
  • WetWare
• Notebook
• Sponsors
  • Academic
  • Research
  • Corporate

 

 

Contents 1 Today in the Lab 2 Chris 3 Matt 4 Dan

Today in the Lab

Chris

Digestion and Ligation of OA, OB and T Amp Product

Digested all three according to previous digestion protocol (see August 5 post). Ran 7 samples--six ligations and one digestion products only. Incubated at 37°C for 15 minutes, followed by 20 minutes at 80°C to denature.

Spiked each tube with ligase and ATP then incubated at room temperature for around two hours.

Ran products on a 0.6% gel for 1.5 hours at 80V. Stained the gel in an Ethidium Bromide and TAE Buffer solution for 20 minutes.

Excised desired band and performed gel extraction. Stored at -20°C.

Matt

Absorbance was measured from the ten colonies miniprepped by Chris. I then digested each colony with PST1 to confirm.

All colonies were confirmed and successful.

Used SLN1 primers to amplify the PTP2/GAL10 casette overnight from two colonies chosen from the miniprep.

Dan

p1T miniprep confirmation

p1T was digested with HindIII for confirmation, I did not get the correct product :(

dehydrogenase construct

pSSB37 and pDR197(pure1) were both digested with SphI and HindIII

Master plates of pSSB37 and pDR197(pure1) were streaked

• Recent changes
• What links here
• Related changes
• Special pages
• My preferences

• Printable version
• Permanent link
• Privacy policy
• Disclaimers