"

From 2011.igem.org

Revision as of 12:09, 4 October 2011 (view source) Rhianna (Talk | contribs) ← Older edit		Revision as of 12:18, 4 October 2011 (view source) Rhianna (Talk | contribs) Newer edit →
Line 25:		Line 25:
	[[File:IMG_0194.JPG‎ | 231x125px]]		[[File:IMG_0194.JPG‎ | 231x125px]]
		+
		+	PCR of glnG (lanes 2 and 3), glnAp2 (lanes 5 and 6), and the promoter Plac/ara (lanes 6-8 of the second gel)
		+
		+	[[File:IMG_0195.JPG | 200x125px]]

---

Revision as of 12:18, 4 October 2011

• Home
  • UQ-Australia
  • iGEM 2011
• Team
  • Students
  • Supervisors
• Project
• Parts
• Data
• Modelling
  • Kinetics
  • Synchronisation
  • Microscopy
• Notebook
  • Protocols
  • April
  • May
  • June
  • July
  • August
  • September
• Safety
• Human Practices
  • Patenting
  • Outreach
  • Collaboration
• Attributions

There is a '[HERE]'where you should edit in places where I remembered to put them. [HERE] Summary [HERE]

We conducted a heat cycle PCR to determine the optimum conditions for amplifying our araC gene. The lanes here are loaded as follows:

1: 1kb+ ladder

2: Negative control (H2O)

3-7: pBAD33 plasmid at temperatures 50C, 55C, 58C, 60C and 65C.

8: Negative control (H2O)

9-13: pBAD33 plasmid at temperatures 50C, 55C, 58C, 60C and 65C.

PCR of the lacI gene

PCR of glnG (lanes 2 and 3), glnAp2 (lanes 5 and 6), and the promoter Plac/ara (lanes 6-8 of the second gel)