"

 

From 2008.igem.org

Birds Eye  View Team	Projects	Events	Resources
Sponsors	Experiments	Milestones	Protocols
	Notebook (t)	Meetings (t)

Things we did today

Wetlab work

PCR

Grace

• 25 μl PCR reactions for GFP site directed mutagenesis and extraction of Biobrick pertinent sites from BBa_B0034

Made stocks

Grace

• Made two 500mL batches of SOB
• Made 20 LB + amp₁₀₀ plates

Transformed DH5α with ligations of a Biobrick vector with pnir, slr2016-1, slr2016-2, pilA, or C0012

Grace

• Transformed using 5 μl of 1:1 and 1:10 ligation dilutions
• Transformed using 1 μl vector only (negative control)
• Incubated on ice 10 min as opposed to the recommended 30 min. by iGEM

RE digested PCR products and plasmids

Grace

• XbaI and PstI: GFP fusion brick and BBa_C0012

• Added XbaI and PstI separately
• Ran 25 μl of GFP and 20 μl of BBa_C0012 restriction digest reactions in gel

• HindIII and BamHI: Biobrick segment and pRL1383a

• Ran 25 μl of Biobrick segment (half of total rxn) and 20 μl of pRL1383a restriction digest reactions in gel
• pRL1383a was not visbile under long wave UV. Need to rerun gel tomorrow with much more plasmid

Transformed DB3.1

Margaret

• Transformed: pSB3K3, pSB1A2, pSB1AK3, (+)pUC18, (-)nothing. The positive and negative control verify that the DB3.1 competent cells made on 7/11/08 can take up DNA. The results of this test can be seen here.

Discussion

Quote of the Day

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

• Printable version
• Permanent link
• Privacy policy
• Disclaimers