User:Karmella Haynes/Notebook/BioBrick cloning/2013/01/05

01/05/13

• Golden gate: PCR parts, complete protocol for Brady's construct
• Gibson: PCR parts; waiting on BsmBI from NEB

Gibson Assembly

1. hPCD + BL01 + V0120
2. hPCD + BL01 + pSB1A3

PCR

1. V0120, Gib_BBS F (Gib0001) / Gib_BBP R (Gib0002)
2. pSB1A3, Gib_BBS F (Gib0001) / Gib_BBP R (Gib0002)
3. hPCD, BBP-hPCD fwd (BL9) / hPCD-BL01 rev (BL7)
4. BL01, hPCD-BL01 fwd (BL8) / BL01-BBS rev (BL10)

• 95°C, 3 min.
• [95°C, 30 sec.; 57°C, 30 sec.; 72°C, 2 min.] x 30
• 72°C, 3 min.
• 4°C, ∞

Measure DNA Concentrations

Reaction set-up

• Use 0.2 - 0.5 pmol, per NEB's suggestion
• pmols = ng x 1000 / bp x 650 daltons; ng = (pmols x bp x 650 daltons) / 1000
• Total volume of DNA = 5.0 μL max

1. hPCD + BL01 + V0120

• vector V0120, 0.1 pmol = 208 ng = 1.9 μL (use 1.4 μL)
• 2:1 insert hPCD, 0.2 pmol = 24 ng = 0.7 μL
• 2:1 insert BL01, 0.2 pmol = 328 ng = 2.9 μL

2. hPCD + BL01 + V0120

• vector pSB1A3, 0.1 pmol = 130 ng = 1.3 μL
• 2:1 insert hPCD, 0.2 pmol = 24 ng = 0.7 μL (use 0.8 μL)
• 2:1 insert BL01, 0.2 pmol = 328 ng = 2.9 μL

Gibson reactions:

1. hPCD + BL01 + V0120
2. V0120
3. hPCD + BL01 + pSB1A3
4. pSB1A3

• Add each to one aliquot of 15.0 Gibson mix (Rene); total = 20.0 μL
• Thermal cycler: 50°C,60 min.; 4°C, ∞
• Transform

Golden Gate Assembly

• Try new protocol from Dave Savage

1. hPCD + BL01 + V0120
2. hPCD + BL01 + pSB1A3

• Check the sequences for BsmBI sites!

PCR

1. V0120, gg_BBS F (gg0001) / gg_BBP R (gg0002)
2. pSB1A3, gg_BBS F (gg0001) / gg_BBP R (gg0002)
3. hPCD, gg_BBP-hPCD F (gg0003) / gg_hPCD-BL01 R (gg0004)
4. BL01, gg_BL01 F (gg0004) / gg_BL01-BBS R (gg0005)

• 95°C, 3 min.
• [95°C, 30 sec.; 57°C, 30 sec.; 72°C, 2 min.] x 30
• 72°C, 3 min.
• 4°C, ∞

Measure DNA Concentrations