User:Kathryn Muratore/Notebook/AU CHEM-570 lab prep/2011/07/05

Objective

Add today's objective(s) here...

Bench work

1. Analytical gel
   1. ladder
   2. --
   3. Matt Hartings' sample
   4. - 6. --
   7. 5μL 1:10 pTXB1His
   8. 2.5μL gel-purified double-digested insert from last week
   9. 2.5μL gel-purified double-digested vector(His) from last week
   10. 2.5μL gel-purified double-digested vector from last week
   11. 5μL V(His)+I ligation from last week
   12. 5μL V+I ligation from last week
2. → 50' @ 90V
3. → stain in EtBr
4. Transformation
   1. 100μL DH10B + 5μL V(His)+I from last week (same as what is on gel)
   2. 100μL DH10B + 5μL V+I from last week (same as what is on gel)
   3. 100μL DH10B + 5μL V(His) neg ctrl from last week
   4. 100μL DH10B + 5μL V neg ctrl from last week
   • heat shock is 45s @ 42°C
   • plate 100μL on LBAmp¹⁰⁰
   • → 37°C O/N
5. Miniprep
   1. 10 mL LB + 10μL Amp¹⁰⁰ + V+I in DH10B colony from last week's transformation (100μL plate)
   2. 10 mL LB + 10μL Amp¹⁰⁰ + V+I in NovaBlue colony from last week's transformation, but the 450μL re-plate
   • → 37°C O/N w/ shaking

Results

• can't see undigested vector
• gel-purified samples did not float away and are visible on gel (good!)
• clearly see insert and double-inserts (~3kb). Faint band visible at correct size for vector+insert ligation (~7kb) but hard to see in photo.