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Contents 1 Lab protocols 1.1 Preparation of chemocompetent DH5-alpha cells 1.2 Retransformation of BioBricks 1.3 Transformation of Ligations (in DH5alpha or XL1Blue) 1.4 Mini-Prep (Promega) 1.5 Midi-Prep (Promega) 1.6 Glycerol Stocks (iGEM)

Lab protocols

On this page you can find a list of important standard protocols we used in our project.

Preparation of chemocompetent DH5-alpha cells

• liquid cultures, OD_600 of 0,6-0,8
• centrifugation at 4 °C, 4500 g, 10 min
• decantation
• resuspend with 40 ml inoune transformation buffer
• repeat centrifugation, decantation and resuspendation
• centrifuge and decantate again
• resuspend in 20 ml inoune transformation buffer
• add 1,5 ml DMSO
• shock freeze in liquid nitrogen

Retransformation of BioBricks

• add 10 µl sterile dest water to DNA on plate
  • incubate for 10 min
  • take 2 µl, leave rest on plate
  • store plates at -20 °C
• add the 2 µl DNA solution to 5 µl competent DH5-alpha
  • incubate for 30 min on ice
  • heat shock for 45 s at 42 °C
  • incubate 3 min on ice
  • add 250 µl LB medium of 37 °C
  • incubate for 45 min at 37 °C, 800 rpm

Transformation of Ligations (in DH5alpha or XL1Blue)

• thaw bacteria on ice or carefully in your hand
• add 2-4µl Ligation mixture to 50µl bacteria
• incubate 30min on ice
• heat shock 30s-45s (XL1Blue preferably 35s) at 42°C
• incubate 6min on ice
• add 250µl prewarmed LB medium (37°C)
• incubate for 45min at 37°C, 800rpm
• plate 300µl on apropiate antibiotic
• dry 15min at room temperature
• incubate at 37°C over night

Mini-Prep (Promega)

• add 1,5 ml cell culture in an eppi
• zentrifuge for 30 sec, max speed
• decantate
• resuspend with 600 µl dest water
• ad 100 µl cell lysis buffer
• after ca. 1 min add 350 µl of neutralization buffer
• centrifuge 3min maximum speed
• put Minicolumn into Collection Tube and transfer supernatant into PureYield^TM Minicolumn
• centrifuge for 15 sec at max speed
• centrifuge for 15 sec at max speed with 200 µl Endotoxin Removal Wash
• centrifuge for 30 sec at max speed with 400 µl Column Wash solution
• put Minicolum into new eppi, abolish liquid
• transfer 30 µl elution buffer into Minicolum, wait for 1 min
• centrifuge for 15 sec at max speed
• store DNA at -20 °C

Midi-Prep (Promega)

• centrifuge 50 ml of liquid cell culture for 10min at 5000g
• decantate
• resuspend with 3 ml resuspension solution
• add 3 ml cell lysis solution and incubate for maximal 3 min at room temperature
• add 5 ml neutralization solution
• centrifuge for 20 min at 20 °C, 5000g
• vacuum pump lysat through cleaning column into binding column
• abolish cleaning column
• vacuum pump with 10 ml endotoxin removal wash solution
• vacuum pump with 20 ml column wash solution
• dry membrane by vacuum
• dd 600 µl nuclease free water on membrane
• centrifuge for 5 min at 1750 g into eppi

Glycerol Stocks (iGEM)

• autoclave glycerol (60%)
• add 1,5 ml cell culture and 0,5 ml Glycerol in a kryo tube
• vortexe
• shock freeze in liquid nitrogen
• store at -80 °C