Team:Michigan/Pili August September
From 2010.igem.org
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'''Miniprep pBAD plasmid''' | '''Miniprep pBAD plasmid''' | ||
- | # | + | #Inoculate 5.0mL LB in 50mL conical tubes w/ 100ug/mL of ampilicin |
- | ## | + | ##The cultures (2 of them) grew for ~12hrs (8am to 8pm). |
- | # | + | #Centrifuge (using the 50mL conical tubes) for 5000rpm for 10min at 4ºC |
- | # | + | #Carefully discard the supernatant and resuspend the pellet with 250uL of P1 buffer (kept in the 4ºC fridge) |
- | # | + | #Transfer into a labelled 1.5mL eppendorf tube (set pipetman to 500uL just in case) |
- | # | + | #Add 250uL P2 Buffer--> invert 4-6times (should turn blue)--> add 350uL N3 buffer--> invert 4-6times (should become vicious or clumpy) |
- | ## | + | ##Centrifuge at 13,000 rpm for 10 min |
- | # | + | #Pipette out supernatant into a QIA spin column--> centrifuge for 60s--> discard flow through |
##did not pipet out all of the supernatant | ##did not pipet out all of the supernatant | ||
- | # | + | #Add 500uL PB buffer --> centrifuge 60s--> discard flow through |
- | # | + | #Add 750uL PE buffer--> centrifuge 60s--> discard--> centrifuge 60s again |
- | # | + | #Transfer into a labeled 1.5mL eppendorf tube--> add 50uL EB (elution buffer) |
- | ## | + | ##Allow it to sit for 1 min (it helps to release the DNA from the column) |
'''fimB PCR product Purification''' | '''fimB PCR product Purification''' | ||
#Used sample A and B of PCR product (save C and D for later) | #Used sample A and B of PCR product (save C and D for later) | ||
- | ## | + | ##Total volume of PCR product = 81 uL (40.5uL separately) |
- | # | + | #Add 5 volumes of PB buffer (202.5uL) to 1 volume of PCR product (40.5uL); invert |
- | # | + | #Transfer into a QIAquick spin column (provided in the Qiagen kit) |
- | ## | + | ##Set pipetman to 260uL to be sure to get all of the mixture |
- | # | + | #Centrifuge spin column at 13,000rpm for 60s |
- | # | + | #Discard the flow through (in the collection tube) and add 750uL PE buffer (to wash the DNA) |
- | + | Repeat step 4 again | |
- | # | + | #Discard flow through and centrifuge again to get the remain buffers out |
- | # | + | #Place the column into a labeled 1.5mL eppendorf tube |
- | # | + | #Add 50uL EB buffer (to elute out the DNA) directly to the white inner circle of the column (avoid touching the pipet tip to the column) |
- | ## | + | ##Allow the mix to sit in the column for 1 min, then centrifuge for 1 min (13,000rpm) |
- | ## | + | ##Remember to point the cap of the eppendorf tube in the opposite direction of the centrifuge machine |
'''fimB Digest''' | '''fimB Digest''' | ||
- | # | + | #Pre-programmed PCR machine to Digest (DIG1) |
- | # | + | #Use 5 PCR reaction tubes for each; 5 for fimB and 5 for pBAD |
- | # | + | #Add the following amounts in that order (total volume of 20uL) |
*16 uL of the DNA (fimB and pBAD to their respective tubes) | *16 uL of the DNA (fimB and pBAD to their respective tubes) | ||
*2 uL of NEB 2 buffer | *2 uL of NEB 2 buffer | ||
*1 uL NcoI | *1 uL NcoI | ||
*1uL HindIII | *1uL HindIII | ||
- | # | + | #Incubate for 37ºC overnight (12hrs) |
- | ## | + | ##Place into 4ºC fridge the next day |
==8/16/2010== | ==8/16/2010== |
Revision as of 03:00, 27 October 2010