Team:BYU Provo/Team Thermosensor/The Beginning
From 2011.igem.org
(Difference between revisions)
Cheddar3210 (Talk | contribs) |
Cheddar3210 (Talk | contribs) |
||
Line 11: | Line 11: | ||
<div id='pageContents'> | <div id='pageContents'> | ||
+ | |||
+ | ==Week Feb. 21 – 27== | ||
+ | |||
+ | * Feb. 22 | ||
+ | ** Made PCR for thermosensor will check prouct tomorrow | ||
+ | * Feb. 23 | ||
+ | ** PCR products checked, thermosensor appears to have been amplified correctly | ||
+ | ** pPLAT extracted via qiaprep plasmid prep protocol | ||
+ | |||
+ | |||
+ | ==Week Feb. 28 – Mar. 6== | ||
+ | |||
+ | * Feb. 28 | ||
+ | ** Phusion PCR for GFP in Thermosensor system | ||
+ | *** ~35 uL ddH2O | ||
+ | *** 10uL 5X phusion buffer | ||
+ | *** 1.5uL 10mM dNTP’s | ||
+ | *** 1uL each primer | ||
+ | *** 1uL of diluted template DNA | ||
+ | *** 0.5 uL phusion polymerase | ||
+ | ** Purified PCR samples according to Qiagen Kit | ||
+ | ** Restriction Digest of insert and vector inserting thermosensor into pPLAT | ||
+ | *** PCR product(insert) digestion (50uL rxn) | ||
+ | **** ~14uL H2O | ||
+ | **** 5uL 10X NEB buffer | ||
+ | **** 0.5 uL 100X BSA | ||
+ | **** 30uL DNA sample | ||
+ | **** 1-2uL each restriction enzyme | ||
+ | *** Vector Digestion (50uL rxn) | ||
+ | **** ~14uL H2O | ||
+ | **** 5uL 10X NEB buffer | ||
+ | **** .5 uL 100X BSA | ||
+ | **** 30uL DNA sample | ||
+ | **** 1-2 uL each restriction enzyme | ||
+ | ***** Placed reactions in 37o bath for 1.5 hr+ | ||
+ | |||
+ | * Mar. 2 | ||
+ | ** Restriction Digests actually done today | ||
+ | ** Running a gel of purified thermoswitch and purified GFP | ||
+ | *** (thermoswitch in 3rd well and GFP in 5th well) | ||
+ | |||
+ | * Mar. 4 | ||
+ | ** Product from redo thermoswitch PCR | ||
+ | |||
+ | |||
+ | ==Week Mar. 21 – 27== | ||
+ | |||
+ | * Mar. 23 | ||
+ | ** Low Melt gel ran on vector and insert, bands cut out and gel cut-outs melted at 65oC | ||
+ | ** Received pGLO from Dr. Grose on Monday to be transformed into competent cells to act as a positive control for GFP | ||
+ | ** pPLAT can be transformed into competent cells(DH5-a) as a neg. control | ||
+ | *** (GFP was more widely used by the OxyR team so they did the transformation of pGLO into competent cells) | ||
+ | ** Began ligation for pPLAT and pBAD cut at BamHI and EcoRI | ||
+ | *** 6.5 uL H2O | ||
+ | *** 1.5uL 10X ligase buffer | ||
+ | *** 1 uL T4 DNA ligase | ||
+ | *** 3uL vector | ||
+ | *** 3uL insert (didn’t put insert in control) | ||
</div> | </div> |
Latest revision as of 02:20, 24 September 2011
|
Week Feb. 21 – 27
- Feb. 22
- Made PCR for thermosensor will check prouct tomorrow
- Feb. 23
- PCR products checked, thermosensor appears to have been amplified correctly
- pPLAT extracted via qiaprep plasmid prep protocol
Week Feb. 28 – Mar. 6
- Feb. 28
- Phusion PCR for GFP in Thermosensor system
- ~35 uL ddH2O
- 10uL 5X phusion buffer
- 1.5uL 10mM dNTP’s
- 1uL each primer
- 1uL of diluted template DNA
- 0.5 uL phusion polymerase
- Purified PCR samples according to Qiagen Kit
- Restriction Digest of insert and vector inserting thermosensor into pPLAT
- PCR product(insert) digestion (50uL rxn)
- ~14uL H2O
- 5uL 10X NEB buffer
- 0.5 uL 100X BSA
- 30uL DNA sample
- 1-2uL each restriction enzyme
- Vector Digestion (50uL rxn)
- ~14uL H2O
- 5uL 10X NEB buffer
- .5 uL 100X BSA
- 30uL DNA sample
- 1-2 uL each restriction enzyme
- Placed reactions in 37o bath for 1.5 hr+
- PCR product(insert) digestion (50uL rxn)
- Phusion PCR for GFP in Thermosensor system
- Mar. 2
- Restriction Digests actually done today
- Running a gel of purified thermoswitch and purified GFP
- (thermoswitch in 3rd well and GFP in 5th well)
- Mar. 4
- Product from redo thermoswitch PCR
Week Mar. 21 – 27
- Mar. 23
- Low Melt gel ran on vector and insert, bands cut out and gel cut-outs melted at 65oC
- Received pGLO from Dr. Grose on Monday to be transformed into competent cells to act as a positive control for GFP
- pPLAT can be transformed into competent cells(DH5-a) as a neg. control
- (GFP was more widely used by the OxyR team so they did the transformation of pGLO into competent cells)
- Began ligation for pPLAT and pBAD cut at BamHI and EcoRI
- 6.5 uL H2O
- 1.5uL 10X ligase buffer
- 1 uL T4 DNA ligase
- 3uL vector
- 3uL insert (didn’t put insert in control)