Team:Heidelberg/Notebook synthetic promoters dna
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__NOTOC__ | __NOTOC__ | ||
- | + | =='''Contents'''== | |
+ | {| class="wikitable centered" border="2" rules="rows" width="850px" style="border-color:white;" | ||
+ | |- | ||
+ | ! Week !! colspan="7" |Days | ||
+ | |- | ||
+ | |style="text-align:center"| 25 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-15-2009|6-15-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-16-2009|6-16-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-17-2009|6-17-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-18-2009|6-18-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |style="text-align:center"| 26 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-22-2009|6-22-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-23-2009|6-23-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-24-2009|6-24-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-25-2009|6-25-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-26-2009|6-26-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |style="text-align:center"| 27 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-29-2009|6-29-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#6-30-2009|6-30-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-01-2009|7-01-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-02-2009|7-02-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-03-2009|7-03-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-04-2009|7-04-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-05-2009|7-05-2009]] | ||
+ | |- | ||
+ | |style="text-align:center"| 28 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-06-2009|7-06-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-07-2009|7-07-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-08-2009|7-08-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-09-2009|7-09-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |style="text-align:center"| 30 | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-23-2009|7-23-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-24-2009|7-24-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |style="text-align:center"| 31 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-27-2009|7-27-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-28-2009|7-28-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-29-2009|7-29-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-30-2009|7-30-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#7-31-2009|7-31-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-01-2009|8-01-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-02-2009|8-02-2009]] | ||
+ | |- | ||
+ | |style="text-align:center"| 32 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-03-2009|8-03-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-04-2009|8-04-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-05-2009|8-05-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |style="text-align:center"| 33 | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-11-2009|8-11-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-12-2009|8-12-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-13-2009|8-13-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-14-2009|8-14-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-15-2009|8-15-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-16-2009|8-16-2009]] | ||
+ | |- | ||
+ | |style="text-align:center"| 34 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-17-2009|8-17-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-18-2009|8-18-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-19-2009|8-19-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-20-2009|8-20-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-21-2009|8-21-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | | | ||
+ | |- | ||
+ | |style="text-align:center"| 35 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-24-2009|8-24-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-25-2009|8-25-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-26-2009|8-26-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-27-2009|8-27-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-28-2009|8-28-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-29-2009|8-29-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |style="text-align:center"| 36 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#8-31-2009|8-31-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-01-2009|9-01-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-02-2009|9-02-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-03-2009|9-03-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-04-2009|9-04-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-06-2009|9-06-2009]] | ||
+ | |- | ||
+ | |style="text-align:center"| 37 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-07-2009|9-07-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-08-2009|9-08-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-09-2009|9-09-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-10-2009|9-10-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |style="text-align:center"| 38 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-14-2009|9-14-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-15-2009|9-15-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-16-2009|9-16-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-18-2009|9-18-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-20-2009|9-20-2009]] | ||
+ | |- | ||
+ | |style="text-align:center"| 39 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-21-2009|9-21-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |style="text-align:center"| 40 | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_synthetic_promoters_dna#9-30-2009|9-30-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |} | ||
== 6-15-2009 == | == 6-15-2009 == | ||
- | |||
- | |||
- | |||
- | |||
* Miniprep of GFP template plasmid, pcDNA5/FRT | * Miniprep of GFP template plasmid, pcDNA5/FRT | ||
{| class="wikitable" border="1" | {| class="wikitable" border="1" | ||
Line 37: | Line 177: | ||
|- | |- | ||
|} | |} | ||
- | * Maxiprep pcDNA/FRT 188.7ng/µL | + | * Maxiprep pcDNA/FRT 188.7ng/µL |
- | + | ||
- | + | ||
- | + | ||
* Extraction of CMV promoter from 2008 distribution | * Extraction of CMV promoter from 2008 distribution | ||
* Transformation of DH5a cell with CMV promoter | * Transformation of DH5a cell with CMV promoter | ||
== 6-16-2009 == | == 6-16-2009 == | ||
- | |||
- | |||
* DNA synthesis (JeT, cFos, Min) | * DNA synthesis (JeT, cFos, Min) | ||
Line 57: | Line 192: | ||
== 6-17-2009 == | == 6-17-2009 == | ||
- | |||
- | |||
* No transformations could be observed | * No transformations could be observed | ||
* Replace Phsuion stocks to Phusion Master Mix from Nathan | * Replace Phsuion stocks to Phusion Master Mix from Nathan | ||
* Repeat DNA synthesis with a different protocol: 1:10 - 1:1000 dilution of Oligos, 95° 5', 7* [95° 45'' 58° 45'' 72° 1'], add 1:10 diluted primers, 95° 5' 25* same temperatures | * Repeat DNA synthesis with a different protocol: 1:10 - 1:1000 dilution of Oligos, 95° 5', 7* [95° 45'' 58° 45'' 72° 1'], add 1:10 diluted primers, 95° 5' 25* same temperatures | ||
* Annealing successful for JeT and Min | * Annealing successful for JeT and Min | ||
- | + | Annealing might not have been successful with Fos beacuse it contains a very repetetive proximal promoter. | |
- | [Bild1.jpg|none|frame|Lanes 1-6 Fos (403 Bp); Lanes 7-12 JeT (227 Bp): Lanes 13-18: Min (207 Bp) Lanes 1 : 1µL of 1 :10 diluted oligo 2 : 1 :100 3 : 1 :1000 ;4-6 same, but + DMSO Lanes 7,8,13,14: 1:10 Lanes 9,10,15,16: 1:100 Lanes 11,12,17,18: 1:1000 Even lanes: No DMSO Uneven lanes: DMSO] | + | [[Image:Bild1.jpg|none|frame|Lanes 1-6 Fos (403 Bp); Lanes 7-12 JeT (227 Bp): Lanes 13-18: Min (207 Bp) Lanes 1 : 1µL of 1 :10 diluted oligo 2 : 1 :100 3 : 1 :1000 ;4-6 same, but + DMSO Lanes 7,8,13,14: 1:10 Lanes 9,10,15,16: 1:100 Lanes 11,12,17,18: 1:1000 Even lanes: No DMSO Uneven lanes: DMSO]] |
* gel purfifcation of JeT and Min | * gel purfifcation of JeT and Min | ||
- | * Repeat PCR of pcDNA5/FRT and mcherry with lower annealing temperature (58°C) and fresh Polymerase: Follow PCR protcol from Strategene site directed mutagenesis kit. | + | * Repeat PCR of pcDNA5/FRT and mcherry with lower annealing temperature (58°C) and fresh Polymerase: Follow PCR protcol from Strategene site directed mutagenesis kit. mcherry PCR might not have been successful because we used a template we didn't make ourselves - does it contain TE? |
- | + | ||
- | we used a template we didn't make ourselves - does it contain TE? | + | |
* PCR worked for pcDNA5FRT but not for mcherry | * PCR worked for pcDNA5FRT but not for mcherry | ||
* DpnI digest of pcDNA5FRT 1,3,4,6 | * DpnI digest of pcDNA5FRT 1,3,4,6 | ||
Line 74: | Line 205: | ||
== 6-18-2009 == | == 6-18-2009 == | ||
- | |||
* DNA synthesis for Fos (proximal) and Fos (core) | * DNA synthesis for Fos (proximal) and Fos (core) | ||
[[Image:Bild3.jpg|none|frame|Left two lanes: Proximal (repetetive), right two lanes (core)]] | [[Image:Bild3.jpg|none|frame|Left two lanes: Proximal (repetetive), right two lanes (core)]] | ||
* Transformation of DH5a with pcDNA/FRT ΔPstI | * Transformation of DH5a with pcDNA/FRT ΔPstI | ||
- | + | Gave many 1000 colonies. Probably a contamination (?), whci hwould explain why there was no mutagenesis (see below) | |
* HeLa cells, MCS7 and U20S were splitted 1:3. Therefore DEMED medium (containing additionally 10% FCS, Pen-Strep, glutamate and non-essential aminoacids) was removed. Cells were washed afterwards with HBSS and trypsinised with 1 ml of trypsin and incubated for 5 min. at 37°C 5% CO2. The used flasks were filled up to a final volume of 7 ml with DMEM. 2 ml of the suspension was transfered to a new flask, 5 ml DMEM was added and incubated for another 3-4 days at 37°C and 5% CO2. | * HeLa cells, MCS7 and U20S were splitted 1:3. Therefore DEMED medium (containing additionally 10% FCS, Pen-Strep, glutamate and non-essential aminoacids) was removed. Cells were washed afterwards with HBSS and trypsinised with 1 ml of trypsin and incubated for 5 min. at 37°C 5% CO2. The used flasks were filled up to a final volume of 7 ml with DMEM. 2 ml of the suspension was transfered to a new flask, 5 ml DMEM was added and incubated for another 3-4 days at 37°C and 5% CO2. | ||
== 6-22-2009 == | == 6-22-2009 == | ||
- | |||
* Split cells (Split again Thursday!) | * Split cells (Split again Thursday!) | ||
* Prepare 6well-plate with U20S cells for Zeomycine assay | * Prepare 6well-plate with U20S cells for Zeomycine assay | ||
Line 92: | Line 221: | ||
== 6-23-2009 == | == 6-23-2009 == | ||
- | |||
[[Image:Bild2.jpg|none|frame|2: pcDNA S-1; 3: pcDNA S-4; 4: pcDNA S-2; 5: pcDNA S-3 6:pcDNA S-5 7: pcDNA S-6 8: pcDNA S-7 9: pcDNA S-8; 10: mCherry D-1 11: mcherry S-2; 12: mcherry S-3; 13: pcDNA D-1 14: pcDNA D-2 '''15: pcDNA control 16: mcherry control''']] | [[Image:Bild2.jpg|none|frame|2: pcDNA S-1; 3: pcDNA S-4; 4: pcDNA S-2; 5: pcDNA S-3 6:pcDNA S-5 7: pcDNA S-6 8: pcDNA S-7 9: pcDNA S-8; 10: mCherry D-1 11: mcherry S-2; 12: mcherry S-3; 13: pcDNA D-1 14: pcDNA D-2 '''15: pcDNA control 16: mcherry control''']] | ||
* Added Zeomycine to 6-well platees | * Added Zeomycine to 6-well platees | ||
Line 101: | Line 229: | ||
== 6-24-2009 == | == 6-24-2009 == | ||
- | |||
* DpnI digest | * DpnI digest | ||
* Transformation of Supercompetent Gold TOP10 cells with pcDNA5 ΔEcoRI ΔPstI | * Transformation of Supercompetent Gold TOP10 cells with pcDNA5 ΔEcoRI ΔPstI | ||
Line 118: | Line 245: | ||
* Miniprep, Test digest with EcoRI | * Miniprep, Test digest with EcoRI | ||
- | [ | + | [[Image:HD09_Bild4.jpg|none|frame|Lane 1: Ladder; Lane 3: Control; Lane 4-12: Clones of site directed mutagenesis to remove EcoRI]] |
== 6-29-2009 == | == 6-29-2009 == | ||
Line 128: | Line 255: | ||
* Digest pcDNA with BclI -> BclI does not cut -> cloning strategy must be changed to use ApaI instead of BclI (new primers designed and ordered) | * Digest pcDNA with BclI -> BclI does not cut -> cloning strategy must be changed to use ApaI instead of BclI (new primers designed and ordered) | ||
* Gel purification of vector backbone | * Gel purification of vector backbone | ||
- | [Image: | + | [[Image:HD09_Bild5.jpg|none|frame|Lane 2+3: Preparation of Vector backbone after MfeI/PstI digest; Lane 5: plasmid (pcDNA5/FRT ...) Lane 6: BclI digest of plasmid (same behaviour as Lane 5)]] |
* Ligation of pcDNA5/FRT ΔPstI ΔEcoRI -MCS with JeT and Min promoters | * Ligation of pcDNA5/FRT ΔPstI ΔEcoRI -MCS with JeT and Min promoters | ||
- | |||
== 6-30-2009 == | == 6-30-2009 == | ||
Line 139: | Line 265: | ||
* PCR of mcherry, GFP | * PCR of mcherry, GFP | ||
- | == 7- | + | == 7-01-2009 == |
* Miniprep of pcDNA5/FRT ΔPstI ΔEcoRI JeT, pcDNA5/FRT ΔPstI ΔEcoRI Min, pcDNA5/FRT ΔPstI ΔEcoRI (all unmethylated) | * Miniprep of pcDNA5/FRT ΔPstI ΔEcoRI JeT, pcDNA5/FRT ΔPstI ΔEcoRI Min, pcDNA5/FRT ΔPstI ΔEcoRI (all unmethylated) | ||
Line 147: | Line 273: | ||
* mcherry PCR worked, GFP didn't | * mcherry PCR worked, GFP didn't | ||
- | == 7- | + | == 7-02-2009 == |
* Digest pcDNA5/FRT ΔPstI ΔEcoRI from -dam strains with BclI and PstI, Same for mcherry PCR | * Digest pcDNA5/FRT ΔPstI ΔEcoRI from -dam strains with BclI and PstI, Same for mcherry PCR | ||
Line 154: | Line 280: | ||
* Transformation | * Transformation | ||
- | == 7- | + | == 7-03-2009 == |
- | + | ||
- | + | ||
* Colony PCR - Colonies 1,2,3,8,10 are promising (to be picked, mini-prepped and test-digested) | * Colony PCR - Colonies 1,2,3,8,10 are promising (to be picked, mini-prepped and test-digested) | ||
* Transformation of DH5a with Part BBa_E0040 (GFP) | * Transformation of DH5a with Part BBa_E0040 (GFP) | ||
- | + | == 7-04-2009 == | |
- | == 7- | + | |
- | + | ||
- | + | ||
* Inoculation of LB-Amp media with colony 1,2,3,7,8 and 9 | * Inoculation of LB-Amp media with colony 1,2,3,7,8 and 9 | ||
* Incubation over night at 37°C | * Incubation over night at 37°C | ||
- | == 7- | + | == 7-05-2009 == |
- | + | ||
- | + | ||
* Miniprep of overnight culture | * Miniprep of overnight culture | ||
Line 178: | Line 297: | ||
* 6-well plates with the human cell lines were started for transfection (~10^5 cells per well) | * 6-well plates with the human cell lines were started for transfection (~10^5 cells per well) | ||
* Agerose Gelelktrophorese | * Agerose Gelelktrophorese | ||
- | [ | + | [[Image:HD09_Bild6.jpg|none|frame|(lane 1 marker; lane 2 control (undigested); lane 3 colony 1; lane 4 colony 2, lane 5 colony 3; lane 6 colony 7/1; lane 7 colony 7/2; lane 8 colony 8; lane 9 colony 9]] |
- | ] | + | |
- | == 7- | + | == 7-06-2009 == |
- | + | ||
- | + | ||
* Digest pcDNA5/FRT ΔPstI ΔEcoRI mcherry(PstI-BclI), JeT and Edelman/Min with PstI and MfeI | * Digest pcDNA5/FRT ΔPstI ΔEcoRI mcherry(PstI-BclI), JeT and Edelman/Min with PstI and MfeI | ||
Line 191: | Line 307: | ||
* Transfect HeLa, U20s and MCS7 cells with pROG4 (??) for stable integration of a FRT site | * Transfect HeLa, U20s and MCS7 cells with pROG4 (??) for stable integration of a FRT site | ||
- | == 7- | + | == 7-07-2009 == |
- | + | ||
- | + | ||
* HeLa cells, MCS7 and U20S were splitted 1:5 (see above) | * HeLa cells, MCS7 and U20S were splitted 1:5 (see above) | ||
Line 202: | Line 316: | ||
* Inoculation of medium with colonies (pcDNA5/FRT ΔPstI ΔEcoRI mcherry-min-ligation / pcDNA5/FRT ΔPstI ΔEcoRI mcherry-JeT-ligation) | * Inoculation of medium with colonies (pcDNA5/FRT ΔPstI ΔEcoRI mcherry-min-ligation / pcDNA5/FRT ΔPstI ΔEcoRI mcherry-JeT-ligation) | ||
- | == 7- | + | == 7-08-2009 == |
- | + | ||
- | + | ||
* Digest P.8 (GFPb3mut) PCR (O.47 and O.48) product with Bcl and PstI | * Digest P.8 (GFPb3mut) PCR (O.47 and O.48) product with Bcl and PstI | ||
Line 212: | Line 324: | ||
* Test digest of pcDNA5/FRT ΔPstI ΔEcoRI mcherry-min-ligation / Jet-ligation -> ligation worked (checked by gel) | * Test digest of pcDNA5/FRT ΔPstI ΔEcoRI mcherry-min-ligation / Jet-ligation -> ligation worked (checked by gel) | ||
- | == 7- | + | == 7-09-2009 == |
- | + | ||
- | + | ||
* Randomized promoter synthesis of HIF-1 using | * Randomized promoter synthesis of HIF-1 using | ||
Line 229: | Line 339: | ||
* Digestion of P.9 with ScaI | * Digestion of P.9 with ScaI | ||
* Transfection with P.9 for stable integration; Transfection with mcherry - Jet/min ligation (transient) | * Transfection with P.9 for stable integration; Transfection with mcherry - Jet/min ligation (transient) | ||
- | [ | + | [[Image:HD09_Bild7.jpg|none|frame| From left to right: 2* no DMSO , 2* DMSO; 1:4 1:10 1:4 1:10]] |
Notice that indeed this is no smear but individual bands. | Notice that indeed this is no smear but individual bands. | ||
== | == | ||
- | |||
== 7-23-2009 == | == 7-23-2009 == | ||
- | |||
- | |||
* Retrace and comprehend last weeks' doings | * Retrace and comprehend last weeks' doings | ||
Line 246: | Line 353: | ||
== 7-24-2009 == | == 7-24-2009 == | ||
- | |||
- | |||
* start new cell culture (new media, new cells (HeLa, U2OS from Michaela)...) | * start new cell culture (new media, new cells (HeLa, U2OS from Michaela)...) | ||
- | + | * glutamine and trypsin aliquots are now in freezer II (drawer #3) | |
* pick transformed cells (had single colonies with plasmid 6 as well as with pSB1A3) and culture during the day (5 ml in 37°C incubator with rotation) | * pick transformed cells (had single colonies with plasmid 6 as well as with pSB1A3) and culture during the day (5 ml in 37°C incubator with rotation) | ||
* synthesize I_pSB1A3 and I_pcDNA from oligos (I_pSB1A3 and I_pcDNA contain BBb standard) twice (first try didn't work) | * synthesize I_pSB1A3 and I_pcDNA from oligos (I_pSB1A3 and I_pcDNA contain BBb standard) twice (first try didn't work) | ||
* maxi (250 ml w/ 250 µl Amp and 2,5 ml pre-culture) --> incubate over night | * maxi (250 ml w/ 250 µl Amp and 2,5 ml pre-culture) --> incubate over night | ||
- | + | * those inserts and the according vector will be digested with SspI and PciI (pSB1A3) or SspI and SphI (plasmid 6) respectively | |
== 7-27-2009 == | == 7-27-2009 == | ||
- | |||
- | |||
* PCR of EGFP with BclI/PstI primers | * PCR of EGFP with BclI/PstI primers | ||
Line 269: | Line 372: | ||
== 7-28-2009 == | == 7-28-2009 == | ||
- | |||
- | |||
* Gel electrophoresis of ligation (plasmid 6 + I_pcDNA separate, plasmid 6 + I_pcDNA ligated, pSB1A3 + I_pSB1A3 separated, pSB1A3 + I_pSB1A3 ligated) | * Gel electrophoresis of ligation (plasmid 6 + I_pcDNA separate, plasmid 6 + I_pcDNA ligated, pSB1A3 + I_pSB1A3 separated, pSB1A3 + I_pSB1A3 ligated) | ||
- | |||
* Purification of ligated plasmids with inserts from gel | * Purification of ligated plasmids with inserts from gel | ||
* transformation of the two ligated plasmids (plasmid 6 + I_pcDNA and pSB1A3 + I_pSB1A3), pFRT/lacZeo, mGFPc1, mGFPn2 | * transformation of the two ligated plasmids (plasmid 6 + I_pcDNA and pSB1A3 + I_pSB1A3), pFRT/lacZeo, mGFPc1, mGFPn2 | ||
Line 292: | Line 392: | ||
|- | |- | ||
|} | |} | ||
- | * made fresh LB-medium and LB-amp plates | + | * made fresh LB-medium and LB-amp plates |
== 7-29-2009 == | == 7-29-2009 == | ||
- | |||
- | |||
*Transformation of plasmid 6 + I_pcDNA, pSB1A3 + I_pSB1A3 did not work | *Transformation of plasmid 6 + I_pcDNA, pSB1A3 + I_pSB1A3 did not work | ||
Line 311: | Line 409: | ||
== 7-30-2009 == | == 7-30-2009 == | ||
- | |||
- | |||
*Over day culture of 8M1, 8M3, 8J4, 3J2 in SCS non-methylating cells | *Over day culture of 8M1, 8M3, 8J4, 3J2 in SCS non-methylating cells | ||
*transformation of plasmid6 with I_pcDNA, pSB1A3 with I_pSB1A3 in DH5α cells did not work, maybe mistake in ligation step | *transformation of plasmid6 with I_pcDNA, pSB1A3 with I_pSB1A3 in DH5α cells did not work, maybe mistake in ligation step | ||
*synthesis of I_pSB1A3 and I_pCDNA in two parts for each (idea: maybe previously synthesized inserts (I_pSB1A3 and I_pcDNA) were too long --> synthesize two shorter parts, digest them with EcoRI and ligate them) | *synthesis of I_pSB1A3 and I_pCDNA in two parts for each (idea: maybe previously synthesized inserts (I_pSB1A3 and I_pcDNA) were too long --> synthesize two shorter parts, digest them with EcoRI and ligate them) | ||
- | |||
- | |||
Line 353: | Line 447: | ||
== 7-31-2009 == | == 7-31-2009 == | ||
- | |||
- | |||
* yesterdays transformations did not seem to work (no colonies on any plates) - at 3pm, colonies were found | * yesterdays transformations did not seem to work (no colonies on any plates) - at 3pm, colonies were found | ||
Line 372: | Line 464: | ||
* 31.7.2 = Ligation of 8M3 + GFP (transformation tbd) | * 31.7.2 = Ligation of 8M3 + GFP (transformation tbd) | ||
- | == 8- | + | == 8-01-2009 == |
- | + | ||
- | + | ||
* Transform DH5a with 31.7.1, 31.7.2 | * Transform DH5a with 31.7.1, 31.7.2 | ||
- | == 8- | + | == 8-02-2009 == |
- | + | ||
- | + | ||
* Start Overnight cultures with 30.7.1, 30.7.2, 30.7.3, 30.7.5, 30.7.6, 30.7.7, 31.7.1, 31.7.2 | * Start Overnight cultures with 30.7.1, 30.7.2, 30.7.3, 30.7.5, 30.7.6, 30.7.7, 31.7.1, 31.7.2 | ||
- | == 8- | + | == 8-03-2009 == |
- | + | ||
- | + | ||
* Miniprep of 30.7.1, 30.7.2, 30.7.3, 30.7.5, 30.7.6, 30.7.7, 31.7.1, 31.7.2 | * Miniprep of 30.7.1, 30.7.2, 30.7.3, 30.7.5, 30.7.6, 30.7.7, 31.7.1, 31.7.2 | ||
Line 392: | Line 478: | ||
* Analytic digest with SspI/NheI for 30.7.5, 30.7.6 | * Analytic digest with SspI/NheI for 30.7.5, 30.7.6 | ||
* Gel, sequencing of pcDNA plasmids w/ Jet or Min and mCherry or GFP (test plasmid; also to be transformed tomorrow) | * Gel, sequencing of pcDNA plasmids w/ Jet or Min and mCherry or GFP (test plasmid; also to be transformed tomorrow) | ||
- | [ | + | [[Image:HD09_Bild9.jpg|none|frame| From left to right: 30.7.7#1-4 (used 30.7.7#2 as p.12); 31.7.1#1-4 (used 31.7.1#4 as p.30); 31.7.2#1-2; ladder; control (8M3, 3J2); 31.7.1#3,5-8 (used#6 as p.31); 30.7.1#1-4; 30.7.2#1 ]] |
- | [ | + | [[Image:HD09_Bild10.jpg|none|frame| From left to right: 30.7.2#2-4; 30.7.3#1-3; ladder; 8m3, 3j2 (control); pcdna5+1#1; psb1a3+I #1,2; pcdna5/FRT (control), psB1a3]] |
* insert synthesis for BBb-standardizing of submission and integration plasmids | * insert synthesis for BBb-standardizing of submission and integration plasmids | ||
* overnight culture of P.30, P.31 and P.13 (???) | * overnight culture of P.30, P.31 and P.13 (???) | ||
- | |||
- | + | == 8-04-2009 == | |
'''synthetic promoters''' | '''synthetic promoters''' | ||
Line 414: | Line 499: | ||
* Start overnight ligations | * Start overnight ligations | ||
- | == 8- | + | == 8-05-2009 == |
- | + | ||
- | + | ||
* over night culture (250 ml) of DH5alpha for new competent cells | * over night culture (250 ml) of DH5alpha for new competent cells | ||
Line 427: | Line 510: | ||
* Transformations of ligations | * Transformations of ligations | ||
- | |||
- | |||
- | |||
- | |||
- | |||
- | |||
== 8-11-2009 == | == 8-11-2009 == | ||
- | |||
- | |||
* 1. PCR-amplification of Jet promoter with primer 106 and 71 and template p31 | * 1. PCR-amplification of Jet promoter with primer 106 and 71 and template p31 | ||
Line 454: | Line 529: | ||
== 8-12-2009 == | == 8-12-2009 == | ||
- | |||
* PCR-amplification of CMV-promoter with primer 109 and 108 and template pcDNA5/FRT => failed => wrong primers | * PCR-amplification of CMV-promoter with primer 109 and 108 and template pcDNA5/FRT => failed => wrong primers | ||
Line 462: | Line 536: | ||
==8-13-2009== | ==8-13-2009== | ||
- | |||
* Minipreped 8 clones of pSB1A3 w/ BBbed Jet | * Minipreped 8 clones of pSB1A3 w/ BBbed Jet | ||
Line 469: | Line 542: | ||
==8-14-2009== | ==8-14-2009== | ||
- | |||
'''Promotors''' | '''Promotors''' | ||
Line 479: | Line 551: | ||
==8-15-2009== | ==8-15-2009== | ||
- | |||
* checked transfected cells of flourescence: both transfections with jet/EGFP in pCDNA5/FRT worked (green flourescence), positive controle worked | * checked transfected cells of flourescence: both transfections with jet/EGFP in pCDNA5/FRT worked (green flourescence), positive controle worked | ||
==8-16-2009== | ==8-16-2009== | ||
- | |||
* picked another 8 colonies from plates 3-5 (see 8-11-09) and started overnight culture | * picked another 8 colonies from plates 3-5 (see 8-11-09) and started overnight culture | ||
Line 551: | Line 621: | ||
* digested P.51 with NheI and SpeI --> gel purification | * digested P.51 with NheI and SpeI --> gel purification | ||
- | + | [[Image:08_26_09_p31_speI_NheI.jpg]] | |
* ligated correct BBbJet into P.31 and transformed | * ligated correct BBbJet into P.31 and transformed | ||
Line 700: | Line 770: | ||
** Empty S 1-4 | ** Empty S 1-4 | ||
** Empty L 1-6 | ** Empty L 1-6 | ||
- | |||
- | |||
- | |||
- | |||
- | |||
- | |||
- | |||
- | |||
- | |||
- | |||
- | |||
- | |||
- | |||
- | |||
== 8-31-2009 == | == 8-31-2009 == | ||
Line 740: | Line 796: | ||
* Transfections | * Transfections | ||
- | == 9- | + | == 9-01-2009 == |
'''Synthesis of HIF, p53, NFkB responsive promoters; constitutively active promoter; empty/random promoter:''' | '''Synthesis of HIF, p53, NFkB responsive promoters; constitutively active promoter; empty/random promoter:''' | ||
Line 753: | Line 809: | ||
{| class="wikitable" | {| class="wikitable" | ||
|- bgcolor=grey | |- bgcolor=grey | ||
- | ! height=20px, width= | + | ! height=20px, width=200px | || width=200px| || width=200px| |
|-align="center" | |-align="center" | ||
| style="font-weight:bold;" |Initiale denaturation || 95 °C, 5 min || 1 cycle | | style="font-weight:bold;" |Initiale denaturation || 95 °C, 5 min || 1 cycle | ||
Line 779: | Line 835: | ||
|} | |} | ||
- | == 9- | + | == 9-02-2009 == |
'''Synthesis of HIF, p53, NFkB responsive promoters; constitutively active promoter; empty/random promoter: Screening results''' | '''Synthesis of HIF, p53, NFkB responsive promoters; constitutively active promoter; empty/random promoter: Screening results''' | ||
Line 814: | Line 870: | ||
** NfkB again (less start and stop?) | ** NfkB again (less start and stop?) | ||
- | == 9- | + | == 9-03-2009 == |
'''New attempt to synthesize NFkB and p53 responsive promoters:''' | '''New attempt to synthesize NFkB and p53 responsive promoters:''' | ||
Line 852: | Line 908: | ||
[[Image:HD09_0209_remake.JPG|thumb|600px|none|'''Synthesis of p53, NFkB (I and II) promoters'''<br>1% agarose gel. Note that less short products exist due to lower concentrations of Stop 5 and Stop 3 oligos.]] | [[Image:HD09_0209_remake.JPG|thumb|600px|none|'''Synthesis of p53, NFkB (I and II) promoters'''<br>1% agarose gel. Note that less short products exist due to lower concentrations of Stop 5 and Stop 3 oligos.]] | ||
- | == 9- | + | == 9-04-2009 == |
'''New attempt to synthesize NFkB and p53 responsive promoters:''' | '''New attempt to synthesize NFkB and p53 responsive promoters:''' | ||
Line 865: | Line 921: | ||
* Screening of HIF: HeLa Cell line not suited, dies too fast in minimal media -> to be repeated in MCF-7 cells | * Screening of HIF: HeLa Cell line not suited, dies too fast in minimal media -> to be repeated in MCF-7 cells | ||
- | == 9- | + | == 9-06-2009 == |
'''New attempt to synthesize NFkB and p53 responsive promoters:''' | '''New attempt to synthesize NFkB and p53 responsive promoters:''' | ||
Line 876: | Line 932: | ||
** p53 L 18* | ** p53 L 18* | ||
- | == 9- | + | == 9-07-2009 == |
'''New attempt to synthesize NFkB and p53 responsive promoters:''' | '''New attempt to synthesize NFkB and p53 responsive promoters:''' | ||
Line 883: | Line 939: | ||
[[Image:HD09_0709gel.jpg|thumb|600px|none|'''Synthesis of p53, NFkB (I and II) promoters - test digest'''<br>1% agarose gel. Note that avg. product length is longer than in the previous synthesis round due to lower start/stop concentrations.]] | [[Image:HD09_0709gel.jpg|thumb|600px|none|'''Synthesis of p53, NFkB (I and II) promoters - test digest'''<br>1% agarose gel. Note that avg. product length is longer than in the previous synthesis round due to lower start/stop concentrations.]] | ||
- | == 9- | + | == 9-08-2009 == |
'''New attempt to synthesize NFkB and p53 responsive promoters:''' | '''New attempt to synthesize NFkB and p53 responsive promoters:''' | ||
* Transfections (+/- TNF-a for NFkB, +/- xxx for p53) | * Transfections (+/- TNF-a for NFkB, +/- xxx for p53) | ||
- | == 9- | + | == 9-09-2009 == |
'''Synthesizing AHR, SREBP and pPARy''' | '''Synthesizing AHR, SREBP and pPARy''' | ||
* Gene synthesis (compare Material and Methods) using the following oligo concentrations and a PCR purification step after the 1st seven cycles. | * Gene synthesis (compare Material and Methods) using the following oligo concentrations and a PCR purification step after the 1st seven cycles. | ||
Line 936: | Line 992: | ||
[[Image:HD09_1409_p53.jpg|thumb|800px|none|'''Screening of putative p53 regulated promoters'''. 1-6 corresponds to relative GFP expression strength levels.]] | [[Image:HD09_1409_p53.jpg|thumb|800px|none|'''Screening of putative p53 regulated promoters'''. 1-6 corresponds to relative GFP expression strength levels.]] | ||
- | |||
== 9-10-09 == | == 9-10-09 == | ||
Line 970: | Line 1,025: | ||
* Minipreps of second synthesis round for Estrogen Receptor, pPARγ and SREBP-regulated promoters | * Minipreps of second synthesis round for Estrogen Receptor, pPARγ and SREBP-regulated promoters | ||
[[Image:HD09 2009 gelimages.jpg|thumb|800px|none|'''Test digest of second synthesis round for nuclear recptor regulated promoters''' 1% agarose gel. Digest with HindIII and SpeI, 1h]] | [[Image:HD09 2009 gelimages.jpg|thumb|800px|none|'''Test digest of second synthesis round for nuclear recptor regulated promoters''' 1% agarose gel. Digest with HindIII and SpeI, 1h]] | ||
+ | |||
+ | == 9-21-09 == | ||
+ | |||
+ | Synthesis was remade for the Promoters stated above. We improved gel extraction quality. Still, quality synthesis remained low. We selected clones from the gel that were subjected to screening subsequently. Later, we found out that probably damaged HinDIII enzyme was responsible for the bad synthesis quality. | ||
== 9-30-09 == | == 9-30-09 == | ||
Line 985: | Line 1,044: | ||
- | |width=" | + | == October 2009 == |
+ | |||
+ | In the weeks before wiki freeze, selected promoters were characterized by the measurement subgroup (see [[Team:Heidelberg/Notebook_measure|their Notebook]] ). At the same time, further screenings were conducted as [[Team:Heidelberg/Notebook_MaM#Induction|described]] Also, some promoters were characterized roughly by triple TECAN-reads (namely, pPARγ and p53 responsive clones), or attempted to characterize in this was. We provide all spreadsheets thus generated in a two zip file: [[Media:HD09_raw.zip|raw data]] and [[Media:HD09_analyzed.zip|analyzed data]]. All Spreadsheets are commented with date of measurement. The only of those characterization which yielded reliable results we decided to publish on the registry is for pPARγ (see below or in [[Media:HD09_analyzed.zip|analyzed data]]). | ||
+ | [[Image:HD09_ppary_sheet.jpg|thumb|none|600px]] | ||
+ | |||
+ | |width="0" style="padding: 0 0px 0px 0px; background-color:#ede8e2"| | ||
|} | |} |
Latest revision as of 23:25, 21 October 2009
Contents
6-15-2009
6-16-2009
=> Only bands at ca. 50 Bp => no successful amplification
6-17-2009
Annealing might not have been successful with Fos beacuse it contains a very repetetive proximal promoter.
6-18-2009
Gave many 1000 colonies. Probably a contamination (?), whci hwould explain why there was no mutagenesis (see below)
6-22-2009
6-23-2009
6-24-2009
6-25-2009Split cells!
6-26-2009Change 6well plate medium!
6-29-2009
6-30-2009
7-01-2009
=> ligations had not worked
7-02-2009
7-03-2009
7-04-2009
7-05-2009
7-06-2009
7-07-2009
7-08-2009
7-09-2009
L1389.O53 HIF-1 a 4µL L1389.O54 HIF-1 b 4µL L1389.O55 Ap1 0,5µL L1389.O56 Random 9 µL L1389.O57 Sp1 0,5 µL L1389.O58 Stop3' 1 µL L1389.O59 Stop5' 1 µL To 200µL; dilute mix 1:10 7 cycles as described for gene synthesis (+/- DMSO), then add primers (O.58, O.59) 1:4 and 1:10 diluted
Notice that indeed this is no smear but individual bands. == 7-23-2009
==
7-24-2009
7-27-2009
7-28-2009
7-29-2009
7-30-2009
cell culture:
IDs created
7-31-2009
cell culture:
IDs created
8-01-2009
8-02-2009
8-03-2009
8-04-2009synthetic promoters
BBb submission plasmid
8-05-2009
synthetic promoters
BBb submission plasmid
8-11-2009
8-12-2009
8-13-2009
8-14-2009Promotors
8-15-2009
8-16-2009
8-17-2009
8-18-2009Cloning of cmv core promoter in Jet GFP plasmid (p31)
HindIII and NheI-HF digested PCR product (CMV core promoter from p6), 1 µl ligation buffer (Fermentas), 1 µl T4Ligase, 5 µl water. ligation was done at room temperature for 1 hour.
8-19-2009
8-20-2009
8-21-2009
8-24-2009
8-25-2009
8-26-2009
8-27-2009
Synthesis of HIF, p53, NFkB responsive promoters; constitutively active promoter; empty/random promoter:
--- Protocol optimization
8-28-2009Protocol optimization
Synthesis of HIF, p53, NFkB responsive promoters; constitutively active promoter; empty/random promoter:
8-29-2009Synthesis of HIF, p53, NFkB responsive promoters; constitutively active promoter; empty/random promoter:
8-31-2009Synthesis of HIF, p53, NFkB responsive promoters; constitutively active promoter; empty/random promoter:
9-01-2009Synthesis of HIF, p53, NFkB responsive promoters; constitutively active promoter; empty/random promoter:
Protocol optimization
9-02-2009Synthesis of HIF, p53, NFkB responsive promoters; constitutively active promoter; empty/random promoter: Screening results
This is the way forward
9-03-2009New attempt to synthesize NFkB and p53 responsive promoters:
9-04-2009New attempt to synthesize NFkB and p53 responsive promoters:
Synthesis of HIF, p53 promoters from the first synthesis round:
9-06-2009New attempt to synthesize NFkB and p53 responsive promoters:
9-07-2009New attempt to synthesize NFkB and p53 responsive promoters:
9-08-2009New attempt to synthesize NFkB and p53 responsive promoters:
9-09-2009Synthesizing AHR, SREBP and pPARy
Screening of NfKb, p53 responsive promoters (of second synthesis round)
9-10-09
9-14-09
9-15-09
9-16-09
9-18-09
9-20-09
9-21-09Synthesis was remade for the Promoters stated above. We improved gel extraction quality. Still, quality synthesis remained low. We selected clones from the gel that were subjected to screening subsequently. Later, we found out that probably damaged HinDIII enzyme was responsible for the bad synthesis quality. 9-30-09
October 2009In the weeks before wiki freeze, selected promoters were characterized by the measurement subgroup (see their Notebook ). At the same time, further screenings were conducted as described Also, some promoters were characterized roughly by triple TECAN-reads (namely, pPARγ and p53 responsive clones), or attempted to characterize in this was. We provide all spreadsheets thus generated in a two zip file: raw data and analyzed data. All Spreadsheets are commented with date of measurement. The only of those characterization which yielded reliable results we decided to publish on the registry is for pPARγ (see below or in analyzed data). |