Week 12
08/17 - 08/21
NB-Esterase Assay:
MiniPrep 808030 in the plasmid pDG011.
pNP-Assay
- Culture of DH5-alpha transformed with 808030 in pDG011
- Enzymatic essay (pNP assay) of the first transformation (of the 11/08/15): BBa_808030 and pDG011 plasmid in DH5α
Gibson Assembly:
OD measurement of Cluster 4:
|
Concentration (ng/µL) |
OD(230nm) |
OD(260nm) |
OD(280nm) |
OD(260nm)/OD(230nm) |
OD(260nm)/OD(280nm) |
Cluster_4_start |
30 |
0,025 |
0,575 |
0,375 |
1,50 |
- |
/936011 |
55 |
0,4 |
1,075 |
0,575 |
1,88 |
2,65 |
936011/936023 |
7,5 |
0,6 |
0,125 |
0,05 |
2,41 |
0,21 |
936023/ |
45 |
0,575 |
0,925 |
0,625 |
1,48 |
1,61 |
Cluster_4_end |
47,5 |
0 |
0,925 |
0,575 |
1,64 |
- |
- Gel migration of the PCR product of prom/pNB Est and Cluster_1_start.
Gel plan:
Stain |
1 |
2 |
3 |
4 |
5 |
6 |
7 |
8 |
9 |
10 |
11 |
Tube number |
|
|
A1 |
A2 |
A3 |
A4 |
|
B1 |
B2 |
B3 |
B4 |
Componants |
Ladder |
|
|
|
|
|
|
|
|
|
|
DNA concentration assay :
|
Concentration (ng/µL) |
OD(230nm) |
OD(260nm) |
OD(280nm) |
OD(260nm)/OD(280nm) |
OD(260nm)/OD(230nm) |
Cluster 4 start |
105 |
0,3 |
2,1 |
1,1 |
1,79 |
2,40 |
/936011 |
55 |
0 |
1,1 |
0,55 |
1,99 |
- |
936011/936023 |
520 |
4,325 |
10,425 |
5,825 |
1,79 |
4,38 |
936023/ |
47,5 |
0 |
0,925 |
0,5 |
1,89 |
- |
Cluster 4 end |
130 |
0,6 |
2,625 |
1,475 |
1,79 |
4,38 |
Gibson Assembly:
- Enzymatic digest of K936011, K936023 and K1392932
- Enzymatic digest using Pst I and Spe I
- Gel Migration of digested plasmids K936011, K936023, K1392932. on a 0,8% Agarose Gel
- Gel Purification
Cluster 4A Gibson assembly:
- Gibson Assembly
- PCR amplification of cluster 4A Assembly.
- Gel migration on 0,8% Agarose Gel.
Gel Plan:
Well Number |
1 |
2 |
3 |
4 |
5 |
Contains |
DNA ladder |
No primers |
Primer for only |
Primer rev only |
Both primers |
PCR amplification of Biobricks K808007, K808030, K936011, K936023, K1392932, K316003
- PCR amplification using Phusion polymerase
- Gel Migration on a 1% Agarose Gel
The PCR worked for most of our Biobricks with the exception of the biobrick K808030.
DNA concentration measurement
1/25 dilution |
DNA concentration (ng/µL) |
OD(230nm) |
OD(260nm) |
OD(280nm) |
OD(340nm) |
OD(260nm)/OD(280nm) |
OD(260nm)/OD(230nm) |
808007 |
4,3 |
0,08 |
0,085 |
0,052 |
0,006 |
1,64 |
1,06 |
808030 |
4,6 |
0,151 |
0,092 |
0,058 |
0,003 |
1,59 |
1,61 |
936011 |
5,9 |
0,141 |
0,118 |
0,073 |
0,009 |
1,61 |
0,83 |
936023 |
5,2 |
0,097 |
0,105 |
0,062 |
0,003 |
1,7 |
1,08 |
1392932 |
12,6 |
0,493 |
0,251 |
0,259 |
0,035 |
0,97 |
0,51 |
316003 |
5,5 |
0,1 |
0,11 |
0,062 |
0,0 |
1,76 |
1,10 |
PCR amplification of pSB1C3
- PCR amplification using Phusion Polymerase.
- Gel Migration on a 1% agarose gel
Well Number |
1 |
2 |
3 |
4 |
5 |
6 |
7 |
Contains |
DNA ladder |
Non digested Plasmid |
Digested plasmid |
No primers |
Primer for only |
Primer rev only |
Both primers |
PCR amplification of pSB1C3
- PCR amplification using Takara Ex Taq Polymerase testing different annealing temperatures.
|
No primers |
Primer for |
Primer rev |
|
DNAse, RNAse free water |
41,75 |
40,75 |
40,75 |
39,75 |
10X Ex Taq Buffer |
5 |
5 |
5 |
5 |
dNTP |
2 |
2 |
2 |
2 |
rescue_for |
0 |
1 |
0 |
1 |
rescue_rev |
0 |
0 |
1 |
1 |
DNA Template |
1 |
1 |
1 |
1 |
Ex Taq Polymerase |
0,25 |
0,25 |
0,25 |
0,25 |
Total |
50 |
50 |
50 |
50 |
Cycles:
- 95°C for 4min
- 25 cycles :
- 95°C for 40s
- annealing for 30s:
- 60°C: Tube 1-4
- 61,1°C: Tube 5-8
- 63°C: Tube 9-12
- 65,6°C: Tube 13-16
- 69,2°C: Tube 17-20
- 72,1°C: Tube 21-24
- 73,9°C: Tube 25-28
- 75°C: Tube 28-32
- 72°C for 80s
- 72°C for 7min.
PCR amplification using Takara Ex Taq
- Gel Migration on a 1% Agarose Gel.
PCR amplification of Biobricks K808030
- PCR Amplification using Takara Ex Taq Polymerase.
- Gel migration on 1%
Gel Plan:
Well Number |
1 |
2 |
3 |
4 |
5 |
|
DNA ladder |
No primers |
Primer For |
Primer Rev |
Extract |
PCR amplification of pSB1C3
- PCR amplification using Takara Ex Taq Polymerase testing different annealing temperatures.
- Gel Migration on a 1% Agarose Gel.
PCR amplification of pSB1C3
- PCR amplification using Takara Ex Taq Polymerase testing 8 annealing temperatures.
|
No primers |
Primer for |
Primer rev |
|
DNAse, RNAse free water |
41,75 |
40,75 |
40,75 |
39,75 |
10X Ex Taq Buffer |
5 |
5 |
5 |
5 |
dNTP |
2 |
2 |
2 |
2 |
rescue_for |
0 |
1 |
0 |
1 |
rescue_rev |
0 |
0 |
1 |
1 |
DNA Template |
1 |
1 |
1 |
1 |
Ex Taq Polymerase |
0,25 |
0,25 |
0,25 |
0,25 |
Total |
50 |
50 |
50 |
50 |
Gel Migration on a 1% Agarose Gel
Enzymatic digest of BBa_K808030
- Enzymatic digest by XbaI and Spe I of BBa_K808030
- Gel migration.
Yeast Assembly
The bacteria did not grow because the wrong antibiotic was chosen: BBa_J61047 was in pSB1A2 and not pSB1C3.
- Bacterial culture of BBa_J61047 on liquid LB + Amp 1X at 180 rpm, 37°C. The bacteria grew well.
- Midi-prep has been done with the 50mL of BBa_J61047 culture. (dilution 1/1000)
|
DNA Concentration (ng/µl) |
OD(260nm) |
OD(280nm) |
OD(260nm)/OD(280nm) |
BBa_J61047 |
0,5 |
0,011 |
0,004 |
2,57 |
- Preparation of YPD specific media on specific media (1% yeast extract, 2% Dextrose, 2% Peptone, 2% agar).
- Gel Migration of BBa_J61047.
- NotI enzymatic digest of BBa_J61047 in pSB1A2 enzyme.
- Gel Migration on a 0,8% Agarose Gel and the digestion hasn’t work.
- XbaI and SpeI digestion of BBa_J61047.
- tube 1 « Miniprep XbaI/SpeI » : 5uL 10X buffer cutsmart + 0,5uL XbaI + 0,5uL SpeI + 38uL H2O +5uL ADN, digestion at 37°C during 1 hour.
- tube 2 « Midiprep XbaI/SpeI » : 5uL 10X buffer cut smart + 0,5uL XbaI + 0,5uL SpeI + 38uL H2O + 5uL ADN, digestion at 37°C during 1 hour
- tube 3 « Miniprep NotI » : 5uL 10X buffer cutsmart + 0,5 NotI + 38,5 H2O + 5uL ADN, digestion at 37°C during 1 hour
- tube 4 « MiDiprep NotI » : 5uL 10X buffer cutsmart + 0,5 NotI + 38,5 H2O + 5uL ADN, digestion at 37°C during 1 hour
- tube 5 « Miniprep CTRL » as negative control : 5Ul ADN + 40uL H2O + 5uL 10X buffer cutsmart.
- tube 6 « Midiprep CTRL » as negative control : 5Ul ADN + 40uL H2O + 5uL 10X buffer cutsmart.
- MWT : « Quick-Load Purple 2-Log DNA Ladder (0.1-10.0 kb) NEB
PCR Amplification of the BBa_J61047 using Phusion Polymerase Master Mix.
- Gel Migration on a 0.8% agarose gel
- Culture of the plasmid pRS415 in SC_Leu at 30°C at 150rpm for about 72h.
- PCR Amplification using the Phusion Polymerase of pRS415.
- Gel Extraction of the PCR products.
TPA solubility :
- Determination of the solubilization products of TPA.
- Detection of 2-hydroxy-terephthalate using a TECAN spectrometer.
- Precipitaion of terephthalic acid in H2SO4.
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