Culture for miniprep of C2 v2 and B1 v2
Digestion of B2, E1 and C2 from the 4th of August
Electrophoresis with the results of digestion
PCR of inserts A1⁄A2⁄D1⁄D2
Gel extraction of A1⁄A2⁄D1⁄D2
Gel extraction of B2, E1 and E2
Resuspension of inserts B2⁄E1⁄E2
Ligation of inserts B2⁄E1⁄E2 with pET 43.1 (a+)
Miniprep of C2 v2 (TOP 10 ) and B1 v2 (TOP 10 )
Miniprep preculture of C1 v2 in pET 43.1 (a+)
Preparation of 10 aliquots of carbenicillin at 50 ng⁄m
Electrophoresis of the PCR done on the 8th of August with A1⁄A2⁄D1⁄D2
Transformation of A1⁄A2⁄D1⁄D2 in TOP 10
Transformation of E1⁄E2 and B2 in TOP 10
Miniprep of C1 v2 (culture from the 9 of August)
Digestion of C1 v2 before electrophoresis
Digestion of pET 43.1 (a+) with XbaI and HindIII
Electrophoresis and gel extraction
Electrophoresis of C1 digested
Transformation of B2 (4, 7 and 9), E1 (1 and 2) and E2 (2, 3, 4, 5, 6 and 7)
Aliquot of antibodies 462
Culture of A1⁄A2⁄D1⁄D2
Ligation of A1⁄A2⁄D1⁄D2 in TOPO
Transformation of A1⁄A2⁄D1⁄D2 with TOPO in TOP 10 competent cells
Transformation of B1 and C2 in BL21DE3
Dosage of digested pET 43.1 (a+)
Transformation of C2 and B1 in pET 43.1 (a+) and DH3α
Absorbance of precultures C2 (1, 2, 3) and B1 (1, 2, 16)
Dephosphorylation of pET 43.1 (a+) digested on the 10th of August
Miniprep of B1⁄E1⁄E2 in TOPO
Transformation of B1 colony 8 and C2 colony 16 in pET 43.1 (a+) and in DH 3α
Precultures of B1 v2 and C2 v2
Digestion of pET 43.1 (a+) with XbaI and HindIII
August 12, 2016:
Miniprep from precultures of B2⁄E1⁄E2 in TOPO
Digestion of inserts B2⁄E1⁄E2 with XbaI and HindIII
Culture of C2 and B1 in 1 l of LB
Agarose gel to analyse digestion of pET 43.1 (a+) done on the 11th of August
Aim: As the transformations did not work (B2, E1 and E2 in pET 43.1 (a+) ) with TOP 10 competent cells, we take the products of the midiprep done on the 4th of August and we digest before redoing the transformation.
Protocol: follow in this link
What we did in the lab:
Materials:
• Restriction enzymes: Xba I, Hind III (New England Biolabs, NEB)
• Restriction enzyme buffers
• 37 &176;C water bath
• Shaking incubator (INFORS HT)
• Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this link)
Method:
1. Realize a Mastermix and store it on ice :
Reactants | Volumes (µl) |
---|---|
<> XbaI |
<> 30 |
<> HindIII |
<> 30 |
<> Buffer 2.1 |
<> 90 |
<> Distilled water |
<> 90 |
<> Total |
<> 150 |
Aim: Increase the quantity of insert.
Protocol: follow in this link
What we did in the lab:
Materials:
• Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this link)
• 1.5 ml eppendorfs
• Takara enzyme
• Primers S and AS
• dNTP
• Buffer 6 X
• Distilled water
• MgCl2
Method:
1. Prepare the following tubes :
Mix with two primers | Mix with primer S only | Mix with primer AS only | |
---|---|---|---|
Takara enzyme (µl) |
6 | 6 | 6 |
Primer S (µl) |
6 | 6 | Ø |
Primer AS (µl) |
6 | Ø | 6 |
MgCl2 (µl) |
15 | 15 | 15 |
dNTP (µl) |
15 | 15 | 15 |
Buffer (µl) |
30 | 30 | 30 |
H2O (µl) |
216 | 222 | 222 |
Total (µl) |
294 | 294 | 294 |
Mix with two primers | Mix with primer S only | Mix with primer AS only | |
---|---|---|---|
A1 |
tube 1 | tube 2 | tube 3 |
A2 |
tube 4 | tube 5 | tube 6 |
D1 |
tube 7 | tube 8 | tube 9 |
D2 |
tube 10 | tube 11 | tube 12 |
Aim: Get back purified DNA.
Protocol: follow in this link
What we did in the lab:
Materials:
• Gel of B2⁄E1⁄E2
• QIAGEN Extraction gel kit
Method:
Follow the Qiagen Extraction gel kit steps with :
DNA | Colonies | Weight of the gel (mg) |
---|---|---|
B2 |
Colony 4 | 367 |
Colony 7 | 432 | |
Colony 9 | 269 | |
E2 |
Colony 1 | 300 |
Colony 2 | 355 | |
Colony 3 | 354 | |
Colony 4 | 314 | |
Colony 5 | 299 | |
Colony 6 | 275 | |
Colony 7 | 277 | |
E1 |
Colony 1 | 404 |
Colony 2 | 321 |
Aim: Storage of the inserts.
Protocol: follow in this link
What we did in the lab:
Materials:
• NaAc
• Ethanol 70 %
• Inserts B2⁄E1⁄E2
Method:
1. Use 1/10 volume of NaAc and 2.5 colume of ethanol for each insert :
B2 | E1 | E2 | |
---|---|---|---|
NaAc (µl) |
15 | 10 | 35 |
Ethanol (µl) |
875 | 250 | 375 |
Aim: Prepare the transformation.
Protocol: follow in this link
What we did in the lab:
Materials:
• Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this link)
• Inserts B 2 /E 1 /E 2
• pET 43.1 (a+)
• TOP 10 X
• Distilled water
• Ligase
Method:
Use the following volumes :
E1 | E2 | B2 | pET 43.1 (a+) | |
---|---|---|---|---|
E1 (µl) |
15 | Ø | Ø | Ø |
E2 (µl) |
Ø | 15 | Ø | Ø |
B2 (µl) |
Ø | Ø | 15 | Ø |
pET 43.1 (µl) |
4 | 4 | 4 | 4 |
Ligase (µl) |
1 | 1 | 1 | 1 |
TOP 10 X (µl) |
2.2 | 2.2 | 2.2 | 2.2 |
H2O (µL) |
> Ø | > Ø | > Ø | > 15 |
> Vtotal (µL) |
> 22.2 | > 22.2 | > 22.2 | > 22.2 |
Aim: Increase the quantity of DNA.
Protocol: follow in this link
What we did in the lab:
Materials:
• Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this link)
• Qiagen Miniprep kit
• Digestion enzyme XbaI and HindIII
• Digestion buffer 2.1
• 1.5 ml eppendorfs
• Electrophoresis cuve
• Distilled water
Method:
1. Use the Qiagen kit for our cultures from the 8th of August :
13 eppendorfs of B1.
20 eppendorfs of C2.
2. Digest the plasmid with the following volumes for each sample :
Volumes (µl) | |
---|---|
DNA |
5 |
XbaI |
1 |
HindIII |
1 |
Buffer 2.1 |
2 |
H2O |
11 |
Total |
20 |
Aim: Split the insert and the plasmid.
Protocol: follow in this link
What we did in the lab:
Materials:
• Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this link)
• Qiagen Miniprep kit
• Digestion enzyme XbaI and HindIII
• Digestion buffer 2 X
• 1.5 ml eppendorfs
• Distilled water
• Shaking incubator (INFORS HT)
Method:
1. Realize a master mix with :
Volumes (µl) | |
---|---|
<> XbaI |
<> 20 |
<> HindIII |
<> 20 |
<> Buffer 2 X |
<> 40 |
<> H2O |
<> 220 |
<> Total |
<> 300 |
Aim: We want to produce 5 μ g of dephosphorylated pET 43.1 (a+) from pET 43.1 (a+) at 400 ng⁄ml and we start with the digestion.
Protocol: follow in this link
What we did in the lab:
Materials:
• Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this link)
• Qiagen Miniprep kit
• Digestion enzyme XbaI and HindIII
• CutSmart buffer
• 1.5 ml eppendorfs
• Distilled water
• Shaking incubator (INFORS HT)
Method:
1. Put all the following reactants in a 1.5 ml eppendorf and let digest one hour at 37 °C :
Volumes (µl) | |
---|---|
DNA |
12.5 |
XbaI |
2 |
HindIII |
4 |
Buffer CutSmart |
5 |
H2O |
26.5 |
Total |
50 |
Aim: To produce proteins.
Protocol: follow in this link
What we did in the lab:
Materials:
• Spectrophotometer Ultrospec 3100
• iPTG at 0.5 M
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Method:
1. Make two measures separated of 30 minutes :
Sample | 1 | 2 | 3 | 4 | 5 | 6 | Time of addition of iPTG | Concentration (ng⁄μl) |
---|---|---|---|---|---|---|---|---|
B1 (1) |
0.022 | 0.062 | 0.152 | 0.344 | 0.557 | 0.694 | 16 h 55 | 0.859 |
B1 (2) |
0.185 | 0.417 | 0.693 | 15 h 25 | 0.956 | |||
B1 (3) |
0.075 | 0.211 | 0.413 | 0.688 | 15 h 55 | 0.920 | ||
C2 (1) |
0.060 | 0.166 | 0.350 | 0.627 | 0.699 | 16 h 25 | 0.905 | |
C2 (2) |
0.044 | 0.119 | 0.296 | 0.510 | 0.698 | 16 h 25 | 0.910 | |
C2 (16) |
0.080 | 0.230 | 0.445 | 0.689 | 15 h 55 | 0.907 |
Aim: Make the future ligation easier.
Protocol: follow in this link
What we did in the lab:
Materials:
• Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this link)
• onSAP
• CutSmart buffer
• 1.5 ml eppendorfs
• Distilled water
• Shaking incubator (INFORS HT)
Method:
Method
1. Start with tube 2 (8.6 ng⁄μl in 46 μl) and use the following mix :
Volumes ( μl) | |
---|---|
DNA |
46 |
CutSmart |
6 |
H2O |
6.7 |
onSAP |
1.3 |
Total |
60 |
Aim: Check if the colonies we took contain the insert.
Protocol: follow in this link
What we did in the lab
What we did in the lab
Materials
• Microbiology equipment (type of incubator, Bunsen burner, water bath, etc… Follow this link)
• Digestion enzyme XbaI and HindIII
• Digestion buffer 2.1
• 1.5 ml eppendorfs
• Distilled water
• Shaking incubator (INFORS HT)
• Inserts B2⁄E1⁄E2
Method
1. In a 1.5 ml eppendorf, put :
Volumes (μl) | |
---|---|
DNA |
5 |
XbaI |
1 |
H2O |
11 |
HindIII |
1 |
Buffer 2.1 |
2 |
Total |
20 |