Difference between revisions of "Team:Paris Saclay/Notebook/June/29"

(BL21 electro-competent cells transformation)
Line 46: Line 46:
 
====Plasmids digestion====
 
====Plasmids digestion====
 
''By Naiane''
 
''By Naiane''
Plasmids received from Addgene were digested with AvrII using the following quantities: 5 µL DNA, 2µL buffer (Tango), 1 µL enzyme (AvrII), 12µL water. The mix was incubated for 1h at 37°C and 10 min at 55°C and kept at -20°C until the gel electrophoresis was done. Fragments are expected to be as follow:
+
Plasmids received from Addgene were digested with AvrII.
 +
 
 +
{| class="wikitable"
 +
|-
 +
! Component
 +
! Volume (µL)
 +
|-
 +
| Plasmid
 +
| 5
 +
|-
 +
| Tango buffer
 +
| 2
 +
|-
 +
| Water
 +
| 12
 +
|-
 +
| AvrII enzyme
 +
| 1
 +
|}
 +
 
 +
The mix was incubated for 1h at 37°C and 10 min at 55°C and kept at -20°C until the gel electrophoresis was done. Fragments are expected to be as follow:
 
{| class="wikitable"
 
{| class="wikitable"
 
|-
 
|-

Revision as of 15:02, 6 July 2016

Wednesday 29th June

Lab work

Visualization

Culture of clones with gBlocks

By Lea and Marion

6 clones of each construction were selected and grown overnight in 3.5mL of LB (50µg/ml Amp) at 37°C, 180rpm.


BioBrick characterization

BL21 electro-competent cells preparation

By Charlene

200µL of BL21 pre-culture was added to 15mL of LB and incubated for 4h at 37°C. When abs600nm=0.68, cells were centrifuged for 10 minutes at 4000rpm and washed twice with addition of 10mL glycerol (10%) followed by 10 minutes of centrifugation at 4000rpm. Cells were mixed with 200µL glycerol and kept -80°C.

BL21 electro-competent cells transformation

By Charlene

We realized four transformations with the following plasmids:

  • K1372001
  • K1372001+pcl_TAA
  • K1372001+pcl_TAG
  • K1372001+pcl_Tq

50µL of cells were added in the cuvettes with 1µL DNA (diluted 1/10). Everything was done at 4°C.

Transformation did not work for K1372001 and K1372001+pcl_TAA because the cuvettes were broken. Template:Font color. Cells died during transformation. Transformation worked for K1372001+pcl_TAG and K1372001+pcl_Tq. Template:Font color. We added 1mL of LB to the cells and incubated them for 1h at 37°C.

The following cells were plated on Petri dishes (30µg/mL Cm + 50µg/mL streptomycin):

  • BL21|K1372001+pcl_TAG : 50µL of transformed cells
  • BL21|K1372001+pcl_TAG : 500µL of transformed cells concentrated 5x.
  • BL21|K1372001+pcl_Tq : 50µL cells
  • BL21|K1372001+pcl_Tq : 500µL of transformed cells concentrated 5x.

K1372001 plasmid digestion

By Naiane

K1372001 plasmid was digested with BglI using the following quantities: 3 µL DNA, 2µL buffer (O), 1 µL enzyme (BglI), 14µL water. The mix was incubated for 1h at 37°C and 10 min at 55°C and kept at -20°C until the gel electrophoresis was done. Fragments are expected to size 1.2kb and 2.4kb.

BL21 cell culture

We added 200µL of the BL21 culture made on 28/06 in 15ml of LB and incubated it overnight at 37°C, 180rpm.

Bringing DNA closer

Plasmids digestion

By Naiane Plasmids received from Addgene were digested with AvrII.

Component Volume (µL)
Plasmid 5
Tango buffer 2
Water 12
AvrII enzyme 1

The mix was incubated for 1h at 37°C and 10 min at 55°C and kept at -20°C until the gel electrophoresis was done. Fragments are expected to be as follow:

Plasmid name Plasmid size (kb) Digestion product size (kb)
DS-NMcas 6 2.2 and 3.7
DS-SPcasN- 6.8 2.2 and 4.5
DS-ST1casN- 6 2.2 and 3.8
DS-TDcasN- 6.9 2.2 and 4.6