Difference between revisions of "Team:Paris Saclay/Notebook/July/4"

(Plasmids extraction)
(Plasmids extraction)
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''By Naiane and Laetitia''
 
''By Naiane and Laetitia''
  
Plasmids from the following strains were extracted with the [[Team:Paris_Saclay/Experiments#InvitrogenPlasmidExtraction|"Charge Switch-Pro Plasmid Miniprep"]] kit:
+
The following plasmids were extracted using the [[Team:Paris_Saclay/Experiments#InvitrogenPlasmidExtraction|"Charge Switch-Pro Plasmid Miniprep"]] kit:
 
*DS-NMcas
 
*DS-NMcas
 
*DS-SPcasN-
 
*DS-SPcasN-

Revision as of 14:47, 12 July 2016

Monday 4th July

Lab work

Visualization

Ligation of gBlock 2.2

By Caroline and Lea


The size of the gBlock is 808bp so the ratio was 11.69 (>7). GBlock was gently centrifugated and resuspended with 75µL of TE. The solution was then vortexed and stored at 50°C for 20 min. 1µL of ligase buffer, 1µL of ligase and 1µL of digested plasmids pUC19 were mixed with 7µL of gBlock 2.2. The resulting plasmid will be called pPS16_004.

2 control solutions were made:

  1. 1µL of digested plasmids pUC19 and 9µL of water
  2. 1µL of plasmid, 1µL of ligase and 1µL of water.

Transformation of Gblocks in DH5α

By Caroline and Lea

6 transformations were performed with the ligation products containing plasmids: pPS16_001, pPS16_002, pPS16_003, pPS16_005, pPS16_006 and pPS16_004 created on the morning. 3 other transformations were performed with plasmids pPS16_007, pPS16_008 and pPS16_009 extracted on 30/06/16. The transformation protocol was followed increasing plasmids quantities (5µL instead of 1µL). After transformation, cells were spread on Petri dishes containing LB + Ampicillin (50µg/mL) + X-Gal + IPTG.

Digestion of plasmids

By Mathilde and Alice

The following plasmids were digested again with EcoR1 and HindIII:

  • pPS16_001 (from the 6 clones that were selected on 29/06/16)
  • pPS16_003 (from the 6 clones that were selected on 29/06/16)
  • pPS16_005 (from the 6 clones that were selected on 29/06/16)
  • pPS16_006 (from the 6 clones that were selected on 29/06/16)
Component Volume (µL)
Plasmid 10
Red buffer 10x 2
Water 7
EcoRI enzyme 0.5
HindIII enzyme 0.5

The digestion products were mixed as follow to be migrated on an agarose gel.

Component Volume (µL)
Digested DNA 20
Loading buffer 3.3

The DNA concentration was still insufficient meaning the extraction step was not efficient.

Bringing DNA closer

Plasmids extraction

By Naiane and Laetitia

The following plasmids were extracted using the "Charge Switch-Pro Plasmid Miniprep" kit:

  • DS-NMcas
  • DS-SPcasN-
  • DS-ST1casN-
  • DS-TDcasN-

Then plasmids were digested with AvrII

Component Volume (µL)
Plasmid 10
Tango buffer 10x 2
Water 7
AvrII enzyme 1

The mix was incubated at 37°C for 1 hour. An electrophoresis was done (0.8% of agarose).

Component Volume (µL)
Digested DNA 5
Water 5
Loading buffer 2

Biobrick K13 characterization

Culture of BL

2 colonies from each petri dishes cultured in 500µL of LB, streptomycin(500µg/mL) and chloramphenicol (30µg/mL). Then each solution were split into 3 parts of 150µL. Each aliquot is composed of different concentration of salycilate (main solution at 10mM) :

Concentration of salycilate Volume of main solution
00 M 00 µL
30 µM 1.5 µL
1 µM 50 µL

For each colony from each condition (KB72001, KB72001 + PCLTAA, KB72001 + PLCTAG, KB72001 + PLCTq), 350µL of mix of LB + streptomycin + chloramphenicol were added to a culture of 500µL of LB streptomycin (50µg/mL).


Preparation of salycilate at 10 mM

By Charlène, Naiane and Léa

0.07g of salycilate was diluted in 50mL of water. The pH was adjusted to 7 with NaOH.7