Notebook : August 26

summary

• started the Restriction digestion and ligation to get the BioBrick fnr into plasmid PSB1C3 by using restrictin ensyme EcoRI and PstI.

• Sent an E-mail to M. Nesbeth from UCL for requesting the Biobrick BBa_K239005 which was created by iGEM UCL team in 2009

• Designed oligonucleotides for the gene coding for BphR2 (regulator, sensitive for PCBs), Transcriptional regulator of Pseudomonas oleovorans /pseudoalcaligenes group

lab work

• A.aero/anaerobic regulation system
  
  • 1.BioBrick promotor fnr(repressor and activator) in plasmid PSB1C3

Digestion for promoter fnr(repressor and activator) in PSB1C3

2 enzymes SPE I and PST I

For promoter fnr(repressor) :

For promoter fnr(activator)nirB clone 6:

For promoter fnr(activator)nark clone 6 :

For promoter fnr(activator)nirB clone 7 :

For promoter fnr(activator)narG clone 6 :

For promoter fnr(activator)narG clone 7 :

For promoter fnr(activator)nark Digested SPE I :

For promoter fnr(activator)narB Digested SPE I :

For promoter fnr(activator)narG Digested SPE I :

Incubate at 37°C for 30 mins.

Then we performed a precipitation by ethanol in order to inactivate the enzymes for those 9 digestion.

Protocol : Ethanl precipitation

Degestion product quantification

We used the nano drop to measure the DNA in 260nm and we found its concentration

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A - Aerobic/Anaerobic regulation system / B - PCB sensing system

1 - Gibson assembly.

• RBS_BphR2_part1, BphR2_part2 and plasmid PSB1C3
• FNR_part1, FNR part1 and plasmid PSB1C3
• RBS_FNR part1, FNR_part2 and plasmid PSB1C3

Sample Volume:

These 3 mixture is incubated at 50°C for up to one hour. Transformation and spread in 6 LB plates with Chlorenphenicol . Incubate at 37°C over night.

Ligation

After 3h of digestion, we mixed the digestion products:

• B.PCBs sensor system
  
  • 1.BioBrick BphR2(regulator) in plasmid PSB1C3
    

Using software gene manager to find the oligopeptide for amplification of BphR2.