Team:Fatih-Medical/Lab/Diary

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WEEK 1 - June 1st-7th

Friday: Today we started with a briefing from Mustafa where the main action points of the day were discussed. We had been planning the project of this year.We determined our parts that will be necessary: -K124014 holin -K559010 halorhodopsin+terminator(X2) -K112806 endolysine/T4 -K112808 endolysine/holin/CMV/antiholin These 4 parts was diluted and tagged. Then we coded these parts: -C1:J23100 cons-promoter -C2:CMV promoter

 -P1:CL promoter 

–H1:Holorodopsin -P2:IPTG -L1:endolsin -L2:holin -l3:eth+antiholin
 We prepared 35 plates and 200 ml LB broth for next experiments. -Transformation (L1,L2,L3) 
 -C1,C2 streak -Coloniese are incubated in liquid culture.(C1)


Saturday - Coloniese are incubated liquid culture.( 1,5 ml AMP ) for : C1(x2),C2,N1,L2,L3. -We made this process 2 times because of high mistake risk for first times


Sunday -Single colony isolation has made for C1-x,C1-y,C2,L1,L2 and L3. -C1-x and C1-y are digested with EcoR1 and Pst1. -We prepared liquid culture for C2,L1,L3 again.Because there was not enough DNA for digestion.

Monday -Single colony isolation has been made for L1,L2 and L3. -Digestion has been made with EcoR1 and Pst1 for L1,L3 and C2. -electrophoresis was performed for C1-x,C2,L1,L2 and L3. -After electrophoresis,results of L1,L3 was true but the others was wrong.


Tuesday -Digestion has been made with Xba1 and Pst1 for L1 and L3. -34 mg/ml chloramphenicol included 49 tubes was prepared. -Chloramphenicol included 17 plates was prepared. -IPTG induceble promoter was coded as P2. -Transformation has been made for H1,L1P2 and L3P2 -We prepared liquid culture for C1,C2,L2


Wednesday -Single colony isolation has been made for C1,C2,L2 - We prepared liquid culture for C2 again.Because there was not enough DNA for digestion. - C1 and L2 are digested. - electrophoresis was performed for C1 and L2. -The result of C1 was true but the result of L2 was wrong so a new digestion will been performed and after that electrophoresis will been performed for new L2 and old L2. -We prepared liquid culture for P2L1,P2L3,C2,H1 and L2.

Thursday -We made isolation for P2L1,P2L3,H1,C2,L2 and then digestion has been made with EcoR1 and Pst1 for all of these parts.After that electrophoresis was performed for these parts. -The results of P2L1 and P2L3 might be true , we are not sure about this so we need some expert assistance and we need to sequence these part for being sure. Unfortunately the result of L2 was wrong again. -We prepared a new liquid culture for L2.


WEEK 2

Friday -In order of isoation, digestion and electrophoresis was performed to L2 and C2.By the way electrophoresis was performed 2 times for being sure but both of results were wrong. -Digestion has been made with Xba1 and Spe1 for H1. -Ligation was performed for P2 and H1 ,C1 and GFP.


WEEK 3

Wednesday - Transformation has been made for C2,L2,P2H1 and C1-GFP (unsuccessful) - We prepared 200 ml LB broth for next experiments.

Thursday - Transformation has been made for C2,L2,P2H1 and C1-GFP. -C2 and L2 (successful)

Friday - We prepared 200 ml LB broth and 15 plates for next experiments - Transformation was made for P2H1 and C1-GFP. - We prepared liqued culture for C2 and L2.

Saturday - Single colony isolation has been made for C2 and L2. -C2 and L2 are digested with EcoR1 and Pst1.


WEEK 4

Monday -electrophoresis was performed for C2 and L2.(Unsuccessful) -We prepared Tfb1 and Tfb2 for compatent cell. -We prepared liquid culture for C2 and L2.

Tuesday - Single colony isolation has been made for C2 and L2.
- electrophoresis was performed for C2 and L2. - C2 and L2 are digested with EcoR1 and Pst1.


WEEK 5

Monday - We added compotent cells to ampicilin included liquid culture and plate. -We added compotent cells to cloramphenicoli included plate. -We incubated cloramphenicol resistance bacteria to ampicilin included plate. -We added compatent cells to plate without antibiotic.

Tuesday -We prepared 15 CHL plates. -We tested compatent cell by RFB transformation. -We prepared liquid culture for preparetion of compatent cell.

Wednesday - Transformation was made for C2,L2 and C1-GFP.

Thursday -Ligation was performed for P2 and GFP. - We prepared liqued culture for L2 and C2. - We tested new compatent cell by RFB transformation. - We prepared kanamycin including plate.

Friday - Single colony isolation was made for C2 and L2. - C2 and L2 are digested with EcoR1 and Pst1. - electrophoresis was performed for C2 and L2.(Unsuccessful) - Ligation was performed for P2H1 with kanamycin. - We prepared kanamycin including plate. - We prepared liqued culture for P2GFP and L2. - Transformation was made for P2H1.


WEEK 6

Saturday -Isolation was made for L2 and P2-GFP.After that digestion was made with EcoR1 and Pst1 for these parts.Finally electrophoresis was performed to these parts.The result of P2-GFP was true but L2 was wrong. -We prepared 5 liquid culture for P2H1. -Digestion was made with EcoR1 and Spe1 for P2-GFP

Sunday --Isolation was made 5 coloni for 69h.But microcantifuge is broked. - We prepared liqued culture for J04450(400) - Transformation was made for J04450(500-700) -Our parts were renamed.


WEEK 7

Tuesday - Transformation was made for J04450(500-700) -Digestion was made J04450(500-700) EcoR1 and Pst-1. -We diluted Lac-1. - Transformation was made for Lac-1. - electrophoresis was performed for J04450(500-700) -Ligation was performed for 705-79h. - Transformation was made for 40h,705 and 79h.

Thursday -We made isolation from liquid culture of 40h for testing contamination.Then we made digestion with EcoR1 and Pst1. After that electrophoresis was performed . -Ligation was made for 40h and 70h.After that transformation was made for these parts. -We prepared 3 liquid cultures for each one of LacI,705 and 79h (totally 9 liquid cultures were prepared )

Friday -Isolation was made for LacI,705 and 79h.Then digestion was made with EcoR1 and Pst1 for 705 and 79h , with EcoR1 and Spe1 for LacI.After that electrophoresis was performed for all of these parts.But results werent good.

Sunday - We prepared liqued cultures for Zt and K. -Isolation was made 0,H and U. -Digestion was made 0,H and U. - Electrophoresis was performed for 0,H and U. -Transformation was made W,P,Z,Alpha,Zt,K. -We prepared compatent cell and AMP plates


WEEK 8

Monday - We prepared liqued cultures for W,P,Z,Alpha,Zt and k. -Transformation was made 40hgx,40h and 70h. -Digestion was made u1,u2 and u3.(unsuccessful) - Electrophoresis was performed for u1,u2 and u3.

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