Team:Paris Liliane Bettencourt/Notebook/2011/09/05/

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The rest of the tube is placed in 500µL of LB, incubated for an hour and then plated.
The rest of the tube is placed in 500µL of LB, incubated for an hour and then plated.
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== Hovannes-Baptiste ==
== Hovannes-Baptiste ==
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=== Preparation of slides ===
=== Preparation of slides ===
-
Dillution of an overnight of YC164 and YC227 (SinOp Design).
+
Dilution of overnight cultures : YC164 and YC227 (SinOp Design) . <br>
-
Two well slides > 1-control   2-Mix  
+
 
 +
YC227 produces SinI which enhances biofilm formation. If SinI diffuses through the nanotubes we expect to see fluorescence from Peps-gfp construct in the receiver cells. <br>
 +
 
 +
Two well slides : 1-control (YC164 with IPTG)  2-Mix (both strains with IPTG)
 +
<br>
=== Observation  ===
=== Observation  ===
-37°C Microscopy-<br>
-37°C Microscopy-<br>
-
YC164 grows fast<br>
+
We observed the plate with TRANS and YFP-filter settings on the Old Zeiss. Unfortunately, this microscope gets quickly out of focus so we need to take each picture manually. As expected, YC227 was producing GFP at the begining of the experiment, while YC164 was not. Our observations over 4 hours are the following:
-
YC227 does not grow at all<br>
+
* YC164 grows fast (several divisions over the experiments)
-
YC164 does not change its state<br>
+
* YC227 does not grow at all and keeps its fluorescence pretty well
-
We can see some GFP after an overnight<br>
+
* YC164 does not change its state (no obvious biofilm formation)
 +
* After letting the plate overnight we still see some florescence but not as if YC164 changed its fluorescence status.
 +
 
 +
[[File:0905_SinOp_trans1.jpg|500px|thumb|center|TRANS at t=0min]]
 +
[[File:0905_SinOp_GFP1.jpg|500px|thumb|center|GFP at t=0min]]
 +
[[File:0905_SinOp_trans14.jpg|500px|thumb|center|TRANS at t=90min]]
 +
[[File:0905_SinOp_GFP14.jpg|500px|thumb|center|GFP at t=90min]]
 +
 
 +
=== Our conclusions ===
 +
We might have poorly chosen the exact phase growth or our timing when plating the strains. Nanotube formation seems to require a more tightly packed colony. We will try this tomorrow. Biofilm formation is usually observed at lower temperatures and it could mean we will never see anything with this design (be reminded that we did not do any cloning for this construction, we only add to reuse strains from another scientific team).
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Latest revision as of 21:32, 21 September 2011

Team IGEM Paris 2011

Contents

Cyrille

Miniprep

Miniprep of 2 clones of TetO array in pSB1C3, 2 clones of TetO array in pHM3 Miniprep of Mathias: S21 S82 1 2 3 4; S75 S67 and S75

With good yeilds (>500ng)

Gel Extraction

Gel extraction of pHM3 Digested in EP and pVeg YFP TetR D EP and DXP.

Ligation

Ligation of pHM3 Digested EP with pVeg-YFP-TetR D. EP with ratio 1:1 1:10 1:100 Ligation pHM3 TetO D. SP with pVeg-YFP-TetR D. SP

Transformation

Transformation of the ligation product + ComS ligated in pSB1C3 + YFP TetR BB ligated in pSB1C3

Contol of the comptent cells

Two tests of transformation was done with the B7 plasmid in TurboCell competent cells.

The rest of the tube is placed in 500µL of LB, incubated for an hour and then plated.

Hovannes-Baptiste

Preparation of slides

Dilution of overnight cultures : YC164 and YC227 (SinOp Design) .

YC227 produces SinI which enhances biofilm formation. If SinI diffuses through the nanotubes we expect to see fluorescence from Peps-gfp construct in the receiver cells.

Two well slides : 1-control (YC164 with IPTG) 2-Mix (both strains with IPTG)

Observation

-37°C Microscopy-

We observed the plate with TRANS and YFP-filter settings on the Old Zeiss. Unfortunately, this microscope gets quickly out of focus so we need to take each picture manually. As expected, YC227 was producing GFP at the begining of the experiment, while YC164 was not. Our observations over 4 hours are the following:

  • YC164 grows fast (several divisions over the experiments)
  • YC227 does not grow at all and keeps its fluorescence pretty well
  • YC164 does not change its state (no obvious biofilm formation)
  • After letting the plate overnight we still see some florescence but not as if YC164 changed its fluorescence status.
TRANS at t=0min
GFP at t=0min
TRANS at t=90min
GFP at t=90min

Our conclusions

We might have poorly chosen the exact phase growth or our timing when plating the strains. Nanotube formation seems to require a more tightly packed colony. We will try this tomorrow. Biofilm formation is usually observed at lower temperatures and it could mean we will never see anything with this design (be reminded that we did not do any cloning for this construction, we only add to reuse strains from another scientific team).