Team:UNIPV-Pavia/Notebook/Week4Jun

From 2009.igem.org

(Difference between revisions)
(June, 23rd)
(June, 27th)
 
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__NOTOC__  
__NOTOC__  
<div>
<div>
 +
<html><a name="week_start"></a></html>
= Week from June 22nd, to June 28th, 2009 =
= Week from June 22nd, to June 28th, 2009 =
<html>
<html>
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<tr>
<tr>
<td align="left" width="50%">
<td align="left" width="50%">
-
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week3Jun">
+
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week3Jun#week_start">
  <img src="https://2009.igem.org/Special:FilePath?file=Left_arrow.png"/>
  <img src="https://2009.igem.org/Special:FilePath?file=Left_arrow.png"/>
</a>
</a>
-
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week3Jun">Previous Week</a>
+
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week3Jun#week_start">Previous Week</a>
</td>
</td>
<td align="right" width="50%">  
<td align="right" width="50%">  
-
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week1Jul">Next Week</a>
+
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week1Jul#week_start">Next Week</a>
-
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week1Jul">
+
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week1Jul#week_start">
  <img src="https://2009.igem.org/Special:FilePath?file=Right_arrow.png"/>
  <img src="https://2009.igem.org/Special:FilePath?file=Right_arrow.png"/>
</a>
</a>
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**an aTc->GFP measurement system (A6-E0240 = J23100-RBS-tetR-TT-Ptet-RBS-GFP-TT) and
**an aTc->GFP measurement system (A6-E0240 = J23100-RBS-tetR-TT-Ptet-RBS-GFP-TT) and
**a control construct that should always express GFP(A4-E0240 = RBS-tetR-TT-Ptet-RBS-GFP-TT)
**a control construct that should always express GFP(A4-E0240 = RBS-tetR-TT-Ptet-RBS-GFP-TT)
 +
*Moreover, we planned to begin the construction of a lysis actuator with K117000 (=celB) BioBrick and also a test construct with J23118 to assay GFP expression.
 +
*We infected 5 ml of LB + Amp with 10 ul of these glycerol stocks (to prepare samples for this week's ligations):
*We infected 5 ml of LB + Amp with 10 ul of these glycerol stocks (to prepare samples for this week's ligations):
Line 36: Line 39:
|A4
|A4
|A6
|A6
 +
|B0015
|}
|}
*We incubated the 5 ml cultures overnight at 37°C, 220 rpm.
*We incubated the 5 ml cultures overnight at 37°C, 220 rpm.
 +
 +
*We transformed BOL1 plasmid in TOP10 and plated transformed bacteria in a LB + Amp agar plate. We incubated the plate overnight at 37°C.
*Wiki updating.
*Wiki updating.
 +
 +
 +
 +
*We ordered ''pdc'' and ''adhB'' coding sequences from ''Zymomonas mobilis'' to Mr Gene. They had the following specifications:
 +
**the sequences were taken from the online data banks, considering the most recent entries;
 +
**the organism of interest was ''Z. mobilis'' CP4 (ATCC 31821);
 +
**the sequences were codon-optimized for ''E. coli'';
 +
**prefix and suffix sequences were added, considering that both genes start with ATG;
 +
**an additional stop codon (TAA) was addad at the end of the coding sequence, just before the suffix, in order to have a double stop codon;
 +
**restriction sites EcoRI, XbaI, SpeI, PstI and NotI had to be avoided during codon optimization (while the original coding sequences didn't have any of them).
<div align="right">
<div align="right">
Line 48: Line 64:
== <html><font class="dayw_style">June, 23rd</font></html> ==
== <html><font class="dayw_style">June, 23rd</font></html> ==
-
*Miniprep for: E0240 (5 samples), A4, A6, TT, J23118 and K117000
+
*BOL1 plate showed colonies! We picked a colony from BOL1 plate and infected 1 ml of LB + Amp. We incubated the inoculum at 37°C, 220 rpm for 5 and 1/2 hours.
 +
 
 +
*Glycerol stock for the grown culture of BOL1.
 +
 
 +
*We re-filled the remaining 250 ul of BOL1 culture with 5 ml of LB + Amp and incubated the culture overnight at 37°C, 220 rpm. The next day it will be miniprepped and sent to BMR for sequencing!
 +
 
 +
<table cellspacing="20px">
 +
<tr>
 +
<td>
 +
<table>
 +
<tr>
 +
<td>
 +
*Miniprep for: E0240 (5 samples), A4, A6, B0015, J23118 and K117000
*Digestions:
*Digestions:
{|cellpadding="20"
{|cellpadding="20"
Line 57: Line 85:
|A4(S-P)
|A4(S-P)
|A6(S-P)
|A6(S-P)
-
|TT(E-X)
+
|B0015(E-X)
|}
|}
*The bands were cut from the gel and the following ligations were performed:
*The bands were cut from the gel and the following ligations were performed:
Line 64: Line 92:
**A9 = A6(S-P) + E0240(X-P)
**A9 = A6(S-P) + E0240(X-P)
**A10 = K117000(E-S) + TT(E-X)
**A10 = K117000(E-S) + TT(E-X)
-
 
*The ligation reactions were incubated overnight at 16°C.
*The ligation reactions were incubated overnight at 16°C.
 +
</td>
 +
</tr>
 +
</table>
 +
</td>
 +
<td>
 +
[[Image:pv_elisa_letizia_wiki.jpg|thumb|300px|right|Elisa and Letizia working on our wiki.]]
 +
</td>
 +
</tr>
 +
</table>
== <html><font class="dayw_style">June, 24th</font></html> ==
== <html><font class="dayw_style">June, 24th</font></html> ==
-
*We resuspended R0011 (=pLac) and K112808 from the iGEM plates with 15 ul of RNAse free water.
+
*Miniprep for BOL1. We also sent the purified plasmid to BMR Genomics for sequencing.
-
*Trasformations in Top10 bacteria were done for: A7, A8, A9, A10, K112808 and R0011.
+
*We resuspended R0011 (=Plac) and K112808 (=lysis actuator from T4 phage) from the iGEM plates with 15 ul of RNAse free water.
 +
*Trasformations in TOP10 bacteria were done for: A7, A8, A9, A10, K112808 and R0011. We plated the transformed bacteria and incubated the plates overnight at 37°C.
*Team meeting
*Team meeting
 +
*We received sequencing results for:
 +
**K131009 - MIT sequencing was confirmed: celB had a point mutation which changes 1 amino acid L->M, while both prefix and suffix had a nucleotide deletion (anyway, the restriction sites were not corrupted). We will document it on K131009 page, but by now we don't know if it is a good idea to use this BioBrick...
 +
**A3 - correct! (long part, but lacZ had already been successfully tested)
 +
**A4 - correct!
 +
**A5? - correct! (long part, but lacZ had already been successfully tested), we were very lucky: the colony had been chosen randomly from the A5 plate:):) Now "A5?" will be called "A5"!
 +
**A6 - correct!
== <html><font class="dayw_style">June, 25th</font></html> ==
== <html><font class="dayw_style">June, 25th</font></html> ==
 +
 +
*All the overnight plates showed colonies!
 +
 +
*We picked a colony from R0011 and K112808 plates to infect 1 ml of LB + Amp. We incubated the two inocula at 37°C, 220 rpm for 5 and 1/2 hours.
 +
 +
*Glycerol stocks for R0011 and K112808. The remaining 250 ul of R0011 grown culture had been re-filled with 5 ml of LB + Amp to grow an overnight culture (37°C, 220 rpm).
 +
 +
*We also infected 5 ml of LB + Amp with 10 ul of BOL1 glycerol stock to grow an overnight culture (37°C, 220 rpm).
 +
 +
*Colony PCR for:
 +
**A7 - 3 colonies (few colonies because we picked non red coloured colonies)
 +
**A8 - 8 colonies (important ligation!)
 +
**A9 - 12 colonies (important ligation!)
 +
**A10 - 3 colonies (it's quite unuseful to screen this ligation, because probably we are not able to discriminate the positive and the negative transformants)
 +
 +
*The picked colonies used in the PCR were inoculated in 1 ml of LB + Amp and incubated at 37°C, 220 rpm, waiting for the gel results.
 +
 +
*We performed two different PCR programs:
 +
**one for A7 (expected size of positive plasmid: ~1 Kb) and A10 (expected size of positive plasmid: ~600 bp), with 3 min elongation time
 +
** and a different one for A8 and A9 (expected size of positive plasmids: ~2 Kb for both).
 +
 +
*Electrophoresis for the resulting reactions.
 +
 +
 +
<font class='didascalia'>
 +
{|align="center"
 +
|[[Image:pv_colonypcr_A7_A8_A9_A10.jpg|thumb|500px|left|Colony PCR on A7, A8, A9, A10: we chose the 1st screened colony for A7 (A7-1), while we did not choose any colony for the other ligations because they did not look correct.]]
 +
|}
 +
</font>
 +
 +
*Gel results:
 +
**A7 - all colonies were good, we kept A7-1 to store a glycerol stock.
 +
**A8, A9 and A10 unfortunately showed extra bands. So, we didn't keep any colony for them.
 +
**Blank reaction also showed a contaminant band.
 +
 +
*We planned:
 +
**not to care about A10 at the moment because the priority was to test aTc sensing device with A8 and A9;
 +
**to re-examinate the gel results to explain the lengths of the extra bands (on Monday);
 +
**to re-transform the ligations (stored at -20°C) because probably more than one plasmid had been incorporated in the screened colonies...
 +
 +
''Preparation of experiment with Tecan F200''
 +
 +
*We infected 5 ml of LB + Amp with 10 ul of:
 +
**T9002 (the following day it will be diluted and induced with different concentrations of 3OC6-HSL)
 +
**E0240 (negative control)
 +
**A1 (positive control)
 +
*glycerol stocks. We incubated the inocula overnight at 37°C, 220 rpm.
<div align="right">
<div align="right">
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== <html><font class="dayw_style">June, 26th</font></html> ==
== <html><font class="dayw_style">June, 26th</font></html> ==
 +
 +
<font class='didascalia'>
 +
 +
<table cellspacing="30px">
 +
<tr>
 +
<td valign="top">
 +
[[Image:pv_susanna_miniprepBOL1_R0011.jpg|thumb|300px|left|Susanna resuspending pellets during miniprep.]]
 +
</td>
 +
<td>
 +
<table>
 +
<tr>
 +
<td>
 +
*Miniprep for R0011 and BOL1. The purified plasmids were stored at -20°C ready to be cut!
 +
</td>
 +
</tr>
 +
<tr>
 +
<td>
 +
*We diluted 1:20 the A8 and A9 ligations, which were stored at -20°C, and transformed 1 ul of the dilution in TOP10 E. coli. We plated the transformed bacteria on LB + Amp agar plates and incubated the two plates at 37°C overnight.
 +
</td>
 +
</tr>
 +
</table>
 +
</td>
 +
</tr>
 +
</table>
 +
</font>
 +
 +
''Preparation of experiment with Tecan F200''
 +
 +
*We diluted 1:1000 the overnight cultures of:
 +
**T9002 (24 different 5 ml cultures)
 +
**E0240 (one 5 ml culture)
 +
**A1 (one 5 ml culture)
 +
 +
*We induced the 24 cultures of T9002 with eigth different concentrations of 3OC6-HSL (three 5 ml cultures for each concentration): 0 nM, 0.1 nM, 1 nM, 10 nM, 100 nM, 1 uM, 10 uM, 100 uM.
 +
 +
*We incubated the cultures overnight at 37°C, 220 rpm for 3 hours.
 +
<div align="right">
<div align="right">
Line 85: Line 212:
</div>
</div>
 +
== <html><font class="dayw_style">June, 27th</font></html> ==
 +
 +
*The two overnight plates showed colonies. We put the two grown plates at +4°C: next week they will be screened!
 +
 +
''Experiment with Tecan F200''
 +
* <html><a href="http://aimed11.unipv.it/iGEM2009/TestTECANInfiniteF200/T9002 induction test TEST 27-06-09.pdf" target="_blank">Download Protocol</a></html>
 +
 +
<div align="right">
 +
[[#top|Top]]
 +
</div>
<html>
<html>
Line 91: Line 228:
<tr>
<tr>
<td align="left" width="50%">
<td align="left" width="50%">
-
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week3Jun">
+
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week3Jun#week_start">
  <img src="https://2009.igem.org/Special:FilePath?file=Left_arrow.png"/>
  <img src="https://2009.igem.org/Special:FilePath?file=Left_arrow.png"/>
</a>
</a>
-
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week3Jun">Previous Week</a>
+
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week3Jun#week_start">Previous Week</a>
</td>
</td>
<td align="right" width="50%">  
<td align="right" width="50%">  
-
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week1Jul">Next Week</a>
+
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week1Jul#week_start">Next Week</a>
-
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week1Jul">
+
<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week1Jul#week_start">
  <img src="https://2009.igem.org/Special:FilePath?file=Right_arrow.png"/>
  <img src="https://2009.igem.org/Special:FilePath?file=Right_arrow.png"/>
</a>
</a>

Latest revision as of 15:18, 20 October 2009

EthanolPVanimation.gif

December 2008
M T W T F S S
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March 2009
M T W T F S S
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2 3 4 5 6 7 8
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30 31
April 2009
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13 14 15 16 17 18 19
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27 28 29 30
May 2009
M T W T F S S
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11 12 13 14 15 16 17
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25 26 27 28 29 30 31
June 2009
M T W T F S S
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29 30
July 2009
M T W T F S S
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27 28 29 30 31
August 2009
M T W T F S S
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September 2009
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October 2009
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November 2009
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30

Week from June 22nd, to June 28th, 2009

Previous Week Next Week

June, 22nd

  • This week we planned to ligate the GFP protein generator under the control of Ptet in A4 and A6 constructs, in order to have:
    • an aTc->GFP measurement system (A6-E0240 = J23100-RBS-tetR-TT-Ptet-RBS-GFP-TT) and
    • a control construct that should always express GFP(A4-E0240 = RBS-tetR-TT-Ptet-RBS-GFP-TT)
  • Moreover, we planned to begin the construction of a lysis actuator with K117000 (=celB) BioBrick and also a test construct with J23118 to assay GFP expression.


  • We infected 5 ml of LB + Amp with 10 ul of these glycerol stocks (to prepare samples for this week's ligations):
K117000 E0240 (X5) J23118
A4 A6 B0015
  • We incubated the 5 ml cultures overnight at 37°C, 220 rpm.
  • We transformed BOL1 plasmid in TOP10 and plated transformed bacteria in a LB + Amp agar plate. We incubated the plate overnight at 37°C.
  • Wiki updating.


  • We ordered pdc and adhB coding sequences from Zymomonas mobilis to Mr Gene. They had the following specifications:
    • the sequences were taken from the online data banks, considering the most recent entries;
    • the organism of interest was Z. mobilis CP4 (ATCC 31821);
    • the sequences were codon-optimized for E. coli;
    • prefix and suffix sequences were added, considering that both genes start with ATG;
    • an additional stop codon (TAA) was addad at the end of the coding sequence, just before the suffix, in order to have a double stop codon;
    • restriction sites EcoRI, XbaI, SpeI, PstI and NotI had to be avoided during codon optimization (while the original coding sequences didn't have any of them).

Top

June, 23rd

  • BOL1 plate showed colonies! We picked a colony from BOL1 plate and infected 1 ml of LB + Amp. We incubated the inoculum at 37°C, 220 rpm for 5 and 1/2 hours.
  • Glycerol stock for the grown culture of BOL1.
  • We re-filled the remaining 250 ul of BOL1 culture with 5 ml of LB + Amp and incubated the culture overnight at 37°C, 220 rpm. The next day it will be miniprepped and sent to BMR for sequencing!
  • Miniprep for: E0240 (5 samples), A4, A6, B0015, J23118 and K117000
  • Digestions:
E0240(X-P) (5 samples) J23101(E-S) K117000(E-S)
A4(S-P) A6(S-P) B0015(E-X)
  • The bands were cut from the gel and the following ligations were performed:
    • A7 = J23118(S-P) + E0240(X-P)
    • A8 = A4(S-P) + E0240(X-P)
    • A9 = A6(S-P) + E0240(X-P)
    • A10 = K117000(E-S) + TT(E-X)
  • The ligation reactions were incubated overnight at 16°C.
Elisa and Letizia working on our wiki.

June, 24th

  • Miniprep for BOL1. We also sent the purified plasmid to BMR Genomics for sequencing.
  • We resuspended R0011 (=Plac) and K112808 (=lysis actuator from T4 phage) from the iGEM plates with 15 ul of RNAse free water.
  • Trasformations in TOP10 bacteria were done for: A7, A8, A9, A10, K112808 and R0011. We plated the transformed bacteria and incubated the plates overnight at 37°C.
  • Team meeting
  • We received sequencing results for:
    • K131009 - MIT sequencing was confirmed: celB had a point mutation which changes 1 amino acid L->M, while both prefix and suffix had a nucleotide deletion (anyway, the restriction sites were not corrupted). We will document it on K131009 page, but by now we don't know if it is a good idea to use this BioBrick...
    • A3 - correct! (long part, but lacZ had already been successfully tested)
    • A4 - correct!
    • A5? - correct! (long part, but lacZ had already been successfully tested), we were very lucky: the colony had been chosen randomly from the A5 plate:):) Now "A5?" will be called "A5"!
    • A6 - correct!

June, 25th

  • All the overnight plates showed colonies!
  • We picked a colony from R0011 and K112808 plates to infect 1 ml of LB + Amp. We incubated the two inocula at 37°C, 220 rpm for 5 and 1/2 hours.
  • Glycerol stocks for R0011 and K112808. The remaining 250 ul of R0011 grown culture had been re-filled with 5 ml of LB + Amp to grow an overnight culture (37°C, 220 rpm).
  • We also infected 5 ml of LB + Amp with 10 ul of BOL1 glycerol stock to grow an overnight culture (37°C, 220 rpm).
  • Colony PCR for:
    • A7 - 3 colonies (few colonies because we picked non red coloured colonies)
    • A8 - 8 colonies (important ligation!)
    • A9 - 12 colonies (important ligation!)
    • A10 - 3 colonies (it's quite unuseful to screen this ligation, because probably we are not able to discriminate the positive and the negative transformants)
  • The picked colonies used in the PCR were inoculated in 1 ml of LB + Amp and incubated at 37°C, 220 rpm, waiting for the gel results.
  • We performed two different PCR programs:
    • one for A7 (expected size of positive plasmid: ~1 Kb) and A10 (expected size of positive plasmid: ~600 bp), with 3 min elongation time
    • and a different one for A8 and A9 (expected size of positive plasmids: ~2 Kb for both).
  • Electrophoresis for the resulting reactions.


Colony PCR on A7, A8, A9, A10: we chose the 1st screened colony for A7 (A7-1), while we did not choose any colony for the other ligations because they did not look correct.

  • Gel results:
    • A7 - all colonies were good, we kept A7-1 to store a glycerol stock.
    • A8, A9 and A10 unfortunately showed extra bands. So, we didn't keep any colony for them.
    • Blank reaction also showed a contaminant band.
  • We planned:
    • not to care about A10 at the moment because the priority was to test aTc sensing device with A8 and A9;
    • to re-examinate the gel results to explain the lengths of the extra bands (on Monday);
    • to re-transform the ligations (stored at -20°C) because probably more than one plasmid had been incorporated in the screened colonies...

Preparation of experiment with Tecan F200

  • We infected 5 ml of LB + Amp with 10 ul of:
    • T9002 (the following day it will be diluted and induced with different concentrations of 3OC6-HSL)
    • E0240 (negative control)
    • A1 (positive control)
  • glycerol stocks. We incubated the inocula overnight at 37°C, 220 rpm.

Top

June, 26th

Susanna resuspending pellets during miniprep.
  • Miniprep for R0011 and BOL1. The purified plasmids were stored at -20°C ready to be cut!
  • We diluted 1:20 the A8 and A9 ligations, which were stored at -20°C, and transformed 1 ul of the dilution in TOP10 E. coli. We plated the transformed bacteria on LB + Amp agar plates and incubated the two plates at 37°C overnight.

Preparation of experiment with Tecan F200

  • We diluted 1:1000 the overnight cultures of:
    • T9002 (24 different 5 ml cultures)
    • E0240 (one 5 ml culture)
    • A1 (one 5 ml culture)
  • We induced the 24 cultures of T9002 with eigth different concentrations of 3OC6-HSL (three 5 ml cultures for each concentration): 0 nM, 0.1 nM, 1 nM, 10 nM, 100 nM, 1 uM, 10 uM, 100 uM.
  • We incubated the cultures overnight at 37°C, 220 rpm for 3 hours.


Top

June, 27th

  • The two overnight plates showed colonies. We put the two grown plates at +4°C: next week they will be screened!

Experiment with Tecan F200

Top


Previous Week Next Week