From 2009.igem.org

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Latest revision as of 09:05, 20 October 2009

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Week from July 13rd, to July 19th, 2009

Previous Week

Next Week

July, 13th

This week we planned to assemble GFP protein generator under the control of Plac in our IPTG/lactose sensor (i.e. A11) in order to test it. We also planned to build up another aTc sensor in which tetR is expressed constitutively, but in smaller amount than in A9 BioBrick. Finally, we planned to put lacZ protein generator under the control of the lactose sensor in order to build up one of the final parts for our project: this part will express beta-galactosidase when lactose is present in the medium and this expression will be glucose-independent (see R0011 page in the Registry for more info).

We infected 5 ml of LB + Amp with 8 ul of the following glycerol stocks:

F2620	A11-1 (X2)	A3-1
A4 (X2)	E0240 (X2)	J23118

We incubated the inocula at 37°C, 220 rpm overnight.

Top

July, 14th

Miniprep for:

F2620 (for seq)	A11-1 (X2)	A3-1
A4 (X2)	E0240 (X2)	J23118

Digestion for:

A11-1(E-S)	A11-1(S-P)	A3-1(E-X)
A4(X-P)(X2)	E0240(X-P)(X2)	J23118(S-P)

Gel run/cut/purification: DNA yield was good for all the extracted parts, except A11-1(E-S), which was quantified as 3 ng/ul after Nanodrop measurement. Anyway, we decided to try to ligate it.

Ligations:
- A12 = J23118(S-P) + A4(X-P) in ~pSB1A2
- A13 = A11(E-S) + A3(E-X) in pSB1AK3
- A14 = A11(S-P) + E0240(X-P) in pSB1A2

We incubated the ligations at 16°C overnight.

Top

July, 15th

We received pdc and adhB genes from Mr Gene! we will call them MRGENE1 and MRGENE2.
- MRGENE1: 5 ug of liophylized DNA, Kan resistance plasmid;
- MRGENE2: 5 ug of liophylized DNA, Amp resistance plasmid.

We transformed the overnight ligations in TOP10 and plated the transformed bacteria. We incubated the plates at 37°C overnight.

Top

July, 16th

Plates results:
- A12 showed colonies! and they were not red (as we expected, because RFP protein generator had been excided from BBa_J61002 plasmid);
- A13 showed no colonies:( We will repeat this ligation one of the next days...
- A14 showed colonies! some of them seemed to be green under the sun light; this was probably caused to GFP accumulation due to the leaky activity of Plac promoter.

Colony PCR for A12. We didn't perform colony PCR screening for A14 because the insert was almost 1.5 Kb long and it contains two copies of B0015 BioBrick, which may corrupt PCR results. (Even A12 had B0015, but it was located at the end of the BioBrick!). During colony PCR, the colonies used for the reaction were inoculated in 1 ml of LB + Amp and incubated at 37°C, 220 rpm waiting for the end of the reaction.

Colony PCR: all the screened colonies contained the correctly ligated plasmid.

Gel results: all the picked colonies had the insert with the expected length! we decided to keep and prepare a glycerol stock for:
- A12-2 (in case of failure)
- A12-3 (to use)

We re-filled (with 5 ml of LB + Amp) A12-2 and A12-3 cultures, using the remaining 250 ul. We incubated the cultures at 37°C, 220 rpm overnight.

We picked 7 random colonies from A14 plate and infected 1 ml of LB + Amp. We incubated the inocula for 5 and 1/2 hours and then we prepared a glycerol stock for all of them.

We re-filled the remaining 250 ul of bacterial culture with 5 ml of LB + Amp and incubated the new cultures at 37°C, 220 rpm overnight. Tomorrow they will be miniprepped and screened!

We resuspended all the 5 ug of MRGENE1 and MRGENE2 with 20 ul of ddH2O.

We transformed 1 ul of the resuspended DNA in TOP10. For each of the 2 plasmids, we plated 150 ul of transformed bacteria + SOC on an Amp plate and also on a Kan plate. In this way we could check if the plasmid had the expected antibiotic resistance.

We incubated the 4 plates at 37°C overnight. We stored the resuspended DNA at -20°C.

Top

July, 17th

Plates results:
- MRGENE1 Amp plate - no colonies
- MRGENE1 Kan plate - bacterial carpet!
- MRGENE2 Amp plate - bacterial carpet!
- MRGENE2 Kan plate - no colonies
The results were consistent with our expectations about the antibiotic resistances!

We picked a single colony from MRGENE1 and MRGENE2 plates and infected 3 ml of LB + suitable antibiotic. We incubated these inocula for about 6 hours. Then, we prepared three glycerol stocks for each of the two cultures in order to have good long term stocks.

We aliquoted the remaining 750 ul (=3 ml-750x3) in three falcon tubes containing 250 ul of bacterial culture and then we re-filled the falcon tubes with 5 ml of LB + suitable antibiotic to grow 6 overnight cultures.

We also infected 5 ml of LB + Amp with 8 ul of B0030 glycerol stock to grow 3 identical 5 ml overnight cultures.

All the 9 cultures were incubated at 37°C, 220 rpm overnight.

Miniprep for the 7 cultures coming from the colonies of A14 plate.

Digestion E-P of 1 ug of DNA for all the 7 miniprepped plasmids (20 ul reaction volume).

Electrophoresis for the digestions.

Digestion screening: colonies 2 and 5 were negative, while the other colonies showed the correctly ligated plasmid, but with a smaller amount of unwanted plasmid.

Gel results:
- A14-1 - positive insert(~2250 bp) + unwanted insert(~1400 bp) + unexpected band(~1100 bp)
- A14-2 - unwanted insert(~1400 bp)
- A14-3 - positive insert(~2250 bp) + unwanted insert(~1400 bp) + unexpected band(~1100 bp)
- A14-4 - positive insert(~2250 bp) + unwanted insert(~1400 bp) + unexpected band(~1100 bp)
- A14-5 - unwanted insert(~1400 bp)
- A14-6 - positive insert(~2250 bp) + unwanted insert(~1400 bp)
- A14-7 - positive insert(~2250 bp) + unwanted insert(~1400 bp) + unexpected band(~1100 bp)

We decided to keep A14-4 glycerol stock in order to perform: i)inoculum, ii)miniprep, iii)dilution, iv) 5 pg transformation, v)plating, vi)digestion screening, as we performed for A8 and A9.

Miniprep for A12-2 and A12-3: DNA yield was quite low...next week they will be inoculated and miniprepped again in order to prepare the samples for sequencing.

Top

July, 18th

Miniprep for:

MRGENE1	MRGENE1-2	MRGENE1-3
MRGENE2	MRGENE2-2	MRGENE2-3
B0030(X3)

We stored the miniprepped DNA at -20°C. Next week we will be ready to assemble these bricks;)

Top

Previous Week

Next Week

@@ Line 3: / Line 3: @@
 <div>
-= Week from July 6th, to July 12nd, 2009 =
+<html><a name="week_start"></a></html>
+= Week from July 13rd, to July 19th, 2009 =
 <html>
 <table width="100%">
 <tr>
 <td align="left" width="50%">
-<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week1Jul">
+<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week2Jul#week_start">
   <img src="https://2009.igem.org/Special:FilePath?file=Left_arrow.png"/>
 </a>
-<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week1Jul">Previous Week</a>
+<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week2Jul#week_start">Previous Week</a>
 </td>
 <td align="right" width="50%">
-<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week3Jul">Next Week</a>
+<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week4Jul#week_start">Next Week</a>
-<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week3Jul">
+<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week4Jul#week_start">
   <img src="https://2009.igem.org/Special:FilePath?file=Right_arrow.png"/>
 </a>
@@ Line 23: / Line 24: @@
 </html>
-== <html><font class="dayw_style">July, 6th</font></html> ==
+== <html><font class="dayw_style">July, 13th</font></html> ==
-*We planned to dedicate this week to the assembly of an IPTG/lactose->PoPS device in order to have a lactose sensor for our project, but also a useful inducible system for general purpose applications.
+*This week we planned to assemble GFP protein generator under the control of Plac in our IPTG/lactose sensor (i.e. A11) in order to test it. We also planned to build up another aTc sensor in which tetR is expressed constitutively, but in smaller amount than in A9 BioBrick. Finally, we planned to put lacZ protein generator under the control of the lactose sensor in order to build up one of the final parts for our project: this part will express beta-galactosidase when lactose is present in the medium and this expression will be glucose-independent (see R0011 page in the Registry for more info).
-*We already had R0011 and BOL1 purified plasmids stored at -20°C. Digestion for:
+*We infected 5 ml of LB + Amp with 8 ul of the following glycerol stocks:
 {|cellpadding="20"
-|R0011(E-X)
+|F2620
-|BOL1(E-S)
+|A11-1 (X2)
+|A3-1
+|-
+|A4 (X2)
+|E0240 (X2)
+|J23118
 |}
-*Gel run/cut and band purification.
+*We incubated the inocula at 37°C, 220 rpm overnight.
-*The purified DNA gave a good result at Nanodrop, but we decided to perform the entire work on BOL1 again because we were not sure that we had extracted a pure band.
+<div align="right">
+[[#top|Top]]
+</div>
-*We stored R0011(E-X) DNA at -20°C.
+== <html><font class="dayw_style">July, 14th</font></html> ==
-*We infected 5 ml of LB + Amp with 8 ul of BOL1 glycerol stock to grow two identical overnight cultures (37°C, 220 rpm).
+*Miniprep for:
+{|cellpadding="20"
+|F2620 (for seq)
+|A11-1 (X2)
+|A3-1
+|-
+|A4 (X2)
+|E0240 (X2)
+|J23118
+|}
+*Digestion for:
+{|cellpadding="20"
+|A11-1(E-S)
+|A11-1(S-P)
+|A3-1(E-X)
+|-
+|A4(X-P)(X2)
+|E0240(X-P)(X2)
+|J23118(S-P)
+|}
+*Gel run/cut/purification: DNA yield was good for all the extracted parts, except A11-1(E-S), which was quantified as 3 ng/ul after Nanodrop measurement. Anyway, we decided to try to ligate it.
+*Ligations:
+**A12 = J23118(S-P) + A4(X-P) in ~pSB1A2
+**A13 = A11(E-S) + A3(E-X) in pSB1AK3
+**A14 = A11(S-P) + E0240(X-P) in pSB1A2
-''Preparation of experiment with Tecan F200''
+*We incubated the ligations at 16°C overnight.
-*We picked a colony of B0030 plate (stored at +4°C) and infected 5 ml of LB + Amp.
-*We also infected 5 ml of LB + Amp with 10 ul of A1 and J23100 glycerol stocks.
-*We incubated the inocula overnight at 37°C, 220 rpm.
 <div align="right">
@@ Line 57: / Line 83: @@
 </div>
-== <html><font class="dayw_style">July, 7th</font></html> ==
+== <html><font class="dayw_style">July, 15th</font></html> ==
-*Miniprep for BOL1 (X2).
+*We received ''pdc'' and ''adhB'' genes from Mr Gene! we will call them MRGENE1 and MRGENE2.
+**MRGENE1: 5 ug of liophylized DNA, Kan resistance plasmid;
+**MRGENE2: 5 ug of liophylized DNA, Amp resistance plasmid.
-*Digestion for BOL1(E-S)(X2).
-*Gel run/cut/purification: none of the two BOL1 samples gave a good results in DNA quantification...we decided to cut the miniprepped plasmids again, but this time through an overnight digestion (both plasmids E-S).
+*We transformed the overnight ligations in TOP10 and plated the transformed bacteria. We incubated the plates at 37°C overnight.
-*In case of failure, we also infected 5 ml of LB + Amp with 8 ul of BOL1 glycerol stock to grow an overnight culture at 37°C, 220 rpm.
+<div align="right">
+[[#top|Top]]
+</div>
-*We prepared 0.5 l of LB + Amp.
+== <html><font class="dayw_style">July, 16th</font></html> ==
-*We received sequencing results for:
+*Plates results:
-**T9002 - long part, but SEQUENCE CONFIRMED! while MIT results were "INCONSISTENT".
+**A12 showed colonies! and they were not red (as we expected, because RFP protein generator had been excided from BBa_J61002 plasmid);
-**A10 - results showed a good chromatogram, but K117000 had not been correctly ligated. We will repeat this ligation one of the next weeks.
+**A13 showed no colonies:( We will repeat this ligation one of the next days...
+**A14 showed colonies! some of them seemed to be green under the sun light; this was probably caused to GFP accumulation due to the leaky activity of Plac promoter.
+*Colony PCR for A12. We didn't perform colony PCR screening for A14 because the insert was almost 1.5 Kb long and it contains two copies of B0015 BioBrick, which may corrupt PCR results. (Even A12 had B0015, but it was located at the end of the BioBrick!). During colony PCR, the colonies used for the reaction were inoculated in 1 ml of LB + Amp and incubated at 37°C, 220 rpm waiting for the end of the reaction.
-''Preparation of experiment with Tecan F200''
+<table align="center">
+<tr>
+<td>
+<font class='didascalia'>
+[[Image:pv_colonypcr_A12.jpg|thumb|500px|left|Colony PCR: all the screened colonies contained the correctly ligated plasmid.]]
+</font>
+</td>
+</tr>
+</table>
-*We diluted 1:100 the overnight cultures of A1, B0030 and J23100.
+*Gel results: all the picked colonies had the insert with the expected length! we decided to keep and prepare a glycerol stock for:
+**A12-2 (in case of failure)
+**A12-3 (to use)
-*We incubated the diluted cultures for 5 hours (37°C, 220 rpm).
+*We re-filled (with 5 ml of LB + Amp) A12-2 and A12-3 cultures, using the remaining 250 ul. We incubated the cultures at 37°C, 220 rpm overnight.
+*We picked 7 random colonies from A14 plate and infected 1 ml of LB + Amp. We incubated the inocula for 5 and 1/2 hours and then we prepared a glycerol stock for all of them.
-''Experiment with Tecan F200''
+*We re-filled the remaining 250 ul of bacterial culture with 5 ml of LB + Amp and incubated the new cultures at 37°C, 220 rpm overnight. Tomorrow they will be miniprepped and screened!
-* <html><u>Description</u></html>
-* <html><u>Purpose:</u></html>
-* <html><u>Materials & Methods</u></html>
-* <html><u>Protocol</u></html>
-* <html><u>Results</u></html>
+*We resuspended all the 5 ug of MRGENE1 and MRGENE2 with 20 ul of ddH2O.
-''Preparation of tomorrow's experiment with Tecan F200''
+*We transformed 1 ul of the resuspended DNA in TOP10. For each of the 2 plasmids, we plated 150 ul of transformed bacteria + SOC on an Amp plate and also on a Kan plate. In this way we could check if the plasmid had the expected antibiotic resistance.
-*We picked a colony from B0030 native plate (stored ad +4°C) and infected 5 ml of LB + Amp. We incubated the inoculum at 37°C, 220 rpm overnight.
+*We incubated the 4 plates at 37°C overnight. We stored the resuspended DNA at -20°C.
 <div align="right">
@@ Line 105: / Line 142: @@
 </div>
-== <html><font class="dayw_style">July, 8th</font></html> ==
+== <html><font class="dayw_style">July, 17th</font></html> ==
-*Gel run/cut/band purification for BOL1(E-S) overnight digestion. Results: gel showed that the enzymes had cut very well and this time also the purification gave a good quantification at Nanodrop.
+*Plates results:
+**MRGENE1 Amp plate - no colonies
+**MRGENE1 Kan plate - bacterial carpet!
+**MRGENE2 Amp plate - bacterial carpet!
+**MRGENE2 Kan plate - no colonies
+*The results were consistent with our expectations about the antibiotic resistances!
-*We took R0011(E-X) stored ad -20°C and we were ready to ligate;)
+*We picked a single colony from MRGENE1 and MRGENE2 plates and infected 3 ml of LB + suitable antibiotic. We incubated these inocula for about 6 hours. Then, we prepared three glycerol stocks for each of the two cultures in order to have good long term stocks.
-*Ligation:
+*We aliquoted the remaining 750 ul (=3 ml-750x3) in three falcon tubes containing 250 ul of bacterial culture and then we re-filled the falcon tubes with 5 ml of LB + suitable antibiotic to grow 6 overnight cultures.
-**A11: BOL1(E-S) + R0011(E-X) in pSB1A2
-*We incubated the ligation overnight at 16°C.
+*We also infected 5 ml of LB + Amp with 8 ul of B0030 glycerol stock to grow 3 identical 5 ml overnight cultures.
+*All the 9 cultures were incubated at 37°C, 220 rpm overnight.
-''Preparation of experiment with Tecan F200''
-*We diluted 1:100 the overnight culture of B0030.
+*Miniprep for the 7 cultures coming from the colonies of A14 plate.
+*Digestion E-P of 1 ug of DNA for all the 7 miniprepped plasmids (20 ul reaction volume).
+*Electrophoresis for the digestions.
+<table align="center">
+<tr>
+<td>
+<font class='didascalia'>
+[[Image:pv_digestion_A14.jpg|thumb|500px|left|Digestion screening: colonies 2 and 5 were negative, while the other colonies showed the correctly ligated plasmid, but with a smaller amount of unwanted plasmid.]]
+</font>
+</td>
+</tr>
+</table>
-''Experiment with Tecan F200 (continues the next day)''
+*Gel results:
+**A14-1 - positive insert(~2250 bp) + unwanted insert(~1400 bp) + unexpected band(~1100 bp)
+**A14-2 - unwanted insert(~1400 bp)
+**A14-3 - positive insert(~2250 bp) + unwanted insert(~1400 bp) + unexpected band(~1100 bp)
+**A14-4 - positive insert(~2250 bp) + unwanted insert(~1400 bp) + unexpected band(~1100 bp)
+**A14-5 - unwanted insert(~1400 bp)
+**A14-6 - positive insert(~2250 bp) + unwanted insert(~1400 bp)
+**A14-7 - positive insert(~2250 bp) + unwanted insert(~1400 bp) + unexpected band(~1100 bp)
-* <html><u>Description</u></html>
+*We decided to keep A14-4 glycerol stock in order to perform: i)inoculum, ii)miniprep, iii)dilution, iv) 5 pg transformation, v)plating, vi)digestion screening, as we performed for A8 and A9.
-* <html><u>Purpose:</u></html>
-* <html><u>Materials & Methods</u></html>
-* <html><u>Protocol</u></html>
-* <html><u>Results</u></html>
-<div align="right">
-[[#top|Top]]
-</div>
-== <html><font class="dayw_style">July, 9th</font></html> ==
-*We resuspended F2620 BioBrick from iGEM 2009 plates.
-*We transformed about 40 pg of the overnight ligation and 1 ul of the resuspended F2620 BioBrick. We plated transformed bacteria and incubated the two plates overnight at 37°C.
+*Miniprep for A12-2 and A12-3: DNA yield was quite low...next week they will be inoculated and miniprepped again in order to prepare the samples for sequencing.
-''End of experiment with Tecan F200 (last measurement)''
 <div align="right">
@@ Line 153: / Line 198: @@
 </div>
-== <html><font class="dayw_style">July, 10th</font></html> ==
+== <html><font class="dayw_style">July, 18th</font></html> ==
-*A11 and F2620 overnight plates showed colonies!
+*Miniprep for:
+{|cellpadding="20"
-*Colony PCR for 6 colonies of A11 plate: the picked colonies were inoculated in 1 ml of LB + Amp and incubated at 37°C, 220 rpm waiting for PCR results.
+|MRGENE1
+|MRGENE1-2
-*We also picked a colony from F2620 to infect 1 ml of LB + Amp. We incubated this inoculum with the others.
+|MRGENE1-3
+|-
-<font class='didascalia'>
+|MRGENE2
-{|align="center"
+|MRGENE2-2
-|[[Image:pv_colonypcr_A11.jpg|thumb|300px|left|Colony PCR for A11 plate: all the colonies showed the correct plasmid. We kept the 1st, 3rd and 6th colonies.]]
+|MRGENE2-3
+|-
+|B0030(X3)
 |}
-</font>
+*We stored the miniprepped DNA at -20°C. Next week we will be ready to assemble these bricks;)
-*Gel results: all the picked colonies showed the expected amplicon of a correctly ligated plasmid! We decided to prepare a glycerol stock for:
-**A11-1
-**A11-3
-**A11-6
-*Next week, only A11-1 will be used, but the other colonies will be used in case of failure.
-*We also prepared a glycerol stock for F2620 culture.
 <div align="right">
 [[#top|Top]]
 </div>
 <html>
 <hr/>
@@ Line 187: / Line 222: @@
 <tr>
 <td align="left" width="50%">
-<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week2Jul">
+<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week2Jul#week_start">
   <img src="https://2009.igem.org/Special:FilePath?file=Left_arrow.png"/>
 </a>
-<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week2Jul">Previous Week</a>
+<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week2Jul#week_start">Previous Week</a>
 </td>
 <td align="right" width="50%">
-<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week4Jul">Next Week</a>
+<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week4Jul#week_start">Next Week</a>
-<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week4Jul">
+<a href="https://2009.igem.org/Team:UNIPV-Pavia/Notebook/Week4Jul#week_start">
   <img src="https://2009.igem.org/Special:FilePath?file=Right_arrow.png"/>
 </a>