Team:UNIPV-Pavia/Calendar/September/settimana5

From 2010.igem.org

(Difference between revisions)
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<br>
<br>
-
<html><p align="center"><font size="4"><b>SEPTEMBER: WEEK 4</b></font></p></html><hr><br>
+
<html><p align="center"><font size="4"><b>SEPTEMBER: WEEK 5</b></font></p></html><hr><br>
<html><a name="indice"/></html>
<html><a name="indice"/></html>
==September, 27th==
==September, 27th==
 +
<font size=4>[[Team:UNIPV-Pavia/Material Methods/Measurements/Tecan/test27settembre|Tecan Test]]</font>
 +
 +
----
MiniPrep and E-P digest for I62-a, I62-b, I62-c, I62-d, I62-e, I62-f
MiniPrep and E-P digest for I62-a, I62-b, I62-c, I62-d, I62-e, I62-f
-
DNA pcr for MyYeast 1-2-3
+
DNA PCR for MyYeast 1-2-3
Gel run
Gel run
-
[[Image:UNIPV10_27_09_2010_I62_screen.jpg|thumb|200px|center|I62 and MyYeast series screening (I62, blank, MyYeastx,xbis).]]
+
[[Image:UNIPV10_27_09_2010_I62_screen.jpg|thumb|200px|center|I62 and MyYeast screening.]]
Line 48: Line 51:
-
Protein electrophoresis for phasins (Fede)
+
Protein electrophoresis for phasins.
<div align="right"><small>[[#indice|^top]]</small></div>
<div align="right"><small>[[#indice|^top]]</small></div>
==September, 28th==
==September, 28th==
-
Tecan Test Giacomo
+
<font size=4>[[Team:UNIPV-Pavia/Material Methods/Measurements/Tecan/test28settembre|Tecan Test]]</font>
----
----
Line 76: Line 79:
==September, 29th==
==September, 29th==
-
Tecan Test Giacomo
 
-
----
 
Colony PCR for 6 newly picked colonies.
Colony PCR for 6 newly picked colonies.
-
[[Image:UNIPV10_29_09_2010_I55_screen.jpg|thumb|200px|center|I55 colony PCR screening (blank blank 1 ..).]]
+
[[Image:UNIPV10_29_09_2010_I55_screen.jpg|thumb|200px|center|I55 colony PCR screening.]]
No positives nor this time.
No positives nor this time.
----
----
Line 86: Line 87:
Gel run for all digested parts
Gel run for all digested parts
-
[[Image:UNIPV10_29_09_2010_digestions.jpg|thumb|200px|center|Digestions (4C5 myYeast3 I4 I53 J04450-2 J04450-1 I1).]]
+
[[Image:UNIPV10_29_09_2010_digestions.jpg|thumb|200px|center|Digestions.]]
-
and gel run/cut/purification for:
+
and cut/gel purification for:
*4C5 (E-P): 19,3 ng/ul
*4C5 (E-P): 19,3 ng/ul
*My Yeast 3 (E-S): 20,8 ng/ul
*My Yeast 3 (E-S): 20,8 ng/ul
Line 108: Line 109:
|}
|}
 +
----
 +
Inoculum of MC43, MG43 in 5ml LB with chloramphenicol concentration of 12.5 ug/ml.
Line 114: Line 117:
==September, 30th==
==September, 30th==
 +
<font size=4>[[Team:UNIPV-Pavia/Material Methods/Measurements/Tecan/test30settembre|Tecan Test]]</font>
 +
 +
----
 +
Transformation of I73 (1ul) into ''E. coli'' TOP10. It was plated on LB+Amp 100 ug/ml agar plate.
Transformation of I73 (1ul) into ''E. coli'' TOP10. It was plated on LB+Amp 100 ug/ml agar plate.
 +
 +
Trasformation of:
 +
*I70 (myYeast with I4, Ptef1-mOrange-tAdh1) in TOP10 and plated on LB+Amp
 +
*I71 (myYeast with I1, mOrange-tAdh1) in TOP10 and plated on LB+Amp
 +
*I72 (pLac-RFP in pSB4C5) in TOP10 and plated on LB+Cm 12,5
 +
 +
All plates were incubated at 37°C ON
Line 120: Line 134:
*I20: (E-X)
*I20: (E-X)
-
Gel run/cut
+
Gel run/cut/extraction/quantification
 +
[[Image:UNIPV10_30_09_2010_I20_E_X.jpg|thumb|70px|center|I20 E-X digest.]]
 +
I20 E-X: 13,4 ng/ul
-
[[Image:UNIPV10_30_09_2010_I20_E_X.jpg|thumb|200px|center|I20 E-P digest.]]
 
We repeated I55 ligation using newly digested vector and already digested I38 (E-S)
We repeated I55 ligation using newly digested vector and already digested I38 (E-S)
 +
 +
I55: I38 (E-S) + I20 (E-X)
Inoculum into 5ml LB+Amp of:
Inoculum into 5ml LB+Amp of:
Line 137: Line 154:
----
----
 +
Inoculum of E. coli TOP10 in 1,5 ml LB, grown ON at 37°C 220 rpm. Tomorrow we will prepare competent cells!!
 +
Inoculum of:
 +
 +
*S1 in 500ul M9+Cm 12,5
 +
*I47-S1  in 500ul M9+Amp+Cm 12,5
 +
*GFP-S1  in 500ul M9+Amp+Cm 12,5
 +
*RBS32  in 500ul M9+Amp
 +
 +
Cultures were grown ON at 37°C 220 rpm.
 +
 +
Tomorrow we will test the ability of these strains to produce GFP and to lyse when HSL is added.
 +
 +
----
 +
In order to excise the chloramphenicol resistance cassette from the integrants in E.coli genome we transformed the cells with a plasmid (pCP20 plasmid) carrying the gene encoding for the flippase protein. This protein is able to cut fragment between two FRT flanking sequences. pCP20 was transformed in MC43-a and MG43-a and plated on LB+Amp agar plate.
<div align="right"><small>[[#indice|^top]]</small></div>
<div align="right"><small>[[#indice|^top]]</small></div>
Line 143: Line 174:
==October, 1st==
==October, 1st==
-
Transformation of I55 into ''E. coli'' DH5-alpha. It was plated on LB+Amp 100 agar plate.
+
<font size=4>[[Team:UNIPV-Pavia/Material Methods/Measurements/Tecan/test1ottobre|Tecan Test]]</font>
----
----
-
Miniprep and Nanodrop quantification for:
+
This morning, we checked tranformed plates:
-
*I31:
+
-
*I35:
+
-
*I60:
+
-
(they were also send sequencing)
+
*I72 showed NO colony!! :/ we will repeat this ligation next week
-
*INTEIN
+
*I70 and I71 showed colonies, 5 for each plate were picked and inoculated in 1ml LB+Amp to prepare glycerol stocks and for screening.
-
*<partinfo>pSB1C3</partinfo>:
+
*I73 showed colonies; six of them were picked and inoculated into 5 ml LB+Amp and let grow ON at 37°C, 220rpm in order to do E-P screeening the following day.
-
*I37:
+
 
-
*I53:
+
----
 +
 
 +
Transformation of I55 into ''E. coli'' DH5-alpha. It was plated on LB+Amp 100 agar plate and let grow ON at +37°C.
 +
 
 +
----
 +
 
 +
Miniprep and Nanodrop quantification for:
 +
*I31: 76,1 ng/ul
 +
*I35: 66,8 ng/ul
 +
*I60: 279,7 ng/ul
 +
(they were also sent sequencing)
 +
*INTEIN: 123,8 ng/ul
 +
*<partinfo>pSB1C3</partinfo>-1: 104,8 ng/ul
 +
*<partinfo>pSB1C3</partinfo>-2: 141,2 ng/ul
 +
*<partinfo>pSB1C3</partinfo>-3: 113,5 ng/ul
 +
*I37: 174,9 ng/ul
Digest:
Digest:
Line 165: Line 208:
*I60: E-S
*I60: E-S
*I31: S-P
*I31: S-P
-
*I35: X-P
+
*I35: E-P
 +
*I35: E-X
*I37: E-X
*I37: E-X
*I57: E-X
*I57: E-X
Gel run/cut/extraction/quantification:
Gel run/cut/extraction/quantification:
 +
{|align="center"
 +
|[[Image:UNIPV10_01_10_2010_digestioni_medio.jpg|thumb|200px|center|Intein, I31, I35, I37, I57, I60 digestions]] || [[Image:UNIPV10_01_10_2010_digestioni_psb1c3.jpg|thumb|150px|center|<partinfo>pSB1C3</partinfo> digested E-P (both vector and insert were kept), E-S, X-P.]]
 +
|}
-
(foto)
+
*I37 (E-X): 20,4 ng/ul
-
 
+
*I57 (E-X): 17,6 ng/ul
-
*I60:
+
*I60 (E-S): 9,5 ng/ul
-
*I37:
+
They were stored at -20°C.
-
*I57:
+
*I31 (E-S): 5,4 ng/ul
-
They were stored at -20°C
+
*I35 (E-P): 1,0 ng/ul ;-(
-
*I31:
+
*I35 (E-X): 14,4 ng/ul
-
*I35:
+
*<partinfo>pSB1C3</partinfo> (E-P): 14,3 ng/ul
 +
*<partinfo>pSB1C3</partinfo> (E-S): 15,2 ng/ul
 +
*<partinfo>pSB1C3</partinfo> (X-P): 13,9 ng/ul
ON ligation of:
ON ligation of:
-
*IXX: I31 (S-P) + I35 (X-P) (in vector <partinfo>pSB1A2</partinfo>)
+
*I74: I31 (E-S) + I35 (E-X)
*INTEIN_C3: INTEIN (E-P) + <partinfo>pSB1C3</partinfo> (E-P)
*INTEIN_C3: INTEIN (E-P) + <partinfo>pSB1C3</partinfo> (E-P)
----
----
-
Pick and inoculum of I73 into 5 ml LB+Amp 100. It was let grow ON at 37°C, 220 rpm.
+
Single colony was picked from MC43 and MG43 plates and inoculated in 5 ml of LB and incubated at 37°C, 220 rpm ON.
-
 
+
12 hours late 5 ul were streaked on non selective LB plates and incubated at 43°C ON in order to ensure the loss of pCP20 plasmid.
Line 193: Line 242:
==October, 2nd==
==October, 2nd==
 +
 +
PCR from colony for I55 (eleven colonies were picked).
 +
 +
Gel run:
 +
 +
[[Image:UNIPV10_02_10_2010_I55_screening.jpg|thumb|200px|center|I55 colony PCR screening.]]
 +
 +
We decided to make glycerol stock for I55-1. Inoculum into 5 ml LB+Amp of the positive culture that was let grow ON at 37°C, 220 rpm.
 +
----
 +
Miniprep and quantification for I73-1/2/3/4/5/6:
 +
*I73-1: 154 ng/ul
 +
*I73-2: 177 ng/ul
 +
*I73-3: 154,7 ng/ul
 +
*I73-4: 145,5ng/ul
 +
*I73-5: 152,6 ng/ul
 +
*I73-6: 154,2 ng/ul
 +
1,5 hours E-P digest (for screening) and gel run
 +
 +
[[Image:UNIPV10_02_10_2010_I73_screening.jpg|thumb|200px|center|I70, I71, I73, A9_4C5, A99_4C5 screening.]]
 +
 +
As you can see they are (except for I73-6) all positive. So we stocked I73-1 and stored it at -80°C.
 +
 +
----
 +
Transformation of I74 and INTEIN_C3 (1ul) in ''E. coli'' TOP10. They were plated on LB+Amp100 and LB+Cm34 agar plates respectively. They were let grow ON at +37°C.
 +
 +
----
 +
Inoculum of I55-1 into 5 ml LB+Amp. ON growth at +37°C, 220 rpm.
 +
 +
----
 +
 +
3 colonies each plate were picked from MC43_flip and MG43_flip plates and inoculated in 5 ml of non selective LB. To confirm the loss of the chloramphenicol resistance cassette and of the pCP20 plasmid, each colony was inoculated also in 5 ml of LB+Cm12.5 and 5 ml of LB+Amp.
 +
 +
<div align="right"><small>[[#indice|^top]]</small></div>
 +
 +
==October, 3rd==
 +
Glycerol stock for:
 +
*I55-1
 +
*IC-1/2/3/4-4C5
 +
 +
----
 +
Pick of a single non-red colony of INTEIN_C3 and inoculum into 5 ml LB+Cm34. Sample was let grow ON at +37°C, 220 rpm.
 +
 +
----
 +
Miniprep and quantification of:
 +
*I55-1: 57,4 ng/ul
 +
*I55-1bis: 79,6 ng/ul
 +
 +
I55-1bis was digested E-S for about three hours and than gel run/cut.
 +
 +
----
 +
 +
Colony PCR for I74-1..6.
 +
 +
----
 +
Gel run for PCR samples and I55 (E-S) and cut for this one.
 +
[[Image:UNIPV10_03_10_2010_I74_screen_I55_cut.jpg|thumb|200px|center|I74 screening and I55 E-S cut.]]
 +
Very bad PCR. We performed a massive PCR from colony during the night (I74-7..24), we ran it the following day.
 +
 +
Gel extraction and quantification:
 +
*I55 (E-S): 5,0 ng/ul
 +
 +
Ligation of I55 (E-S) with already available DNA:
 +
*I75: I55 (E-S) + I37 (E-X)
 +
*I77: I55 (E-S) + I57 (E-X)
 +
----
 +
Inoculum of I35 (last quantification after gel extraction was too poor; we will digest it again E-P) and I54 into 5 ml LB+Amp: ON growth at +37°C, 220 rpm.
 +
 +
----
 +
Each culture of MC43_flip and MG43_flip in selective LB didn't grown, confirming the loss of pCP20 plasmid and of the chloramphenicol resistance cassette integrated into the E.coli genome.
<div align="right"><small>[[#indice|^top]]</small></div>
<div align="right"><small>[[#indice|^top]]</small></div>

Latest revision as of 18:36, 27 October 2010
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Week 5


SEPTEMBER: WEEK 5


September, 27th

Tecan Test

MiniPrep and E-P digest for I62-a, I62-b, I62-c, I62-d, I62-e, I62-f

DNA PCR for MyYeast 1-2-3

Gel run

I62 and MyYeast screening.


I62-e was positive, so we made glycerol stock and stored it at -80°C.


Protein electrophoresis for phasins.

September, 28th

Tecan Test

Miniprep and quantification for:

  • I1: 59,6 ng/ul
  • I4: 109,9 ng/ul
  • I53: 160,3 ng/ul
  • <partinfo>BBa_J04450</partinfo>-1:55,9 ng/ul
  • <partinfo>BBa_J04450</partinfo>-2: 47 ng/ul

ON digestion of:

  • I1 (E-S)
  • I4 (E-S)
  • I53 (E-X)
  • <partinfo>BBa_J04450</partinfo>-1 (E-P)
  • <partinfo>BBa_J04450</partinfo>-2 (E-P)
  • MyYeast-3 (DNA already available) (E-S)
  • <partinfo>pSB4C5</partinfo> (DNA already available) (E-P)


September, 29th

Colony PCR for 6 newly picked colonies.

I55 colony PCR screening.

No positives nor this time.


Gel run for all digested parts

Digestions.

and cut/gel purification for:

  • 4C5 (E-P): 19,3 ng/ul
  • My Yeast 3 (E-S): 20,8 ng/ul
  • I1: 3,8 ng/ul
  • I4 (E-S): 14,2 ng/ul
  • I53 (E-X): 21,6 ng/ul
  • <partinfo>BBa_J04450</partinfo> (pLac-RBS-mRFP-TT) (E-P): 5,6 ng/ul
  • <partinfo>pSB1C3</partinfo>: 10 ng/ul


Ligation of:

I70=MyYeast 3(E-S)+I4(E-S)
I71=MyYeast 3(E-S)+I1(E-S)
I72=<partinfo>BBa_J04450</partinfo>(E-P)+<partinfo>pSB4C5</partinfo>
I73= I38 (E-S) + I53 (E-X)

Inoculum of MC43, MG43 in 5ml LB with chloramphenicol concentration of 12.5 ug/ml.


September, 30th

Tecan Test

Transformation of I73 (1ul) into E. coli TOP10. It was plated on LB+Amp 100 ug/ml agar plate.

Trasformation of:

  • I70 (myYeast with I4, Ptef1-mOrange-tAdh1) in TOP10 and plated on LB+Amp
  • I71 (myYeast with I1, mOrange-tAdh1) in TOP10 and plated on LB+Amp
  • I72 (pLac-RFP in pSB4C5) in TOP10 and plated on LB+Cm 12,5

All plates were incubated at 37°C ON


Since I55 was negative again we decided to ligate it again (probably we had a bad digest for vector - I20 - and a good one for insert - we used I38 in other ligations without problems). We diegested already miniprepped DNA for three hours with 1 ul of enzymes:

  • I20: (E-X)

Gel run/cut/extraction/quantification

I20 E-X digest.

I20 E-X: 13,4 ng/ul

We repeated I55 ligation using newly digested vector and already digested I38 (E-S)

I55: I38 (E-S) + I20 (E-X)

Inoculum into 5ml LB+Amp of:

  • I31
  • I35
  • I37
  • I57
  • I60
  • INTEIN
  • 3x <partinfo>BBa_J04450</partinfo> (to take <partinfo>pSB1C3</partinfo>, so <partinfo>pSB1C3</partinfo> from now on)

Cultures were let grow ON at 37°C, 220 rpm.

Inoculum of E. coli TOP10 in 1,5 ml LB, grown ON at 37°C 220 rpm. Tomorrow we will prepare competent cells!!

Inoculum of:

  • S1 in 500ul M9+Cm 12,5
  • I47-S1 in 500ul M9+Amp+Cm 12,5
  • GFP-S1 in 500ul M9+Amp+Cm 12,5
  • RBS32 in 500ul M9+Amp

Cultures were grown ON at 37°C 220 rpm.

Tomorrow we will test the ability of these strains to produce GFP and to lyse when HSL is added.

In order to excise the chloramphenicol resistance cassette from the integrants in E.coli genome we transformed the cells with a plasmid (pCP20 plasmid) carrying the gene encoding for the flippase protein. This protein is able to cut fragment between two FRT flanking sequences. pCP20 was transformed in MC43-a and MG43-a and plated on LB+Amp agar plate.

October, 1st

Tecan Test

This morning, we checked tranformed plates:

  • I72 showed NO colony!! :/ we will repeat this ligation next week
  • I70 and I71 showed colonies, 5 for each plate were picked and inoculated in 1ml LB+Amp to prepare glycerol stocks and for screening.
  • I73 showed colonies; six of them were picked and inoculated into 5 ml LB+Amp and let grow ON at 37°C, 220rpm in order to do E-P screeening the following day.

Transformation of I55 into E. coli DH5-alpha. It was plated on LB+Amp 100 agar plate and let grow ON at +37°C.

Miniprep and Nanodrop quantification for:

  • I31: 76,1 ng/ul
  • I35: 66,8 ng/ul
  • I60: 279,7 ng/ul

(they were also sent sequencing)

  • INTEIN: 123,8 ng/ul
  • <partinfo>pSB1C3</partinfo>-1: 104,8 ng/ul
  • <partinfo>pSB1C3</partinfo>-2: 141,2 ng/ul
  • <partinfo>pSB1C3</partinfo>-3: 113,5 ng/ul
  • I37: 174,9 ng/ul

Digest:

  • <partinfo>pSB1C3</partinfo>: E-P
  • <partinfo>pSB1C3</partinfo>: E-S
  • <partinfo>pSB1C3</partinfo>: X-P
  • INTEIN: E-P
  • I60: E-S
  • I31: S-P
  • I35: E-P
  • I35: E-X
  • I37: E-X
  • I57: E-X

Gel run/cut/extraction/quantification:

Intein, I31, I35, I37, I57, I60 digestions
<partinfo>pSB1C3</partinfo> digested E-P (both vector and insert were kept), E-S, X-P.
  • I37 (E-X): 20,4 ng/ul
  • I57 (E-X): 17,6 ng/ul
  • I60 (E-S): 9,5 ng/ul

They were stored at -20°C.

  • I31 (E-S): 5,4 ng/ul
  • I35 (E-P): 1,0 ng/ul ;-(
  • I35 (E-X): 14,4 ng/ul
  • <partinfo>pSB1C3</partinfo> (E-P): 14,3 ng/ul
  • <partinfo>pSB1C3</partinfo> (E-S): 15,2 ng/ul
  • <partinfo>pSB1C3</partinfo> (X-P): 13,9 ng/ul

ON ligation of:

  • I74: I31 (E-S) + I35 (E-X)
  • INTEIN_C3: INTEIN (E-P) + <partinfo>pSB1C3</partinfo> (E-P)

Single colony was picked from MC43 and MG43 plates and inoculated in 5 ml of LB and incubated at 37°C, 220 rpm ON. 12 hours late 5 ul were streaked on non selective LB plates and incubated at 43°C ON in order to ensure the loss of pCP20 plasmid.


October, 2nd

PCR from colony for I55 (eleven colonies were picked).

Gel run:

I55 colony PCR screening.

We decided to make glycerol stock for I55-1. Inoculum into 5 ml LB+Amp of the positive culture that was let grow ON at 37°C, 220 rpm.

Miniprep and quantification for I73-1/2/3/4/5/6:

  • I73-1: 154 ng/ul
  • I73-2: 177 ng/ul
  • I73-3: 154,7 ng/ul
  • I73-4: 145,5ng/ul
  • I73-5: 152,6 ng/ul
  • I73-6: 154,2 ng/ul

1,5 hours E-P digest (for screening) and gel run

I70, I71, I73, A9_4C5, A99_4C5 screening.

As you can see they are (except for I73-6) all positive. So we stocked I73-1 and stored it at -80°C.

Transformation of I74 and INTEIN_C3 (1ul) in E. coli TOP10. They were plated on LB+Amp100 and LB+Cm34 agar plates respectively. They were let grow ON at +37°C.

Inoculum of I55-1 into 5 ml LB+Amp. ON growth at +37°C, 220 rpm.

3 colonies each plate were picked from MC43_flip and MG43_flip plates and inoculated in 5 ml of non selective LB. To confirm the loss of the chloramphenicol resistance cassette and of the pCP20 plasmid, each colony was inoculated also in 5 ml of LB+Cm12.5 and 5 ml of LB+Amp.

October, 3rd

Glycerol stock for:

  • I55-1
  • IC-1/2/3/4-4C5

Pick of a single non-red colony of INTEIN_C3 and inoculum into 5 ml LB+Cm34. Sample was let grow ON at +37°C, 220 rpm.

Miniprep and quantification of:

  • I55-1: 57,4 ng/ul
  • I55-1bis: 79,6 ng/ul

I55-1bis was digested E-S for about three hours and than gel run/cut.

Colony PCR for I74-1..6.

Gel run for PCR samples and I55 (E-S) and cut for this one.

I74 screening and I55 E-S cut.

Very bad PCR. We performed a massive PCR from colony during the night (I74-7..24), we ran it the following day.

Gel extraction and quantification:

  • I55 (E-S): 5,0 ng/ul

Ligation of I55 (E-S) with already available DNA:

  • I75: I55 (E-S) + I37 (E-X)
  • I77: I55 (E-S) + I57 (E-X)

Inoculum of I35 (last quantification after gel extraction was too poor; we will digest it again E-P) and I54 into 5 ml LB+Amp: ON growth at +37°C, 220 rpm.

Each culture of MC43_flip and MG43_flip in selective LB didn't grown, confirming the loss of pCP20 plasmid and of the chloramphenicol resistance cassette integrated into the E.coli genome.



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