Team:Paris/Addressing testing

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Latest revision as of 03:53, 22 October 2009

iGEM > Paris > WetLab > Addressing

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WetLab - Addressing the message

Main | Addressing| Production| Reception

Global constructions :

The green color means the experiment was a success

Experiments ran :

Column 1	Column 2	Column 3	Column 4
PCR : pBAD: plate 2008 ClyA Cterm matrix : F4 Oligo :O10 and O31 TM :55°C mRFP Nterm plasmid : pSB1A3 Oligo :O57 and O58 TM : ClyA Nterm matrix : F4 Oligo : O32 and O9 TM :55°C mRFP Cterm matrix : pSB1A3 Oligo :O59 and O60 TM :	-	-	-
Verification on gel : ok	-	-	-
Purification on gel : ok	-	-	-
Digestion: ClyA Cterm S/P RFP Nterm X/P pBAD vector : ? E/S	Digestion: ClyA Cter-RFP Nter vector PSB1A3 E/X	-	-
Verification digestion: ok	Verification digestion: ok	-	-
Ligation: ClyA Cter-RFP Nter vector PSB1A3	Ligation: PBAD E/S ClyA Cter-RFP Nter PSB1A3 E/X (x2) PBAD S/P ClyA Cter-RFP Nter PSB2K3 X/P (x2)	Ligation: -
Colony PCR : ok	Colony PCR : ok	Colony PCR : ok
Miniprep: clone :	Miniprep: clone :	Miniprep: clone 3 clone 5
Sequencing : ok	Sequencing : ok	Sequencing : ok	-
Stock glycerol: ClyA CTer: S47(clone 3) and S48(clone 7) ClyA Nter: S72 RFP Cter: S55 (Clone 3) RFP Nter: S56 (Clone 3)	Stock glycerol Cly A(Cter)-(Nter)RFP: S72(clone 8)	Stock glycerol pBAD ClyA RFP : S89 (clone 3) pBAD ClyA RFP: S90 (clone 5)

Functional Testing:

PBAD ClyA RFP was transformed into Top10 bacteria in order to localize the fluorescence, we are supposed to have a superior fluorescence in the membrane.

PBAD ClyA RFP on PSB3T5 was transformed into Delta Tol bacteria , in this case we are supposed to see fluorescent vesicles when the medium contains 1 % arabinose , and to have no fluorescent on 1% glucose.

To learn more, see the Conclusion page

Export system

We finally thought that it won't be neccesary to overexpress the Tat system, nevertheless we have run a few experiments before starting to focus on others parts of the project.

Experiments ran :

Column 1	Column 2	Column 3	Column 4
PCR : TatABCE matrix :	-	-	-
Verification on gel : ok	-	-	-
Purification on gel : ok	-	-	-
Digestion: none	Digestion: none	Digestion: none	Digestion: none
Digestion checking: none	Digestion checking: none	Digestion checking: none	Digestion checking: none
Ligation: none	Ligation: none	Ligation: none	Ligation: none
Colony PCR : none	Colony PCR : none	Colony PCR : none	Colony PCR : none
Miniprep: none	Miniprep: none	Miniprep: none	Miniprep: none
Sequencing : none	Sequencing : none	Sequencing : none	Sequencing : none
Stock glycerol: none	Stock glycerol none	Stock glycerol none	Stock glycerol none

@@ Line 69: / Line 69: @@
-'''global constructions :'''
+<font style="color:black;font-weight:bold; font-size:21px">'''Global constructions :'''</font>
+<center><font style="color:green;font-weight:bold; font-size:16px">The green color means the experiment was a success</font></center>
@@ Line 76: / Line 81: @@
-Time required : A lot !!!!!
+<font style="color:black;font-weight:bold; font-size:18px"><I>'''Experiments ran :'''</I></font>
-'''Experiments ran :'''
 {|
-|- style="background: #0a3585; text-align: center; color:black; font-weight:bold; "
+|- style="background: #0a3585; text-align: center; color:black; font-weight:bold;font-size:14px "
-|width="300px" ; bgcolor="#F8F8F8"| column 1
+|width="300px" ; bgcolor="#F8F8F8"| Column 1
-|width="300px" ; bgcolor="#E0E3FE"| column 2
+|width="300px" ; bgcolor="#E0E3FE"| Column 2
-|width="300px" ; bgcolor="#CBD1FD"| column 3
+|width="300px" ; bgcolor="#CBD1FD"| Column 3
-|width="300px" ; bgcolor="#BCCDFD"| column 4
+|width="300px" ; bgcolor="#BCCDFD"| Column 4
 |- style="background: #bebebe; text-align: center;"
 |bgcolor="#F8F8F8"|'''PCR :'''
-ClyA Cterm  matrix : [https://2009.igem.org/Team:Paris/Fridge F4] Oligo :[https://2009.igem.org/Team:Paris/Freezer_Primers#O10 O10] and [https://2009.igem.org/Team:Paris/Freezer_Primers#O31 O31]  TM :55°C
+pBAD: plate 2008
-ClyA Nterm  matrix : [https://2009.igem.org/Team:Paris/Fridge F4] Oligo : [https://2009.igem.org/Team:Paris/Freezer_Primers#O32 O32] and [https://2009.igem.org/Team:Paris/Freezer_Primers#O9 O9] TM :55°C
-mRFP Cterm  matrix : ? Oligo :O59 and O60  TM :
+ClyA Cterm  matrix : [https://2009.igem.org/Team:Paris/Fridge F4]
-mRFP Nterm  plasmid : ? Oligo :O57 and O58 TM :
+Oligo :[https://2009.igem.org/Team:Paris/Freezer_Primers#O10 O10] and [https://2009.igem.org/Team:Paris/Freezer_Primers#O31 O31]  TM :55°C
-|'''PCR :'''
--
-|'''PCR :'''
--
+mRFP Nterm  plasmid : pSB1A3
-|'''PCR :'''
+Oligo :O57 and O58 TM :
+ClyA Nterm  matrix : [https://2009.igem.org/Team:Paris/Fridge F4]
+Oligo : [https://2009.igem.org/Team:Paris/Freezer_Primers#O32 O32] and [https://2009.igem.org/Team:Paris/Freezer_Primers#O9 O9] TM :55°C
+mRFP Cterm  matrix : pSB1A3
+Oligo :O59 and O60  TM :
+|bgcolor="#E0E3FE"|
+-
+|bgcolor="#CBD1FD"|
+-
+|bgcolor="#BCCDFD"|
 -
@@ Line 115: / Line 133: @@
 ok
-|'''Verification on gel :'''
+|bgcolor="#E0E3FE"|
 -
-|'''Verification on gel :'''
+|bgcolor="#CBD1FD"|
 -
-|'''Verification on gel :'''
+|bgcolor="#BCCDFD"|
 -
 |- style="background: #bebebe; text-align: center;"
-|'''Purification on gel :'''
+|bgcolor="#F8F8F8"| '''Purification on gel :'''
 ok
-|'''Purification on gel :'''
+|bgcolor="#E0E3FE"|
 -
-|'''Purification on gel :'''
+|bgcolor="#CBD1FD"|
 -
-|'''Purification on gel :'''
+|bgcolor="#BCCDFD"|
 -
 |- style="background: #d8d8d8; text-align: center;"
-|'''digestion:'''
+|bgcolor="#F8F8F8"|'''Digestion:'''
 ClyA Cterm S/P
 RFP  Nterm X/P
 pBAD  vector : ? E/S
@@ Line 154: / Line 173: @@
-|'''digestion:'''
+|bgcolor="#E0E3FE"|'''Digestion:'''
 ClyA Cter-RFP Nter vector PSB1A3 E/X
-|'''digestion:'''
+|bgcolor="#CBD1FD"|
 -
-|'''digestion:'''
+|bgcolor="#BCCDFD"|
 -
 |- style="background: #bebebe; text-align: center;"
-|'''verification digestion:'''
+|bgcolor="#F8F8F8"| '''Verification digestion:'''
 ok
-|'''verification digestion:'''
+|bgcolor="#E0E3FE"|'''Verification digestion:'''
 ok
-|'''verification digestion:'''
+|bgcolor="#CBD1FD"|-
+|bgcolor="#BCCDFD"|
 -
-|'''verification digestion:'''
--
 |- style="background: #d8d8d8; text-align: center;"
-|'''ligation:'''
+|bgcolor="#F8F8F8"|'''Ligation:'''
 ClyA Cter-RFP Nter  vector PSB1A3
-|'''ligation:'''
+|bgcolor="#E0E3FE"|'''Ligation:'''
 PBAD  E/S  ClyA Cter-RFP Nter PSB1A3 E/X (x2)
@@ Line 194: / Line 207: @@
 PBAD  S/P  ClyA Cter-RFP Nter PSB2K3   X/P (x2)
-|'''ligation:'''
+|bgcolor="#CBD1FD"|'''Ligation:'''
 -
-|'''ligation:'''
+|bgcolor="#BCCDFD"|
--
 |- style="background: #bebebe; text-align: center;"
-|'''PCR colo :'''
+|bgcolor="#F8F8F8"| '''Colony PCR :'''
 ok
-|'''PCR colo :'''
+|bgcolor="#E0E3FE"|'''Colony PCR :'''
 ok
-|'''PCR colo :'''
+|bgcolor="#CBD1FD"|'''Colony PCR :'''
--
+ok
-|'''PCR colo :'''
+|bgcolor="#BCCDFD"|
--
 |- style="background: #d8d8d8; text-align: center;"
-|'''miniprep:'''
+|bgcolor="#F8F8F8"|'''Miniprep:'''
 clone :
-|'''miniprep:'''
+|bgcolor="#E0E3FE"|'''Miniprep:'''
 clone :
-|'''miniprep:'''
+|bgcolor="#CBD1FD"|'''Miniprep:'''
--
+clone 3
-|'''miniprep:'''
+clone 5
+|bgcolor="#BCCDFD"|
--
 |- style="background: #bebebe; text-align: center;"
-|'''sequencing :'''
+|bgcolor="#F8F8F8"|'''Sequencing :'''
 ok
-|'''sequencing :'''
+|bgcolor="#E0E3FE"|'''Sequencing :'''
 ok
-|'''sequencing :'''
+|bgcolor="#CBD1FD"|'''Sequencing :'''
--
+ok
-|'''sequencing :'''
+|bgcolor="#BCCDFD"|
 -
 |- style="background: #d8d8d8; text-align: center;"
-|'''stock glycerol:'''
+|bgcolor="#F8F8F8"| '''Stock glycerol:'''
 ClyA CTer: S47(clone 3) and S48(clone 7)
@@ Line 264: / Line 278: @@
-|'''stock glycerol'''
+|bgcolor="#E0E3FE"|'''Stock glycerol'''
 Cly A(Cter)-(Nter)RFP: S72(clone 8)
-|'''stock glycerol'''
+|bgcolor="#CBD1FD"|'''Stock glycerol'''
--
+pBAD ClyA RFP : S89 (clone 3)
-|'''stock glycerol'''
--
+pBAD ClyA RFP: S90 (clone 5)
+|bgcolor="#BCCDFD"|
@@ Line 285: / Line 300: @@
-PBAD ClyA RFP on PSB3T5 was transformed into Delta Tol bacteria , in this case we are supposed to see fluorescent vesicles went the medium contains 1 % arabinose , and to have no fluorescent on 1% glucose.
+PBAD ClyA RFP on PSB3T5 was transformed into Delta Tol bacteria , in this case we are supposed to see fluorescent vesicles when the medium contains 1 % arabinose , and to have no fluorescent on 1% glucose.
+To learn more, see the [[Team:Paris/Conclusion | Conclusion page]]
@@ Line 300: / Line 318: @@
-Time required : A week.
+<font style="color:black;font-weight:bold; font-size:18px"><I>'''Experiments ran :'''</I></font>
-Experiments ran :
 {|
-|- style="background: #0a3585; text-align: center; color:black; font-weight:bold; "
+|- style="background: #0a3585; text-align: center; color:black; font-weight:bold;font-size:14px "
-|width="300px" ; bgcolor="#F8F8F8"| column 1
+|width="300px" ; bgcolor="#F8F8F8"| Column 1
-|width="300px" ; bgcolor="#E0E3FE"| column 2
+|width="300px" ; bgcolor="#E0E3FE"| Column 2
-|width="300px" ; bgcolor="#CBD1FD"| column 3
+|width="300px" ; bgcolor="#CBD1FD"| Column 3
-|width="300px" ; bgcolor="#BCCDFD"| column 4
+|width="300px" ; bgcolor="#BCCDFD"| Column 4
 |- style="background: #bebebe; text-align: center;"
-|'''PCR :'''
+|bgcolor="#F8F8F8"|'''PCR :'''
 TatABCE matrix :
-|'''PCR :'''
+|bgcolor="#E0E3FE"|-
-|'''PCR :'''
+|bgcolor="#CBD1FD"|-
-|'''PCR :'''
+|bgcolor="#BCCDFD"|-
 |- style="background: #d8d8d8; text-align: center;"
-|'''Verification on gel :'''
+|bgcolor="#F8F8F8"|'''Verification on gel :'''
 ok
-|'''Verification on gel :'''
+|bgcolor="#E0E3FE"|-
--
+|bgcolor="#CBD1FD"|
-|'''Verification on gel :'''
 -
-|'''Verification on gel :'''
+|bgcolor="#BCCDFD"|
 -
 |- style="background: #bebebe; text-align: center;"
-|'''Purification on gel :'''
+|bgcolor="#F8F8F8"|'''Purification on gel :'''
 ok
-|'''Purification on gel :'''
+|bgcolor="#E0E3FE"|
 -
-|'''Purification on gel :'''
+|bgcolor="#CBD1FD"|
 -
-|'''Purification on gel :'''
+|bgcolor="#BCCDFD"|
 -
@@ Line 359: / Line 374: @@
 |- style="background: #d8d8d8; text-align: center;"
-|'''digestion:'''
+|bgcolor="#F8F8F8"|'''Digestion:'''
-TatABCE
+none
-|'''digestion:'''
+|bgcolor="#E0E3FE"|'''Digestion:'''
-|'''digestion:'''
+none
-|'''digestion:'''
+|bgcolor="#CBD1FD"|'''Digestion:'''
+none
+|bgcolor="#BCCDFD"|'''Digestion:'''
+none
 |- style="background: #bebebe; text-align: center;"
-|'''verification digestion:'''
+|bgcolor="#F8F8F8"|'''Digestion checking:'''
+none
-ok
+|bgcolor="#E0E3FE"|'''Digestion checking:'''
+none
-|'''verification digestion:'''
--
+|bgcolor="#CBD1FD"|'''Digestion checking:'''
-|'''verification digestion:'''
+none
+|bgcolor="#BCCDFD"|'''Digestion checking:'''
--
+none
-|'''verification digestion:'''
--
 |- style="background: #d8d8d8; text-align: center;"
-|'''ligation:'''
+|bgcolor="#F8F8F8"|'''Ligation:'''
-TatABCE
+none
+|bgcolor="#E0E3FE"|'''Ligation:'''
-|'''ligation:'''
+none
-|'''ligation:'''
+|bgcolor="#CBD1FD"|'''Ligation:'''
-|'''ligation:'''
+none
+|bgcolor="#BCCDFD"|'''Ligation:'''
+none
 |- style="background: #bebebe; text-align: center;"
-|'''PCR colo :'''
+|bgcolor="#F8F8F8"|'''Colony PCR :'''
+none
-ok
+|bgcolor="#E0E3FE"|'''Colony PCR :'''
+none
-|'''PCR colo :'''
+|bgcolor="#CBD1FD"|'''Colony PCR :'''
+none
+|bgcolor="#BCCDFD"|'''Colony PCR :'''
+none
--
+|- style="background: #d8d8d8; text-align: center;"
+|bgcolor="#F8F8F8"|'''Miniprep:'''
-|'''PCR colo :'''
+none
--
+|bgcolor="#E0E3FE"|'''Miniprep:'''
-|'''PCR colo :'''
--
+none
-|- style="background: #d8d8d8; text-align: center;"
+|bgcolor="#CBD1FD"|'''Miniprep:'''
-|'''miniprep:'''
-STOPPED
+none
-|'''miniprep:'''
+|bgcolor="#BCCDFD"|'''Miniprep:'''
--
+none
-|'''miniprep:'''
+|- style="background: #bebebe; text-align: center;"
+|bgcolor="#F8F8F8"|'''Sequencing :'''
--
+none
-|'''miniprep:'''
+|bgcolor="#E0E3FE"|'''Sequencing :'''
--
+none
-|- style="background: #bebebe; text-align: center;"
+|bgcolor="#CBD1FD"|'''Sequencing :'''
-|'''sequencing :'''
--
+none
+|bgcolor="#BCCDFD"|'''Sequencing :'''
-|'''sequencing :'''
+none
--
+|- style="background: #d8d8d8; text-align: center;"
+|bgcolor="#F8F8F8"| '''Stock glycerol:'''
-|'''sequencing :'''
+none
+|bgcolor="#E0E3FE"|'''Stock glycerol'''
--
+none
-|'''sequencing :'''
+|bgcolor="#CBD1FD"|'''Stock glycerol'''
--
+none
+|bgcolor="#BCCDFD"|'''Stock glycerol'''
+none
 |}