Latest revision as of 14:47, 6 September 2008

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1 Construction for FIFO
- 1.1 Results of the transformation we did Yesterday
2 Construction of pFlgA - GFP Generator
- 2.1 Transformation of the ligations we did yesterday
3 Construction for Synchronization
- 3.1 Results of the transformation we did yesterday
  - 3.1.1 Number of colonies
- 3.2 Digestion
4 Promoter characterization plasmids
- 4.1 Transformation results: ligations from August 21th

Construction for FIFO

Aim : Construction of pFlgA - YFP tripart (+/- LVA) "pFlgA-RBS-YFP-dbl ter" (pFlgA-E0430/E0432)

Results of the transformation we did Yesterday

Ligation name	Description	Antibio	Number Colonies observed	Fluorescence	Comments
Ligations
L160	D166(FV) - D132(FI) pFlgA - YFP tripart (LVA-)	Amp	44	No	ok
L161	D167(FV) - D132(FI) pFlgA - YFP tripart (LVA+)	Amp	3	No	ok
Controls
TL160	D166 (FV) YFP tripart (LVA-)	Amp	(+++)	No	-
TL161	D167 (FV) YFP tripart (LVA+)	Amp	0	No	ok
Positive Control	pUC19	Amp	720 (efficiency 7.2.10^7)	No	OK

=> Need to screen to know which clones we can use for the  of  pFlgA promotor cconstruction.

Construction of pFlgA - GFP Generator

Aim : Construction of "pFlgA-RBS-GFP-dbl ter" (pFlgA-E0240)

Transformation of the ligations we did yesterday

Protocol

Ligation Name	Description	Antibio
L164	D168 (FV) + D132 (FI) pFlgA - gfp generator	Amp
Control L164	D168 gfp generator	Amp

Construction for Synchronization

Results of the transformation we did yesterday

Number of colonies

Ligation name	Description	Antibio	Number Colonies observed	Fluorescence	Comments
Ligations
L158	D110(BV) - D131(BI) rbs-TetR - gfp tripart	Amp	-	-	to do again
L159	D125(FV) - D109(FI) rbs-LasI - double terminator	Kan	-	-	to do again
L162	D107(BV) - D163(BI) rbs-LasI - gfp generator	Amp	-	-	to do again
L163	D110(BV) - D163(BI) rbs-TetR - gfp generator	Amp	-	-	to do again
Controls
TL158	D110(BV)	Amp	-	-	to do again
TL159	D125(FV)	Kan	-	-	to do again
TL162	D107(BV)	Amp	-	-	to do again
TL163	D110(BV)	Amp	-	-	to do again
Positive Control	pUC19	Amp	358 (efficiency 3.5.10^7)	No	OK

=> We decided to do again the digestions of the ligation's reactions

Digestion

Protocol

Name	Template DNA	Description	Vol MP (µl)	Vol H2O (µl)	Enzymes
D107	MP105.1	rbs-LasI (BV)	14.7 (0.5µg of plasmid)	11	SpeI / PstI
D109	MP105.1	rbs-LasI (FI)	14.7	11	EcoRI / SpeI
D110	MP106	rbs-TetR (BV)	9	15.7	SpeI / PstI
D125	MP118.1	Double terminator (FV)	4.54	20.16	EcoRI and XbaI
D163	MP143	gfp generator (BI)	6.66	18.04	XbaI and PstI

Promoter characterization plasmids

Transformation results: ligations from August 21th

Top 10 cells were used

Protocol

Ligation name	Vector digestion	Vector description	Insert digestion	Insert description	Product description	Antibiotic	Number of colonies
L155	D164	J23101 promoter	D163	gfp generator	J23101 promoter-gfp generator	Amp	0
L156	D161	pTet promoter	D163	gfp generator	pTet promoter-gfp generator	Kana	0
Control L156	D161		none		Vector autoligation control	Kana	1
L157	D125.2	B0015	D162	tetR	tetR-B0015	Kana	1
Control L157	D125.2		none		Vector autoligation control	Kana	0
L166	D185	RBS B0032	D182	tetR	RBS B0032 - tetR	Amp	68
Control L166	D185		none		Vector autoligation control	Amp	49
L167	D181	pTet	D184	gfp generator	gfp generator - pTet	Amp	1

@@ Line 6: / Line 6: @@
 Aim : Construction of pFlgA - YFP tripart (+/- LVA)''' "pFlgA-RBS-YFP-dbl ter" (pFlgA-E0430/E0432)''' [[Image:Part_icon_regulatory.png]][[Image:Part_icon_rbs.png]][[Image:icon_reporter.png]][[Image:Part_icon_terminator.png]][[Image:Part_icon_terminator.png]]
 =='''Results of the transformation we did [[Team:Paris/August 22  |Yesterday]]'''==
@@ Line 25: / Line 24: @@
 | 44
 | No
-| ok
+|style="background: #cbff7B"| ok
 |-
 |L161
@@ Line 32: / Line 31: @@
 | 3
 | No
-| ok
+|style="background: #cbff7B"| ok
 |-
 |colspan="6" |Controls
@@ Line 48: / Line 47: @@
 | 0
 | No
-|  ok
+|style="background: #cbff7B"|  ok
 |-
 |Positive Control
@@ Line 55: / Line 54: @@
 |720 (efficiency 7.2.10^7)
 |No
-|OK
+|style="background: #cbff7B"|OK
 |}
   => Need to screen to know which clones we can use for the  of  '''pFlgA promotor cconstruction'''.
 ='''Construction of pFlgA - GFP Generator'''=
@@ Line 80: / Line 80: @@
 |Amp
 |}
 ='''Construction for Synchronization'''=
@@ Line 209: / Line 210: @@
 |18.04
 |XbaI and PstI
+|}
+='''Promoter characterization plasmids'''=
+==Transformation results: ligations from August 21th==
+'''Top 10 cells were used'''
+[[Team:Paris/Notebook/Protocols#Transformation |Protocol]]
+{|border="1" style="text-align: center"
+|'''Ligation name'''
+|'''Vector digestion'''
+|'''Vector description'''
+|'''Insert digestion'''
+|'''Insert description'''
+|'''Product description'''
+|'''Antibiotic'''
+|'''Number of colonies'''
+|-
+|L155
+|D164
+|J23101 promoter
+|D163
+|gfp generator
+|J23101 promoter-gfp generator
+|Amp
+|0
+|-
+|L156
+|D161
+|pTet promoter
+|D163
+|gfp generator
+|pTet promoter-gfp generator
+|Kana
+|0
+|-
+|Control L156
+|D161
+|
+|none
+|
+|Vector autoligation control
+|Kana
+|1
+|-
+|L157
+|D125.2
+|B0015
+|D162
+|tetR
+|tetR-B0015
+|Kana
+|1
+|-
+|Control L157
+|D125.2
+|
+|none
+|
+|Vector autoligation control
+|Kana
+|0
+|-
+|L166
+|D185
+|RBS B0032
+|D182
+|tetR
+|RBS B0032 - tetR
+|Amp
+|68
+|-
+|Control L166
+|D185
+|
+|none
+|
+|Vector autoligation control
+|Amp
+|49
+|-
+|L167
+|D181
+|pTet
+|D184
+|gfp generator
+|gfp generator - pTet
+|Amp
+|1
 |}

Team:Paris/August 23

From 2008.igem.org

Latest revision as of 14:47, 6 September 2008

Contents

Construction for FIFO

Results of the transformation we did Yesterday

Construction of pFlgA - GFP Generator

Transformation of the ligations we did yesterday

Construction for Synchronization

Results of the transformation we did yesterday

Number of colonies

Digestion

Promoter characterization plasmids

Transformation results: ligations from August 21th