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Latest revision as of 18:08, 4 September 2008

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Construction of OmpR+RBS and EnvZ+RBS: Ligations

Cleaning of the DNA after the digestion

We used the QIAcube to wash the DNA, following the standard protocol.

Measure of DNA concentration of the digestion products

We used the biophotometer.
Settings:

10 µL of template DNA in 50 µL of pure water
Blank : 10 µL of EB buffer in 50 µL of water.

Digestion name	What's in ?	Enzymes	DNA C° (ng/µL)
D 158	OmpR*	XbaI-PstI	12
D 159	EnvZ*	XbaI-PstI	7
D 102	B0034	SpeI-PstI	16

List of ligations

We ligated the DNA following the standard protocol.
T5 is the autoligation control for L148 and L149.

Ligation name	Insert name	V_insert µL	Vector name	V_Vector µL
L 148 (Amp)	D 158 (OmpR*)	4	D 102 (B0034)	3
L 149 (Amp)	D 159 (EnvZ)	7	D 102 (B0034)	3

Creation of a registry of pFliL, pFlhDC, and FlhDC

Analysis of the transformation we did yesterday

L143, L144, T1 and T2 showed no colonies. The positive control with pUC19 worked well.
We suppose that the ligation did not work. We will do it again today.

Cleaning of the DNA after the digestion

We used the QIAcube to wash the DNA, following the standard protocol.

Measure of DNA concentration of the digestion products

We used the biophotometer.
Settings:

10 µL of template DNA in 50 µL of pure water
Blank : 10 µL of EB buffer in 50 µL of water.

Digestion name	What's in ?	DNA concentration (ng/µL)
D 149	pfliL	2
D 150	pfliL	3
D 151	pSB3K3	12
D 152	pSB3K3	20
D 153	gene flhDC	7
D 154	gene flhDC	12
D 155	pflhDC	16
D 136	j61002	12
D 145	pSB1A2	21

List of ligations

We ligated the DNA following the standard protocol.
T1, T2, T3 and T4 are the autoligation controls for L 143, L144, L145 and L147

Ligation name	Insert name	V_insert µL	Vector name	V_Vector µL
L 143 (Kan)	D 149 (pfliL)	8	D 137 (pSB3K3)	4
L 144 (Kan)	D 150 (pfliL)	5	D 152 (pSB3K3)	2.5
L 145 (Amp)	D 153 (g flhDC)	10	D 145 (pSB1A2)	2.5
L 146 (Amp)	D 154 (g flhDC)	5	D 145 (pSB1A2)	2.5
L 147 (Amp)	D 155 (p flhDC)	1	D 136 (J61002)	4

Construction of pLas-TetR-GFP tripart & rbs-LasR-dble ter

Transformation

Transformation protocol

Name	Description	Antibio
Ligations
L150	D105(BV) - D146(BI) pLas - strongest rbs-TetR-GFP tripart	Amp
L151	D147(FI) - D125 (FV) strongest rbs-LasR activator with LVA - Double terminator	Kan
Controls
C1	D105	Amp
C2	D125	Kan
Positive Control	pUC19	Amp

Digestion check from yesterday

Protocol Digestion

Digestion name	Plasmid	Description	Miniprep used	Expected size	Measured size
	MP3	B0015 (double terminator B0010-B0012) - FV	4	No bands
D164	MP101	promoter J23101 - BV	1
D161	MP104	PTet (Tet promoter) - FI	1
D162	MP114	TetR - BI	1
D163	MP143	gfp generator - BV	2

@@ Line 1: / Line 1: @@
 {{Paris/Calendar_Links|August 15|August 17}}
-==''' Analysis of the transformation we did [[Team:Paris/August_15#Transformation_of_the_ligations_we_did__yesterday| yesterday]]'''==
+=Construction of OmpR*+RBS and EnvZ*+RBS: '''Ligations=
-L143, L144, T1 and T2 showed no colonies. The positive control with pUC19 worked well.
-<br>We suppose that the ligation did not work. We will do it again today.
-==Construction of OmpR*+RBS and EnvZ*+RBS: '''Ligations'''==
 ==='''Cleaning of the DNA after the digestion'''===
 We used the QIAcube to wash the DNA, following the [[Team:Paris/Notebook/Protocols#Purification_.28Kit_Promega.29|standard protocol.]]
@@ Line 14: / Line 10: @@
 *10 µL of template DNA in 50 µL of pure water
 *Blank : 10 µL of EB buffer in 50 µL of water.
-{| Border="2"
+{||- style="text-align: center;" border="1"
 |align="center"|'''Digestion name'''
 |align="center"|'''What's in ?'''
-|align="center"|'''DNA concentration (ng/µL)'''
+|'''Enzymes'''
+|align="center"|'''DNA C° (ng/µL)'''
 |-
 |align="center"|D 158
 |align="center"| OmpR*
+|XbaI-PstI
 |align="center"| 12
 |-
 |align="center"|D 159
 |align="center"| EnvZ*
+|XbaI-PstI
 |align="center"| 7
 |-
 |align="center"|D 102
 |align="center"|B0034
+|SpeI-PstI
 |align="center"| 16
 |}
@@ Line 57: / Line 57: @@
 |}
-=='''Ligation'''==
-==='''Cleaning of the DNA after the digestion'''===
+=Creation of a registry of pFliL, pFlhDC, and ''FlhDC''=
+== Analysis of the transformation we did [[Team:Paris/August_15#Transformation_of_the_ligations_we_did__yesterday| yesterday]]==
+L143, L144, T1 and T2 showed no colonies. The positive control with pUC19 worked well.
+<br>We suppose that the ligation did not work. We will do it again today.
+==Cleaning of the DNA after the digestion==
 We used the QIAcube to wash the DNA, following the [[Team:Paris/Notebook/Protocols#Purification_.28Kit_Promega.29|standard protocol.]]
-==='''Measure of DNA concentration of the digestion products'''===
+==Measure of DNA concentration of the digestion products==
 We used the biophotometer.<br>
 '''Settings:'''
@@ Line 108: / Line 114: @@
 |}
-==='''List of ligations'''===
+==List of ligations==
 * We ligated the DNA following the [[Team:Paris/Notebook/Protocols#Ligation|standard protocol]].
@@ Line 185: / Line 191: @@
 |Amp
 |}
@@ Line 197: / Line 202: @@
 |Description
 |Miniprep used
-|Comments
+|Expected size
+|Measured size
 |-
 |
@@ Line 209: / Line 215: @@
 |promoter J23101 - BV
 |1
-|Good expected sized bands
+|
+|style="background: #cbff7B"|
 |-
 |D161
@@ Line 215: / Line 222: @@
 |PTet (Tet promoter) - FI
 |1
-|Good expected sized band
+|
+|style="background: #cbff7B"|
 |-
 |D162
@@ Line 221: / Line 229: @@
 |TetR - BI
 |1
-|Good expected sized bands
+|
+|style="background: #cbff7B"|
 |-
 |D163
@@ Line 227: / Line 236: @@
 |gfp generator - BV
 |2
-|Good expected sized bands
+|
+|style="background: #cbff7B"|
 |}

Team:Paris/August 16

From 2008.igem.org

Latest revision as of 18:08, 4 September 2008

Contents

Construction of OmpR+RBS and EnvZ+RBS: Ligations

Cleaning of the DNA after the digestion

Measure of DNA concentration of the digestion products

List of ligations

Creation of a registry of pFliL, pFlhDC, and FlhDC

Analysis of the transformation we did yesterday

Cleaning of the DNA after the digestion

Measure of DNA concentration of the digestion products

List of ligations

Construction of pLas-TetR-GFP tripart & rbs-LasR-dble ter

Transformation

Digestion check from yesterday

Team:Paris/August 16

From 2008.igem.org

Latest revision as of 18:08, 4 September 2008

Contents

Construction of OmpR*+RBS and EnvZ*+RBS: Ligations

Cleaning of the DNA after the digestion

Measure of DNA concentration of the digestion products

List of ligations

Creation of a registry of pFliL, pFlhDC, and FlhDC

Analysis of the transformation we did yesterday

Cleaning of the DNA after the digestion

Measure of DNA concentration of the digestion products

List of ligations

Construction of pLas-TetR-GFP tripart & rbs-LasR-dble ter

Transformation

Digestion check from yesterday

Construction of OmpR+RBS and EnvZ+RBS: Ligations