Revision as of 18:38, 16 September 2008

Construction of rbs-TetR-mRFP-LVA-tripart (L173)

Ligation L173

Sample	positive control pUC19	negative control no DNA	ligation control (without insert)	L173 (3:1 ratio)	L173 (4:1 ratio)
Number of colonies	many	1	0	2	0

PCR screening

PCR screening programm

Well n°	1	2	3	4	5	6	7
Sample	1 kb DNA ladder	positive PCR control	negative PCR control	negative transformation control clone	L173.1	L173.2	100 bp DNA ladder
Expected size					1894 bp
Measured size					1,2 kb	1,2 kb

Results: the clones are not correct.

Digestion n°	DNA substrat	Digestion by
D112	MP106: S03879 (rbs-TetR) in pSB1A2	EcoRI & SpeI

Incubation 2h30 at 37°C and then 20 min at 65°C.
Not purified yet. Put at -20°C.

=>the measurement of the absorbance was so instable, that we have prefered to do it again but we an another thechnik : by analysis on gel.

=>it has been missed to do adaptated control.

@@ Line 98: / Line 98: @@
 *L184 = pFliL - ECFP LVA+
 *L185 = pFliL - ECFP LVA-
+==Measurement of the concentration of D168 purified==
+[[Team:Paris/Notebook/Protocols#Concentration_of_the_Miniprep | Protocol (it's same that for Miniprep)]]
+{|border="1" style="text-align: center"
+|'''Digestion Name'''
+|'''Concentration (µg/mL)'''
+|'''Ratio 260/280'''
+|-
+|D134.2
+|114
+|nd
+|-
+|D134.2
+|84,4
+|nd
+|-
+|D149.2
+|140
+|nd
+|}
+=>the measurement of the absorbance was so instable, that we have prefered to do it again but we an another thechnik : by analysis on gel.
 ==Ligation==
@@ Line 111: / Line 139: @@
 |L183
 |D187
-|2,5
+|
 |D134
 |
@@ Line 117: / Line 145: @@
 |L184
 |D198
-|1,11
+|
 |D149
 |
@@ Line 123: / Line 151: @@
 |L185
 |D199
-|0,65
+|
 |D149
 |