Team:Paris/July 25

(Difference between revisions)

Revision as of 12:18, 28 July 2008

Use of Promega's protocol for the extraction of: gel n°1 --> 4 : (D100 --> D110 cl-1 ES))
Use of Qiagen's protocol for the extraction of: gel n°5 --> 8 : (D110 cl-2 ES --> D120))

Test of the succeed of the extraction by electrophoresis on 2µl of the parts extracted.

conditions: 2µl of the DNA extracted 98µl of pure water

Reading against the adaptated blank (2µl of the elution's buffer / 98µl of pure water)

D100 --> D110 cl-1 ES : Absorbance ~20-50µg/ml ; DO 260/280 = 1,5 ; DO 260/230 = 0,0-0.20 D110 cl-2 ES --> D120 : Absorbance ~0-10µg/ml

to check for the samples from Qiagen's protocol, if the absence of detection of absorbance, is due to a problem of reading or a problem during the extraction, we realise an electrophoresis.

==> conclusion : we don't succeed to detect DNA by spectrophometry or electrophoresis for the samples produced by Qiagen's protocol.

==> we decide to repeat all the samples from the beginning, so we culture O/N at 37°c all the strains usefull for the experiments

Name	Biobrick	Description
MP100	B0034	Strongest RBS (Efficiency = 1)
MP116	J23100	Strong constitutive promoter in J61002
MP120	B0030	Strong RBS (Efficiency = 0,6)
MP121	E0422	ECFP (RBS+LVA+Term)
MP122	E0840	gfp tri-part; strong rbs

@@ Line 22: / Line 22: @@
 D100 --> D110 cl-1 ES : Absorbance ~20-50µg/ml ;  DO 260/280 = 1,5 ;  DO 260/230 = 0,0-0.20
 D110 cl-2 ES --> D120 : Absorbance ~0-10µg/ml
+=== Determination of DNA concentration by electrophoresis ===
 * to check for the samples from Qiagen's protocol, if the absence of detection of absorbance, is due to a problem of reading or a problem during the extraction, we realise an electrophoresis.
@@ Line 30: / Line 34: @@
 ==> we decide to repeat all the samples from the beginning, so we culture O/N at 37°c all the strains usefull for the experiments
+== Culture ==
 == MiniPreps ==