Team:Paris/July 25

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Latest revision as of 15:32, 31 July 2008

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DNA Extraction

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))

Analysis of the extraction success by electrophoresis on 2µl of the parts extracted.

Determination of DNA concentration by spectrophotometry

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)

Results :

-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.

==> 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

Culture

in 10ml LB with adaptated antibiotics, all the Biobricks used before (MP100 --> MP122)

will be use to do minipreps

MiniPreps

Use of Promega's protocol on all the clones cultivated on the 24th.
Preparation of 50µl of minipreps in simple.

list of Minipreps

Name	Biobrick	Description
MP100	[http://partsregistry.org/Part:BBa_B0034 B0034]	Strongest RBS (Efficiency = 1)
MP116	[http://partsregistry.org/Part:BBa_J23100 J23100]	Strong constitutive promoter in J61002
MP120	[http://partsregistry.org/Part:BBa_B0030 B0030]	Strong RBS (Efficiency = 0,6)
MP121	[http://partsregistry.org/Part:BBa_E0422 E0422]	ECFP (RBS+LVA+Term)
MP122	[http://partsregistry.org/Part:BBa_E0840 E0840]	gfp tri-part; strong rbs

@@ Line 2: / Line 2: @@
-== Extraction of the DNA  ==
+== DNA Extraction ==
 * 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.
+* Analysis of the extraction success by electrophoresis on 2µl of the parts extracted.
+=== Determination of DNA concentration by spectrophotometry ===
+'''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)
+'''Results :'''
+-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 14: / Line 40: @@
 ==> 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 ==
+in 10ml LB with adaptated antibiotics, all the Biobricks used before (MP100 --> MP122)
+* will be use to do minipreps
 == MiniPreps ==
@@ Line 49: / Line 82: @@
 |align="center"|[http://partsregistry.org/Part:BBa_E0840 E0840]
 |align="center"|gfp tri-part; strong rbs
-|
 |}