Team:Paris/August 15

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Revision as of 16:16, 15 August 2008

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Contents

1 Transformation of the ligations we did yesterday
2 Digestion
- 2.1 Measurement of concentration of minipreps
- 2.2 Digestion
3 Analysis of yesterday PCR screening
4 Starting the construction of the Promoter characterization plasmid
- 4.1 Digestion
  - 4.1.1 Measurement of concentration of minipreps
  - 4.1.2 Digestion
- 4.2 Analysis of yesterday PCR screening

Transformation of the ligations we did yesterday

We transformed L 143, L 144 and the negative controls T1 and T2, using Invitrogen's TOP10 chemically competent cells
standard protocol.

Digestion

Measurement of concentration of minipreps

standard protocol

Digestion	Miniprep used	Concentration (µg/mL)	ratio 260/280
D146	MP148.2	123	1.58
D147	MP153.3	113	1.68

Digestion

Protocol Digestion

Analysis of yesterday PCR screening

Starting the construction of the Promoter characterization plasmid

Digestion

Measurement of concentration of minipreps

standard protocol

Plasmid	Miniprep	Concentration (µg/mL)	ratio 260/280
MP3	3	152	1.43
MP3	4	775	1.21
MP101	1	317	1.66
MP101	2	389	1.36
MP101	4	209	1.76
MP104	1	173	1.32
MP104	3	43	1.85
MP104	4	52	1.66
MP114	1	173	1.75
MP114	2	263	1.43
MP143	1	133	1.55
MP143	2	132	1.70

Digestion

Protocol Digestion

Plasmid	Description	Miniprep used	Enzymes
MP3	B0015 (double terminator B0010-B0012)	4	EcoRI and XbaI
MP114	TetR	1	EcoRI and SpeI
MP104	PTet (Tet promoter)	1	SpeI and PstI
MP101	promoter J23101	1	SpeI and PstI
MP143	gfp generator	2	SpeI and PstI

Analysis of yesterday PCR screening

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