Team:Paris Saclay/Notebook/July/12

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Transformation

We suspended the DNA with water from iGEM plate and performed several transformation.

BBa_I732019: LacZ+RBS+terminator into plasmid BBa_I732950(ampicillin resitant).
BBa_B0015: 2 terminators BBa_B0010+BBa_B0012(4F plate 3 kit 2013) into plasmid PSB1C3.
BBa_B0017: 2 terminators BBa_B0010+BBa_B0010 into plasmid PSB1C3.
Simple terminator BBa_B0010 into plasmid PSB1A2.

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Contents

1 Notebook : July 12
- 1.1 Lab work
  - 1.1.1 'A - Aerobic/Anaerobic regulation system
  - 1.1.2 B - PCB sensor system

Notebook : July 12

Lab work

'A - Aerobic/Anaerobic regulation system

Objective : obtaining Bba_K1155003, Bba_K1155007

1 -Transformation of Bba_I732019, Bba_B0015, Bba_B0017, Bba_B0010

Zhou

Transformation of 07/10/13 of Bba_B0010 and Bba_I732019 didn't works. We will do it again.

Protocol : Bacterial transformation

1 -Design of RBS-AmilCP oligos

Abdou, Anaïs

We used software gene manager to find the correct oligopeptides for amplification of RBS-Amil CP.

B - PCB sensor system

Objective : obtaining Bba_K1155001, Bba_K1155002 and BphR2

1 - Stock of clones 5, 6, 7, 8 for BphA1, clones 5, 6 for BphR1 and clones 3, 4 for BphR2

Zhou

Used quantities :

Glycerol 85% : 425
Culture : 1µL

2 - Extraction of clones 5, 6, 7, 8 for BphA1, clones 5, 6 for BphR1 and clones 3, 4 for BphR2 from DH5α

Abdou, Sheng

Protocol : High copy plamid extraction

3 - Streak of BphA1 and BphR2

Anaïs

We strek 25 colonies of 07/10/13 transformation of BphA1 and BphR2 in new solid culture.

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