From 2013.igem.org

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Revision as of 13:35, 3 October 2013

Notebook: March

20.03.2013

Transformation

Investigator: Christian

Aim: Preparation of BioBrick-templates → Transformation into E. coli DH5α.

Transformation of 1 µl pPha-NR, 1 µl pPha-T1 and 1 µl pCAT (diluted 1:3 with H2O) in E. coli DH5α (30 min ice, 90 sec 42°C, 1 min ice, 45 min 37°C + 1 ml LB), plated on LB_amp, oN 37°C.

21.03.2013

Inoculation

Investigator: Christian

Aim: Preparation of BioBrick-templates → Inoculation of transformants for miniprep.

2 colonies of pPha-NR and pPha-T1 inoculated in 5 ml LB_amp, oN 37°C.

pCAT is a Cosmid, transformation failed.

22.03.2013

Miniprep

Investigator: Christian

Aim: Preparation of BioBrick-templates → Miniprep of the template-plasmids.

Miniprep of the liquid cultures (“QIAprep Spin Miniprep Kit” (Qiagen, Düsseldorf)), eluted in 25 µl H2O.

Digest

Investigator: Christian

Aim: Preparation of BioBrick-templates → Control digestion of the template plasmids.

3 µl DNA template
1 µl enzyme 1
1 µl enzyme 2
4 µl buffer 2
31 µl H2O

Samples:

Digestion of pPha-NR with EcoRI and NcoI.

Digestion of pPha-T1 with EcoRI and NdeI.

The samples were incubated for 1 h at 37° C.

Gel electrophoresis

Gel substances

1% Agarose gel
10 µl RedSafe per 50 ml gel
6 µl GeneRuler™ 1kb plus DNA Ladder (Thermo Scientific)
6x loading buffer (for samples)

Expectations

pPha-NR: 2868 bp + 992 bp
pPha-T1: 3554 bp + 541 bp

All positive.

PCR

Investigator: Christian

Aim: Construction of BioBricks → Deletion of restriction sites in iBB3, iBB4 and iBB5 via mutagenesis PCR.

Mutagenesis PCR of Pf_cpB (iBB3), P_NR (iBB4), and T_fcpA (iBB5).

Volume	Reagent	Temp (°C)	Time
1 µl	Phusion Polymerase	95	3 min
1 µl	Primer fw (100pmol/µl)	95	30 sec
1 µl	Primer rv (100pmol/µl)	65	45 sec	x19
1 µl	Template pPha-NR (diluted 1:100)	72	4:10 min
1 µl	dNTPs	72	6 min
5 µl	10x buffer	4	Hold
35 µl	ddH20

Gel electrophoresis

Gel substances

1% Agarose gel
10 µl RedSafe in 50 ml gel
6 µl GeneRuler™ 1kb plus DNA Ladder (Thermo Scientific)
6x loading buffer (for samples)

Digest

Investigator: Christian

Aim: Construction of BioBricks → Digestion of the template plasmid.

Digestion of the template with 1 µl DppI.

Gel electrophoresis

Gel substances

1% Agarose gel
10 µl RedSafe per 50 ml gel
6 µl GeneRuler™ 1kb plus DNA Ladder (Thermo Scientific)
6x loading buffer (for samples)

Transformation

Investigator: Christian

Aim: Construction of BioBricks → Transformation of mutagenised plasmids.

Transformation of 1 µl PCR-product into E. coli DH5α (30 min ice, 60 sec 42°C, 1 min ice, 30 min 37°C + 1 ml LB), plated on LB_amp, oN 37°C.

26.03.2013

Inoculation

Investigator: Christian

Aim: Construction of BioBricks → Inoculation of transformants for miniprep.

Transformation of iBB5 failed, new mutagenesis primers ordered.

3 colonies of iBB3 and iBB4 inoculated in 5 ml LB_amp, oN 37°C.

Inoculation

Investigator: Christian

Aim: Production of chemo-competent E. coli cells → Inoculation of E. coli DH5α pre-culture.

Inoculation of Ca-competent E. coli DH5α in 2x5 ml LB, oN 37°C.

Inoculation

Investigator: Christian

Aim: Preparation of BioBrick-templates → Inoculation for glycerol stocks.

PPha-NR and pPha-T1 were inoculated in 5 ml LB, oN 37°C (for glycerol stocks).

27.03.2013

Miniprep

Investigator: Christian

Aim: Construction of BioBricks → Miniprep of transformants.

Miniprep of of iBB3 and iBB4 (“QIAprep Spin Miniprep Kit” (Qiagen, Düsseldorf)), eluted in 30 µl H2O.

Inoculation

Investigator: Christian

Aim: Production of chemo-competent E. coli cells → Inoculation of E. coli DH5α pre-culture.

3 ml E. coli DH5α pre-culture inoculated in 100 ml LB.

PCR

Investigator: Christian

Aim: Construction of BioBricks → Amplification of iBB2 via PCR.

PCR on CAT-cassette (iBB2):

Volume	Reagent	Temp (°C)	Time
1 µl	Q5 Polymerase	95	3 min
1 µl	Primer fw (1pmol/µl)	95	30 sec
1 µl	Primer rv (1pmol/µl)	65	30 sec	x26
1 µl	Template	72	1 min
1 µl	dNTPs	72	7 min
10 µl	5x Q5-buffer	4	Hold
36 µl	ddH20

Gel electrophoresis

Gel substances

1% Agarose gel
10 µl RedSafe in 50 ml gel
6 µl GeneRuler™ 1kb plus DNA Ladder (Thermo Scientific)
6x loading buffer (for samples)

The relevant fragments were cut from the gel and then purified via “Qiagen Gel Extraction Kit” (Qiagen, Düsseldorf). Elution into 20 µl elution buffer.

Transformation

Investigator: Christian

Aim: Production of chemo-competent E. coli → Control of cells.

Competent cells harvested and frozen.

Controlled with several Transformations:

on LB
on LB_amp
on LB_amp with 1 µl pPha-T1
cells from AG Bange as control

30 min ice, 60 sec 42°C, 60 sec ice, 60 min 37°C + 1 ml LB; plated, oN 37°C.

Digest

Investigator: Christian

Aim: Construction of BioBricks → Control digestion of mutations.

3 µl DNA template
1 µl enzyme 1
1 µl enzyme 2
1 µl buffer
5 µl H2O

Samples:

Digestion of iBB3 with PvuII.

Digestion of IBB4 with PstI.

The samples were incubated for 1 h at 37° C.

Gel electrophoresis

Gel substances

1% Agarose gel
10 µl RedSafe per 50 ml gel
6 µl GeneRuler™ 1kb plus DNA Ladder (Thermo Scientific)
6x loading buffer (for samples)

Expectations

iBB3: no cut, vector in different forms
iBB4: 1 cut, linearized plasmid

All positive.

28.03.2013

Sequencing

Investigator: Christian

Aim: Construction of BioBricks → Sequencing.

IBB3 and iBB4 with point mutations prepared for sequencing:

AGBOOOK 128: iBB4 1
AGBOOOK 129: iBB4 2
AGBOOOK 130: iBB4 3
AGBOOOK 131: iBB3 1
AGBOOOK 132: iBB3 2
AGBOOOK 133: iBB3 3

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Team:Marburg/Notebook:March

From 2013.igem.org

Revision as of 13:35, 3 October 2013

Notebook: March

20.03.2013

21.03.2013

22.03.2013

26.03.2013

27.03.2013

28.03.2013