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Notebook

11.11.2011

Investigator: X,Y

Aim: We attempt to get results.

Wichtig ist, dass immer die verwendete Materialien (Plasmide, genomische DNA [aus welchen Stamm], Primer) genau benannt und/oder ggf. irgendwo nummeriert werden. Es sollte alles nachvollziehbar sein, wann ihr mit welchen Proben was gemacht habt.

Auf den folgenden Seiten sind Beispiele, wie wir uns das Notebook vom Aufbau und Detailgrad vorstellen.

17.04.2013

Ligation

Investigator: Franzi, Lucas

Aim: Assemble the Bricks 1, 3, 4, 5, 6, 7 and 8 into the vector pSB1C3.

5 µl vector DNA (pSB1C3)
20 µl insert DNA (1, 3, 4, 5, 6, 7 or 8)
3 µl 10x T4 DNA ligase buffer
2 µl T4 DNA ligase

The samples were incubated for 14 h at 18° C.

Digest

Investigator: Christian, Patrick

Aim: Digest of pSB1C3-J04450 with MluI and HindIII.

4 µl DNA (pSB1C3-J04450)
1 µl MluI
1 µl HindIII
1,5 µl 10x red buffer
1,5 µl 10x orange g loading buffer
6 µl H2O

The samples were incubated for 4 h at 37° C.

Gel electrophoresis

Gel substances

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

Expectations

Lane 1: 5300 kbp
Lane 2: 3300 kbp
Lane 3: 1300 kbp

We don’t receive all expected fragments. The expected fragment in lane 1 is missing.

18.04.2012

Transformation

Investigator: Franzi, Christian

Aim: Transformation of the plasmid DNA pB201-40JO in E. coli for amplification.

The chemo competent E. coli DH5a cells were transformed with pB201-40JO DNA and plated on dYT-Amp-plates.
The plates were incubated over night at 37° C .

PCR

Investigator: Patrick, Lucas

Aim: Receive PvuII point-mutation on colonies 3 and 5 of E. coli pB201-40JO.

Volume	Reagent	Temp (°C)	Time
10 µl	5x Buffer	95	3 min
1,5 µl	Primer fwd 13	95	3 sec
1,5 µl	Primer rev 14	58	30 sec	x17
1 µl	Template	72	1 min
36 µl	H2O	7 min	3 min
1 µl Phusion	Phusion Polymerase	4	Hold

Gel electrophoresis

Gel substances

1% Agarose gel
10 µl RedSafe in 50 ml gel
x µl Hyper Ladder

Expectations

Lane 1: 5300 kbp
Lane 2: 3300 kbp
Lane 3: 1300 kbp

We don’t receive all expected fragments. The expected fragment in lane 1 is missing.

Digest

Investigator: Dominik

Aim: Digest of pSB1C3-iBB4+iBB11+iBB9, pSB1C3-iBB4+iBB12+iBB9, pSB1C3-iBB6315 and pSB1A3.

1000 ng Plasmid (pSB1C3-iBB4+iBB11+iBB9, pSB1C3-iBB4+iBB12+iBB9)
0.5 µl EcoRI
0.5 µl SpeI
2 µl CutSmart
ad 20 µl ddH2O

1000 ng Plasmid (pSB1C3-iBB6315)
0.5 µl XbaI
0.5 µl PstI
2 µl CutSmart
ad 20 µl ddH2O

1000 ng Plasmid (pSB1A3)
0.5 µl EcoRI
0.5 µl PstI
2 µl CutSmart
ad 20 µl ddH2O

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

Gel electrophoresis

Gel substances

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

Expactations

Lane 1: 5300 kbp
Lane 2: 3300 kbp
Lane 3: 1300 kbp

All expected fragments were present. The relevant fragments were cut from the gel and then purified via “Qiagen Gel Extraction Kit” (Qiagen, Düsseldorf).

Inoculation

Investigator: Dominik

Aim: inoculation of colonies for plasmid preparation

4 colonies of pSB1A3-iBB395146 and 4 colonies of pSB1A3-iBB496315 were inoculated in 5 ml LB medium containing ampicillin.

Sequencing

Investigator: Dominik

Aim: Complete sequencing of pSB1A3-iBB496315.

8 new sequencing samples were sent out.

Competent cells

Investigator: Dominik

Aim: Overnight culture for making new aliquots of competent cells.

For making new aliquots of E. coli DH5α cells 50 ml LB medium were inoculated with 500 µl of an E. coli DH5α culture.

Miniprep

Investigator: Dominik

Aim: preparation of the plasmids pSB1A3-iBB10+iBB9, pSB1A3-iBB11+iBB9, pSB1A3-iBB12+iBB9 and pSB1A3-iBB13+iBB9.

The plasmids were isolated with the “QIAprep Spin Miniprep Kit” (Qiagen, Düsseldorf) according to the producer instructions.

Team:Marburg/Notebook:Template

From 2013.igem.org

Notebook

11.11.2011

17.04.2013

18.04.2012