Precipitator
Miniprep
Qiagen Kit
Name:
Sophie
| Date:
22.07
|
Continue from Experiment (Date) Trafo 20.07 Ruediger
(Name)
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Project Name:
GFPpbd
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Documentation:
Why are you doing this experiment? Name the parts which you extract.
1abc: S39+M14+P28+P18
2abc: S39+M14+P28+P19
3abc: S39+M14+P28+P20
4abc: S43+M14+P28+P18
5abc: S43+M14+P28+P19
6abc: S43+M14+P28+P20
all CM resistance ps131C3
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Describe your results and mistakes and measure the DNA concentration with the Nanodrop and note the results.
Mistakes: some lids broke
nanodrop labeling partly confused
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Sample ID
| Nucleic Acid Conc.
| Unit
| 260/280
| 260/230
|
1a
| 60.6
| ng/µl
| 1.85
| 1.75
|
1b
| 102.8
| ng/µl
| 1.66
| 0.96
|
1c
| 41.5
| ng/µl
| 1.74
| 1.63
|
1d
| 85.5
| ng/µl
| 1.58
| 1.09
|
2a
| 72.4
| ng/µl
| 1.62
| 1.04
|
2b
| 9.7
| ng/µl
| 0.86
| 0.34
|
2c
| 116.8
| ng/µl
| 1.64
| 0.9
|
2d
| 38.5
| ng/µl
| 1.56
| 0.95
|
3a
| 86.5
| ng/µl
| 1.56
| 0.75
|
3b
| 77.9
| ng/µl
| 1.57
| 0.89
|
3c
| 94
| ng/µl
| 1.66
| 1.07
|
3d
| 88.1
| ng/µl
| 1.64
| 0.95
|
4a
| 91.3
| ng/µl
| 1.64
| 0.91
|
4b
| 93.4
| ng/µl
| 1.67
| 1.09
|
4c
| 111.5
| ng/µl
| 1.7
| 1.15
|
4d
| 71.5
| ng/µl
| 1.86
| 1.95
|
5a
| 73.2
| ng/µl
| 1.81
| 1.75
|
5b
| 172.3
| ng/µl
| 1.79
| 2.01
|
5c
| 53
| ng/µl
| 1.61
| 1.98
|
5d
| 97
| ng/µl
| 1.72
| 1.43
|
6a
| 92
| ng/µl
| 1.7
| 1.27
|
6b
| 92.8
| ng/µl
| 1.62
| 1.05
|
6c
| 81.3
| ng/µl
| 1.66
| 1.14
|
6d
| 106.8
| ng/µl
| 1.73
| 1.26
|
Testdigest
Name:
Ruediger
| Date:
21.07
|
Continue from Experiment (Date)
Miniprep Sophie (Name)
|
Project Name: GFPPbd
|
For one reaction you need: For Mastermix: Number of samples+2extra
4μl
| H2O
| 104
|
|
1μl
| Buffer, NEB4
| 26
|
|
1μl
| BSA (10x)
| 26
|
|
0,5 μl
| Enzym 1
|
|
|
0,5 μl
| Enzym 2
|
|
|
3 μl
| DNA
|
|
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DNA from todays Miniprep. See labeling there.
10 μl total volume
Give 3 μl of DNA in an eppi and add 7μl of the mastermix.
Incubate for about 1h at 37°C.
Add 1 μl Loading dye buffer and load the gel.
Take a picture of the gel, print picture and label the lanes!
Meeting
attendants: Jakob, Julia, Manuel, Ruediger, Sandra, Sophie, Theo (later), Tobi
time: 9:00 - 10:30
green light receptor
already done:
- CcaS was amplified again from the genomic DNA
To-do:
- 3-A-Assembly of CcaR into an empty vector with a medium promotor
- 3-A-Assembly of CcaS into an empty vector with a weak promotor
- 3-A-Assembly of CcaR and CcaS to get the final construct
blue light receptor
already done:
- Primer-Design for the Gibson-Assembly
- growth medium without tryptophane is already ordered
To-do:
red light receptor
already done:
- one positive colony from the 3-A of ho1 and the terminator
- no positive colony from the 3-A of pcyA and the terminator
- the PCR to amplify cph8 didn't give a product, we asked the team from Mexico to send us the cph8
- the team from Upsala (Sweden) has succeeded in amplifying the cph8 (according to their notebook)
To-do:
- 3-A-Assembly of the ho1-term with a mediumPromotor-mediumRBS
Lysis cassette
already done:
- the quick change didn't work the first time, we should repeat this
- possible alternative to express the lysis cassette could be: temperature regulated RNA
To-do:
Precipitator
already done:
- the GFP-PBD was cloned (colonies showed up)
To-do:
- test digest and sequencing of the GFP-PBD (first have a look if you see the GFP fluorescence)
- possible test of the PBD: grow the E. coli, lyse them, put the lysate into a plate (96 well?), wash the wells to get rid of the other proteins, measure the GFP fluorescence with a plate reader
- microscope the E. coli cells
other suff
- think about possible give-aways for the sponsoring video
- jacob will create a Youtube account and upload the sponsoring video
- meeting for the wiki takeover: wednesday 9:00 am (new time: 12:15)
- modelling should be started now, either Ni-binding and release or GFP-PBD binding and release, Ruediger will do this
Lysis cassette
Quickchange PCR
Name: Theo
| Date: 22.07.2011
|
Project Name: Quickchange V.3 with correct lysis template
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PCR-Mixture for one Reaction:
For a 50 µl reaction use
32,5µl
| H20
| Name
|
10µl
| 6x Phusion HF Buffer
|
|
2.5µl
| Primer fw
| P29 (1:10)
|
2.5µl
| Primer dw
| P30 (1:10)
|
1µl
| dNTPs
|
|
1µl
| DNA-Template
| S11 (->diluted to 10ng/µl)
|
0.5 µl
| Phusion (add in the end)
|
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What program do you use?
| 95°C - 15 sec
|
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95°C - 5 min
| 55°C / 66°C - 15 sec
| 72°C -5 min
| 4°C - ∞
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| 72°C - 1’ + 2’’
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| 20x
|
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