09.07.2012

Inoculation

E. coli strain C600 Mucts62 in dYT-medium

10.07.2012

Isolation of chromosomal DNA

E. coli strain C600 Mucts62 (lysogenic for temperature sensitive phage Mu cts62)

Inoculation

E. coli strain DH5α and TOP10 in dYT-medium

11.07.2012

Preparation of chemically competent E. coli cells

TOP10

12.07.2012

Transformation

GFP, GFP_fusion, CFP, mRFP, RBS, P108, P100, Plac with E.coli TOP10

16.07.2012

PCR

AmiC (primer: MS1 + MS2)

HU (primer: MS3 + MS4)

GroES (primer: MS5 + MS6)

GixR (primer: MS7 + MS8)

Enhancer (primer: MS9 + MS10)

⇒ template-DNA: chromosomal DNA, denaturation: 30 sec at 95°C; annealing: 30 sec at 60°C; elongation: 30 sec at 72°C; 35 cycles

Inoculation

GFP

GFP_fusion

CFP

mRFP

RBS

P108

LacIQ

P100

17.07.2012

Plasmid preparation

GFP

GFP_fusion

CFP

mRFP

RBS

P108

LacIq

P100

18.07.2012

1% Agarose gel

M:1kb gene ruler plus, 1:enhancer, 2:GroES, 3:AmiC, 4:HU, 5:GixR, 6:GFP, 7:GFP-Fusion, 8:CFP, 9:mRFP, 10:RBS, 11:LacIQ, 12:P108, 13:P100, 14:λ-DNA (PCR 18.07.2012)

DNA Gel extraction

Enhancer

GroES

HU

GixR Hybridization

• 5 µl primer MS7 (100 µM) + 5 µl primer MS8 (100 µM)
  • 5 min 99°C
  • over night, room temperature
  • -80°C

19.07.2012

Fill-in reaction (primer extension)

Enhancer

Restriction

Enhancer (EcoRI/PstI)

PCR

AmiC (primer: MS1 + MS2)

⇒ template-DNA: chromosomal DNA, annealing: 30 sec; 85 °C, elongation: 36 sec; 72 °C, 35 cycles, 1) 2 µl DMSO; 1 µl chrom. DNA | 2) 2 µl DMSO; 5 µl chrom. DNA | 3) without DMSO; 1 µl chrom. DNA | 4) without DMSO; 5 µl chrom. DNA | 5) 2 µl DMSO; without chrom. DNA

Test restriction digest

7) CFP (EcoRI/PstI)

8) GFP (EcoRI/PstI)

9) GFP-fusion (EcoRI/PstI)

10) mRFP (EcoRI/PstI)

⇒ all negative

1% Agarose gel

M:1kb gene ruler plus, 1-5:AmiC PCR conditions (see above), 6-9: control digest (E/P), 6:GFP, 7:GFP-Fusion, 8:CFP, 9:mRFP (PCR 19.07.2012)

Control digest

CFP (EcoRI/PstI)

GFP (EcoRI/PstI)

GFP-fusion (EcoRI/PstI)

mRFP (EcoRI/PstI)

⇒ restriction over night

20.07.2012

1% Agarose gel from the control digest

M:1kb gene ruler plus, 1:GFP, 2: GFP-Fusion, 3: CFP, 4: mRFP (control digest 18.07.2012)

26.07.2012

Restriction

pSB1T3 (XbaI/SpeI and DpnI)

pSB1A3 (XbaI/SpeI and DpnI)

pSB1K3 (XbaI/SpeI and DpnI)

pSB1C3 (XbaI/SpeI and DpnI)

Ligation

GixR + pSB1A3

Enhancer + pSB1K3

cyclisation of pSB1C3, pSB1K3, pSB1A3, pSB1T3 (couldn’t work)

27.07.2012

Our lab-dragon "Hugo" is born

30.07.2012

PCR

CFP (primer: MS16 + MS17) ⇒ template-DNA: [http://partsregistry.org/Part:BBa_E0020 BBa_E0020]

⇒ positive

mRFP (primer: MS14 + MS15) ⇒ template-DNA: [http://partsregistry.org/Part:BBa_E1010 BBa_E1010]

⇒ positive

Gin (primer: MS11 + MS13) ⇒ template-DNA: chromosomal DNA (that was wrong)

RBS-Gin (primer: MS13 + MS12) ⇒ template-DNA: chromosomal DNA (that was wrong)

⇒ annealing: 30 sec; 60 °C, elongation: 40 sec; 72 °C, 35 cycles

Transformation

all vector-backbone-ligations

Enhancer (K3)

GixR (A3)

31.07.2012

Result

transformation

pSB1A3: 3 colonies

pSB1K3: 60 colonies

pSB1C3: 9 colonies

pSB1T3: 0 colonies

Enhancer (K3): 0 colonies

GixR (A3): 0 colonies

1% Agarose gel

M:Marker, 1: Gix, 2-6: AmiC (PCR 16.07.2012)

1% Agarose gel

M:1kb gene ruler plus, 1: AmiC(PCR 16.07.2012)

1% Agarose gel

M:1kb gene ruler plus, 1: RBS-Gin from 30.07, 2:AmiC from 16.07., 3:Gin from 30.07., 4:CFP from 30.07., 5:mRFP from 30.07., 6: control (PCR 30.07.2012)

Resuspension of a biobrick

[http://partsregistry.org/Part:BBa_B0010 BBa_B0010](Terminator)

DNA Gel extraction

CFP

mRFP

PCR

AmiC (primer: MS1 + MS2)

RBS-Gin (primer: MS12 + MS13)

Gin (primer: MS11 + MS13)

⇒ template-DNA: chromosomal DNA, annealing: 30 sec; 55 °C, elongation: 40 sec; 72 °C, 35 cycles

Restriction

pSB1A3 (EcoRI/PstI)

CFP (EcoRI/PstI)

mRFP (EcoRI/PstI)

Transformation

pSB1A3

pSB1C3

pSB1T3

Terminator

GixR

Enhancer

Inoculation

pSB1A3

pSB1C3

pSB1K3

Ligation

pSB1A3 + CFP

pSB1A3 + mRFP

GixR Hybridization

• 5 µl primer MS7 (100 µM) + 5 µl primer MS8 (100 µM)
  • 5 min 99°C
  • over night, room temperature
  • -80°C

DNA Gel extraction

AmiC

Ligation

AmiC + pSV2 (suicide vector)

01.08.2012

Result

transformation

Only BBa_B0010 colonies present

Plasmid preparation

pSB1A3 ⇒ only clone 1, 3 Positive

pSB1C3 ⇒ all negative

pSB1K3 ⇒ all negative

Ligation

GixR hyb. + pJET2_1

⇒ over blunt ends

Restriction

GixR hyb. (EcoRI/PstI)

pSB1C3 (EcoRI/PstI)

1% Agarose gel

M:1kb gene ruler plus, 1: RBS-Gin (+DMSO), 2:RBS-Gin (-DMSO), 3:Gin (+DMSO), 4:Gin (-DMSO), 5: control (PCR 31.07.2012)

1% Agarose gel

M:1kb gene ruler plus, 1: AmiC (+DMSO), 2:AmiC (-DMSO), (PCR 31.07.2012)

DNA Gel extraction

RBS-Gin

Gin

AmiC

Test restriction

pSB1A3 (EcoRI)

Restriction

RBS-Gin (EcoRI/PstI)

Gin (EcoRI/PstI)

AmiC (EcoRI/PstI)

pSB1C3 (EcoRI/PstI)

pSB1K3 (EcoRI/PstI)

pSB1T3 (EcoRI/PstI)

Ligation

cyclisation of pSB1T3

Fill-in reaction (primer extension)

Enhancer

Ligation

Enhancer and GixR in pSV2

Enhancer in pSB1K3

GixR in pSB1C3

1% Agarose gel

M:1kb gene ruler plus, 1-3: pSB1A3, 4-7:pSB1C3, 8-11: pSB1K3 (Control digest 01.08.2012)

pSB1A3 c2

pSB1C3 c4

pSB1K3 c3

Transformation

pSB1A3 religation

CFP in A3

mRFP in A3

AmiC in pJET

GixR in pJET

Enhancer in pJET

GixR in C3

Enhancer in K3

Ligation

AmiC + pSB1T3

RBS-Gin + pSB1K3

Gin + pSB1K3

02.08.2012

Resuspension of a biobrick

pSB3C5

⇒ for ccdB

Plasmid preparation

BBa_B0010 (terminator)

Test restriction

Terminator c1,2,3,4 (EcoRI/PstI)

2% Agarose gel

M:1kb gene ruler plus, 1-4: Terminator, M2:Middle Range gene ruler (Control digest 01.08.2012)

Transformation

pSB1T3 recycled

AmiC in T3

Gin-RBS in K3

Gin in K3

pSB3C5 linear (false)

03.08.2012

Plasmid preparation

Enhancer in pJET

06.08.2012

Resuspension and transformation of a biobrick

BBa_J04450 in pSB1A3

BBa_J04450 in pSB1C3

BBa_J04450 in pSB1K3

BBa_J04450 in pSB1T3

Restriction

GFP-fusion (EcoRI/SpeI)

Terminator (XbaI/PstI)

Promoter BBa_J23100 (EcoRI/SpeI)

Promoter BBa_J23108 (EcoRI/SpeI)

RBS (XbaI/PstI)

Ligation

RBS-Gin in T3

Gin in T3

GFP-fusion (EcoRI/SpeI) + Terminator (XbaI/PstI) in pSB1K3

Promoter BBa_J23108 (EcoRI/SpeI) + RBS (XbaI/PstI) in pSB1K3

Promoter BBa_J23100 (EcoRI/SpeI) + RBS (XbaI/PstI) in pSB1K3

GixR Hybridization

• 1(3) µl primer MS77 (100 µM) + 1(3) µl primer MS8 (100 µM) + T4-Ligasebuffer
  • 5 min 95°C
  • over night, room temperature
  • -80°C

Transformation

GixR in C3

Gin in T3

RBS-Gin in T3

mRFP in A3

CFP in A3

07.08.2012

Transformation

GFP-fusion

CFP

J23108-RBS

J23100-RBS

Plasmid preparation

GixR 1,2,3

Restriction

GixR hyb. 1,2,3 (EcoRI/PstI)

pSB1C3 (EcoRI/PstI)

Ligation

GixR hyb. 1,2,3 in pJET

GixR hyb. 1,2,3 in C3

Transformation

GixR hyb. 1,2,3 in pJET

GixR hyb. 1,2,3 in C3

Test restriction

pSB3C5 (XbaI)

pJET (XbaI)

1% Agarose gel

M:1kb gene ruler plus, 1-4: pSB3C5, 5-8:pSB3C5, 9-12: Enhancer-pJET (Control digest 07.08.2012)

⇒ positive: pSB3C5 3,4,7,8,; Enhancer-pJET 9-12

08.08.2012

Result transformation

GFP-fusion (20 clones)

J23108-RBS (20 clones)

J23100-RBS (20 clones)

GixR hyb. 1,2,3 in pJET (10 clones)

GixR hyb. 1,2,3 in C3 (10 clones)

CFP (5 clones)

Restriktion

Enhancer in pJET (EcoRI/PstI)

pSB1C3 (EcoRI/PstI)

2% Agarose gel

M:1kb gene ruler plus, 1: Enhancer, 2:pSB1C3, (Control digest 08.08.2012)

DNA Gel extraction

Enhancer

pSB1C3

Ligation

Enhancer 1,2 in C3

Transformation

Enhancer 1,2 in C3

C3

mRFP

09.08.2012

Result transformation

GFP-fusion ⇒ positive

J23108-RBS ⇒ positive

J23100-RBS ⇒ positive

CFP ⇒ positive

GixR in C3 c1 ⇒ negative

GixR in C3 c2 ⇒ negative

GixR in C3 c3 ⇒ negative

Plasmid preparation

GFP-fusion

J23108-RBS

J23100-RBS

CFP

Test restriction

GFP-fusion (EcoRI/PstI)

J23108-RBS (EcoRI)

J23100-RBS (EcoRI)

CFP (EcoRI/PstI)

1% Agarose gel

M:1kb gene ruler plus, 1-18: GFP-Fusion - Terminator, (Control digest 09.08.2012)

1% Agarose gel

M:1kb gene ruler plus, 1-18: P108-RBS, (Control digest 09.08.2012)

1% Agarose gel

M:1kb gene ruler plus, 1-18: P100-RBS, (Control digest 09.08.2012)

1% Agarose gel

M:1kb gene ruler plus, 1-2: GFP-Fusion - Terminator, 3-4: P108-RBS, 5-6: P100-RBS, 7-11: CFP (Control digest 09.08.2012)

Inoculation

GixR in C3

Gin in T3

Gin-RBS in T3

pSB1C3

Enhancer in C3

mRFP in A3

13.08.12

PCR

GroES (primer: MS5 + MS6b)

HU (primer: MS3 + MS4b)

⇒ with and without DMSO, template-DNA: chromosomal DNA, annealing: 30 sec; 60 °C, elongation: 40 sec; 72 °C, 35 cycles

1% Agarose gel

M:1kb gene ruler plus, 1: HU (+DMSO), 2: HU (-DMSO), 3: GroES (+DMSO), 4: GroES (-DMSO), (PCR 13.08.2012)

Transformation

LacIQ (BBa_I14032)

14.08.12

Restriction

pSB1K3 (EcoRI/PstI)

Enhancer 3,4 (EcoRI/ PstI)

GFP-fusion (EcoRI/SpeI)

Terminator (XbaI/PstI)

Test restriction

RBS-Gin in T3 (EcoRI/ PstI)

Ligation

GFP-fusion (EcoRI/SpeI) + Terminator (XbaI/PstI) in pSB1K3 (EcoRI/PstI)

Promotor J23108 (EcoRI/SpeI) + RBS (XbaI/PstI) in pSB1K3 (EcoRI/PstI)

Enhancer 3,4 (EcoRI/ PstI) + pSB1K3 (EcoRI/PstI)

Transformation

GFP-fusion-Terminator in pSB1K3

Promotor-RBS in pSB1K3

Enhancer 3 in pSB1K3

Enhancer 4 in pSB1K3

GixR in pJET

15.08.2012

PCR

GroES (primer: MS5 + MS6b)

HU (primer: MS3 + MS4b)

⇒ with and without DMSO, template-DNA: chromosomal DNA, annealing: 30 sec; 55 °C, elongation: 30 sec; 72 °C, 35 cycles

1% Agarose gel

M:1kb gene ruler plus, 1: HU (-DMSO), 2: HU (+DMSO), 3: GroES (-DMSO), 4: GroES (+DMSO), (PCR 15.08.2012)

DNA Gel extraction

HU 1,2

Resuspension of a biobrick

BBa_J04450 in pSB1A3

BBa_J04450 in pSB1T3

BBa_J04450 in pSB1C3

BBa_J04450 in pSB1K3

Transformation

BBa_J04450 in pSB1A3

BBa_J04450 in pSB1T3

BBa_J04450 in pSB1C3

BBa_J04450 in pSB1K3

Test restriction

pSB1T3 (EcoRI/PstI and DpnI)

pSB1K3 (EcoRI/PstI and DpnI)

pSB1C3 (EcoRI/PstI and DpnI)

pSB1A3 (EcoRI/PstI and DpnI)

16.08.2012

PCR

GroES (primer: MS5 + MS6b)

⇒ with and without DMSO, template-DNA: chromosomal DNA, annealing: 30 sec; 55 °C, elongation: 30 sec; 72 °C , 35 cycles

1% Agarose gel

M:1kb gene ruler plus, 1: GroES (-DMSO), 2: GroES (+DMSO), (PCR 16.08.2012)

Plasmid preparation

P-RBS

Test restriction

P-RBS (EcoRI/PstI)

1% Agarose gel

M:1kb gene ruler plus, 1: control, 2: P108-RBS, (control digest 16.08.2012)

Restriction

Enhancer 3,4 (EcoRI/ PstI)

HU (EcoRI/ PstI)

AmiC (EcoRI/ PstI)

Promoter, GFP (EcoRI/SpeI)

RBS; Terminator (XbaI/PstI)

Ligation

HU, AmiC in pSB1A3

Enhancer 3,4 in pSB1K3

P-RBS in pSB1K3

GFP fusion-Terminator in pSB1K3

DNA Gel extraction

GroES 1, P-RBS

Transformation

AmiC

HU

Enhancer 3,4, 3 alt,4 alt

Inoculation

BBa_J04450 in pSB1A3

BBa_J04450 in pSB1T3

BBa_J04450 in pSB1C3

BBa_J04450 in pSB1K3

AmiC

P-RBS

17.08.2012

Restriction

GroES (EcoRI/SpeI)

Ligation

GroES in pSB1C3

Transformation

GroES in pSB1C3

Test restriction

P-RBS (EcoRI/PstI)

BBa_J04450 in pSB1A3 (EcoRI/PstI)

BBa_J04450 in pSB1T3 (EcoRI/PstI)

BBa_J04450 in pSB1C3 (EcoRI/PstI)

BBa_J04450 in pSB1K3 (EcoRI/PstI)

1% Agarose gel

M:1kb gene ruler plus, 1-4: BBa_J04450 in pSB1A3, 5-8: BBa_J04450 in pSB1K3 P108-RBS, 9-12: BBa_J04450 in pSB1C3, (control digest 17.08.2012)

1% Agarose gel

M:1kb gene ruler plus, 1-4: P-RBS (E/P), 5-8: P-RBS (RsaI), 9-12: BBa_J04450 in pSB1T3, (control digest 17.08.2012)

20.08.2012

PCR

Backbone (primer MS24 + MS25)

⇒ template-DNA: pSB1A3, pSB1T3, pSB1C3 and pSB1K3, annealing: 30 sec; 55 °C, elongation: 30 sec; 72 °C , 35 cycles

1% Agarose gel

M:1kb gene ruler plus, 1: pSB1A3, 2: pSB1T3, 3: pSB1C3, 4: pSB1K3 (PCR 20.08.2012)

Transformation

BBa_JH023

Inoculation

GroES

P-RBS

GFP-T

Enhancer 3,4

AmiC

P-RBS alt

GFP-T alt

21.08.2012

Results

colonies of BBa_JH023

inoculations except AmiC and P-RBS alt successful

PCR

pSB1A3-BBa_J04450 (template DNA)

pSB1T3-BBa_J04450 (template DNA)

pSB1C3-BBa_J04450 (template DNA)

pSB1K3-BBa_J04450 (template DNA)

used primer --> MS24 + MS25

initial denaturation 98°C - 5min

denaturation: 98°C - 1min; annealing: 55°C - 30s; elongation: 72°C - 2.5min -->repeat 35 times

72°C - 5min --> 4°C - 8

miniprep

GroES, Enh 3/4 (+old), P-RBS (+old), GFP-T (+old)

Test restriction

of miniprep

over night, 37°C

1% Agarose gel

M:1kb gene ruler plus, 1:pSB1A3, 2:pSB1K3, 3:pSB1C3, 4:pSB1T3, 5: negative control, (PCR 21.08.2012)

Inoculation

E.coli BBa_I14032

over night, 37°C

22.08.2012

PCR

CFP (MS16 + MS17)

mRFP (MS14 + MS15)

initial denaturation 98°C - 5min

denaturation: 98°C - 10s; annealing: 60°C - 30s; elongation: 72°C - 40s -->repeat 35 times

72°C - 5min --> 4°C - 8

1% Agarose gel

M:1kb gene ruler plus, 1:mRFP, 2:mRFP, 3:CFP, 4:CFP (PCR 22.08.2012)

miniprep

of LacIQ

Test restriction

of LacIQ with EcoRI and PstI

1% Agarose gel

M:1kb gene ruler plus, 1-4:LacIQ, (control digest 22.08.2012)

1% Agarose gel

M:1kb gene ruler plus, 1-4:GroES, 5-12: GFT-Terminator, (control digest 21.08.2012)

1% Agarose gel

M:1kb gene ruler plus, 1-12:Enhancer, (control digest 21.08.2012)

1% Agarose gel

M:1kb gene ruler plus, 1-4:Enhancer, 5-12: P-RBS, (control digest 21.08.2012)

test restriction of Enhancer (->21.08.12), gel 2%

watch picture

test restriction of Enhancer and P-RBS (->21.08.12), gel 2%

watch picture

23.08.2012

PCR

pSB1K3-BBa_J04450 (template DNA)

pSB1T3-BBa_J04450 (template DNA)

used primer --> MS24 + MS25

initial denaturation 98°C - 5min

denaturation: 98°C - 1min; annealing: 55°C - 30s; elongation: 72°C - 2.5min -->repeat 35 times

72°C - 5min --> 4°C - 8

1% Agarose gel

M:gene ruler mix ladder, 1-2:pSB1K3-BBa_J04450, 3-4: pSB1T3-BBa_J04450, (PCR 23.08.2012)

Restriction

GixR (EcoRI/PstI)

Ligation

GixR in pSB1C3

Transformation

GixR in pSB1C3

24.08.2012

PCR

pSB1A3-BBa_J04450 (template DNA)

pSB1T3-BBa_J04450 (template DNA)

pSB1C3-BBa_J04450 (template DNA)

pSB1K3-BBa_J04450 (template DNA)

initial denaturation 98°C - 5min

denaturation: 98°C - 10s; annealing: 60°C - 30s; elongation: 72°C - 40s -->repeat 30 times

72°C - 10min --> 4°C - 8

primer: MS22 + MS23

1% Agarose gel

M:gene ruler mix ladder, 1-2:pSB1A3-BBa_J04450, 3-4: pSB1K3-BBa_J04450, 5-6:pSB1C3-BBa_J04450, 7-8: pSB1T3-BBa_J04450, (PCR 24.08.2012)

Restriction

RBS (XbaI/PstI)

CFP (EcoRI/PstI)

mRFP (EcoRI/PstI)

Ligation

mRFP and CFP in pSB1C3

Transformation

mRFP and CFP in pSB1C3

27.08.2012

Results

CFP: 1 colony

CFP (neu): Colonies

mRFP: colonies

mRFP (neu): no colonies

PCR

template: backbones (pSB1K3/T3/C3/A3)

parameters: 98°C 5min, >> 98°C 1min, 70°C 30s, 72°C 2.5min << x30, 72°C 5min, 4°C 8

primer: MS22 + MS23

colony-PCR

parameters: 98°C 5min, >> 98°C 1min, 72°C 1min << x30, 72°C 5min, 4°C 8

primer: MS18 + MS19

Agarose gel of backbone PCR

no result

elution of the backbones of Friday the 24th

1% Agarose gel

M:1kb gene ruler plus, 1-2:gixR, 3-9: LacIQ-RBS-Gin, 10: CFP, (colony PCR 27.08.2012)

1% Agarose gel

M:1kb gene ruler plus, 1-4:CFP, 5-10: mRFP, (colony PCR 27.08.2012)

Inoculation

pSB1C3_...

mRFP clone 20,24

CFP clone 14,15,17,18

gix clone 1,2

5ml LB, over night, 37°C

28.08.2012

production of competent TOP10

PCR

Enhancer, Terminator, Gix, P-RBS

parameters: 98°C 5', 98°C 1', 66°C 30", 72°C 30", 72°C 5', 4°C ~

primer: MS20 + MS21

1% Agarose gel

M:1kb gene ruler plus, 1:Terminator, 2-3: Enhancer, 4-6: P-RBS, 7-8: GixR, 9-10: Enhancer, (PCR 28.08.2012)

Transformation

[http://partsregistry.org/Part:BBa_I0500 pBad/araC] (plate:1, Well:N14)

pSacB

over night, 37°C

miniprep

GixR (1,2)

CFP (14,15,17,18)

mRFP (20,24)

alle in pSB1C3

29.08.2012

Results

Transformation: no colonies

PCR

Terminator, Gix, Enhancer, P-RBS

diluted templates: Terminator, P-RBS, Gix 1 --> 1:10

Enhancer, Gix 2 --> 1:20

parameters: 98°C 5', 98°C 1', 66°C 30", 72°C 30", 72°C 5', 4°C ~

primer: MS20 + MS21

1% Agarose gel

M:1kb gene ruler plus, 1:Terminator, 2-3: Enhancer, 4-6: P-RBS, 7-8: GixR, 9: Enhancer control, 10: P-RBS control, 11: GixR control, (PCR 29.08.2012)

3AA

CFP, mRFP with Terminator

2µl DNA

1µl SpeI

2µl Tango

15µl dH2O

--> 1h at 37°C

+1µl EcoRI

+2,5µl Tange

--> 1h at 37°C

--> inactivation for 20min at 80°C

Ligation

3AA products in pSB1T3

18.5µl H2O

2.5 µl Buffer

1µl Insert CFP or mRFP (EcoRI + SpeI)

1µl Insert Terminator (BBa_B0010) (XbaI + PstI)

1µl pSB1T3 (EcoRI + PstI)

1µl Ligase

--> 1h at RT

Transformation

pBad --> TOP10 + pSB2K3

CFP-T, mRFP-T --> TOP10 + pSB1T3

Sequencing

CFP_fwd

CFP_rev

mRFP_fwd

mRFP_rev

P-RBS_fwd

GixR_fwd

GixR_fwd

Enhancer_fwd

30.08.2012

Results

Transformation: no colonies --> testing Trafo with BBa_J04450 A/K/T/C

2 colonies at pBad-Trafo from 28.08.2012 --> liquid culture for miniprep

1 colony at pSacB-Trafo from 28.08.2012 --> tested on succrose-sensitivity

31.08.2012

PCR

SacB

Parameters No.1: 95°C 5', >>95°C 30", 60°C 30", 72°C 1'<< x30, 72°C 5', 4°C

Parameters No.2: 95°C 5', >>95°C 30", 72°C 1.5'<< x30, 72°C 5', 4°C

Primer MS26 + MS27

1% Agarose gel

M:1kb gene ruler plus, 1,3,5:SacB, 4,5: none, (PCR 31.08.2012)

Ligation

3AA (CFP-T, mRFP-T)

watch 29.08.

used vector: pSB1K3/T3

Transformation

of ligation in TOP10

miniprep

pBad/araC K.1+2

restriction

GixR rehybridization

cut with EcoRI and PstI

ligation

1µl GixRhyb E+P

1µl pSB1C3 E+P

1µl Th-Pol

2µl Buffer

15µl dH2O

Transformation

ligation + TOP10 --> LB(cam)

Results of test-trafo

Amp, Km, Cm OK --> Km with fewer colonies

Tet --> hardly colonies

--> comp.TOP10 obviously all right, exclusion of Tet in future work

03.09.2012

Results

Transformation

GixR in C3 --> no colonies

CFP-T/mRFP-T in C3(31.8.) --> no colonies

CFP-T/mRFP-T in T3(31.8.) --> many but small colonies

CFP-T/mRFP-T in T3(29.8.) --> less colonies

colony-PCR

of colonies (CFP-T, mRFP-T)

parameters: 98°C 5', >>98°C 1', 72°C 1'<<x30, 72°C 5', 4°C

primer MS18 + MS19

Agarose gel

6x colony pT3-CFP-T from 29./31.8.

6x colony pT3-mRFP-T from 29./31.8.

pC3-CFP (14)

pC3.mRFP (24)

1% Agarose gel

M:1kb gene ruler plus, 1-6:CFP-Terminator, 7:CFP control, 8-13:mRFP-Terminator 14: mRFP control, 15-16: none, (colony-PCR 03.09.2012)

04.09.2012

Results

Transformation

CFP-T/mRFP-T in T3

2 µl -> 5-6 colonies

30 µl -> 1-2 colonies

Gix R in C3 (3.9) --> 4 colonies

colony-PCR

GixR

CFP-T

mRFP-T

parameters: 98°C 5min, >> 98°C 1min, 72°C 1min << x30, 72°C 5min, 4°C ∞

primer MS20 + MS21

gel extraction

P108 (E/S)

RBS (X/P)

ligation

SacB1 + pSB1C3

P-RBS + pSB1C3

Transformation

ligation + TOP10 --> LB(cmp)

1% Agarose gel

M:1kb gene ruler plus, 1-2:pBAD/araC, (mini-prep 31.08.2012)

Inoculation

pBad/araC

5ml LB, over night, 37°C

1% Agarose gel

M:1kb gene ruler plus, 1-4:GixR pSB1C3, 5-9:CFP-Terminator, 10:CFP control, (colony-PCR 04.09.2012)

1% Agarose gel

M:1kb gene ruler plus, 1-9:mRFP-Terminator, 10:mRFP control, (colony-PCR 04.09.2012)

05.09.2012

Results

Transformation

SacB in C3

P-RBS in C3

colony PCR

SacB in C3

P-RBS in C3

parameters: 98°C 5min, >> 98°C 1min, 72°C 1min << x30, 72°C 5min, 4°C ∞

primer MS20 + MS21

miniprep

Gix in C3

pBad

Results

Transformation

CFP-T (03.09) --> 10 colonies

colony PCR

P108-RBS, SacB, GixR

parameters: 98°C 5min, >> 98°C 1min, 72°C 1min << x30, 72°C 5min, 4°C ∞

primer MS19 + MS20

1% Agarose gel

no marker, 1:none, 2-7:SacB, 8-11:P108-RBS, (colony-PCR 05.09.2012)

1% Agarose gel

no marker, 1-5:P108-RBS, 6:none, 7-9:GixR, 10:Scar, 11-12: pBad, 13-15: pGixR, (colony-PCR 05.09.2012)

restriction

pSB1A3 (E/P)

pSB1K3 (E/P)

pSB1C3 (E/P)

pSB1T3 (E/P)

GFP-T K3 (X/P)

GFP K3 (X/P)

CFP C3 (X/P)

mRFP C3 (X/P)

AmiC A (E/S)

GroES A (E/S)

Terminator (X/P)

Inoculation

pRBS

SacB

mRFP-Terminator

5ml LB, over night, 37°C

06.09.2012

miniprep

pRBS

SacB

mRFP-Terminator

ligation

AmiC (E/S) + GFP (X/P) + pSB1T3 (E/P)

AmiC (E/S) + RFP (X/P) + pSB1T3 (E/P)

AmiC (E/S) + GCFP (X/P) + pSB1T3 (E/P)

AmiC (E/S) + Terminator (X+P + pSB1T3 (E/P)

GroES (E/S) + GFP (X/P) + pSB1T3 (E/P)

GroES (E/S) + RFP (X/P) + pSB1T3 (E/P)

GroES (E/S) + CFP (X/P) + pSB1T3 (E/P)

GroES (E/S) + Terminator (X/P) + pSB1T3 (E/P)

PCR of miniprep

SacB in pSB1C3

p-RBS in pSB1C3

terminator in pSB1T3

parameters: 98°C 5min, >> 98°C 30 sec, 72°C 1,5min << x30, 72°C 5min, 4°C ∞

primer MS20 + MS21

1% Agarose gel

M:1kb gene ruler plus, 1:Scar, 2-5:P-RBS, 6-9:SacB, 10-16: mRFP, 17: control, (PCR of miniprep (06.09.2012)

transformation

RBS-Gin T3

amiC A3

groES A3

groES-Terminator T3

groES-GFP T3

groES-CFP T3

groES-mRFP T3

amiC-Terminator T3

amiC-GFP T3

amiC-CFP T3

amiC-mRFP T3

07.09.2012

restriction (6.9.)

ligation

AmiC in pSB1K3

GroES in pSB1K3

mRFP in pSB1K3

Terminator in pSB1K3

CFP in pSB1K3

GFP in pSB1K3

GFP+Terminator in C3

Enhancer in K3

transformation

Ligation

AmiC

GroES

RBS-Gin

miniprep

CFP-Terminator

Sequencing

mRFP T3

P-RBS K12

P-RBS K15

SacB K6

SacB K6

10.09.2012

Restriction

Gin-RBS (01.08)

Ligation

Gin-RBS in pSB1C3

Transformation

Gin-RBS in pSB1C3

Hybridisation

GixR

98 °C 20 min

minus 1 °C to 4 °C in 2 min

Ligation and Transformation

GixR (X+S) + pSB1K3 (X+S)

Inoculation (Tetracycline)

GroES-mRFP

GroES-GFP

GroES-CFP

amiC-mRFP

amiC-GFP

amiC-CFP

5ml LB, over night, 37°C

Inoculation (Kanamycine)

GroES-GFP

amiC-mRFP

amiC-GFP

GroES-Terminator

Enhancer

5ml LB, over night, 37°C

Inoculation (Chloramphenicol)

GFP-Terminator

5ml LB, over night, 37°C

Inoculation (Ampicillin)

Terminator

5ml LB, over night, 37°C

11.09.2012

microscopy-screening

GroES-GFP ⇒; no fluorescence

GroES-CFP ⇒; no fluorescence

AmiC-mRFP ⇒; no fluorescence

AmiC-GFP ⇒; no fluorescence

colony-PCR

GixR

RBS-Gin

Terminator

parameters: 98°C 5', >>98°C 1', 72°C 1'<<x30, 72°C 5', 4°C

primer MS20 + MS21

3A-Assembly (digestion, ligation, transformation)

GroES (E/S) + Terminator (X/P) + pSB1K3 (P/E)

AmiC (E/S) + Terminator (X/P) + pSB1K3 (P/E)

plasmid-prep and control-digestion (E/P)

GroES-GFP

GroES-CFP

AmiC-mRFP

AmiC-GFP

GroES-Terminator

Enhancer

GFP-Terminator

Terminator

12.09.2012

Results

Transformation

- P-RBS --> colonies

- pB10 --> no colonies

- RBS (B0030) --> colonies

- Gro-ES/ AmiC-Terminator --> no colonies

colony-PCR

Gix (2. try)

Gin-RBS (2. try)

RBS (B0030)

P-RBS (108)

parameters: 98°C 5', >>98°C 1', 72°C 1'<<x30, 72°C 5', 4°C

primer MS20 + MS21

Agarose gel

Gin-RBS (5x)

Gin (1x)

Gix (5x)

RBS (6x)

P-RBS (6x)

1% Agarose gel

M:1kb gene ruler plus, 1:Scar, 2-6:RBS-Gin, 7:Gin control 8-12: gixR, 13: control, (colony-PCR 12.09.2012)

1% Agarose gel

M:1kb gene ruler plus, 1:Scar, 2-6:RBS BBa_B0030, 7-12:P-RBS, 13: control, (colony-PCR 12.09.2012)

Restriction (miniprep 11.09.12)

gr-GFP

gr-CFP

gr-T K3

enhancer K3

am-RFP-K3

am-GFP-K3

GFP-T-C3

terminator A2

1% Agarose gel

M:1kb gene ruler plus, 1-3:GroES-GFP, 4:GroES-GFP control, 5:GroES-CFP, 6:GroES-CFP control, 7-10: GroES-Terminator, 11: GroES-Terminator control, 12-15: Enhancer, 16: Enhancer control, (control digest 12.09.2012)

1% Agarose gel

M:1kb gene ruler plus, 1-2:AmiC-mRFP, 3:AmiC-mRFP control, 4-5:AmiC-GFP, 6:AmiC-GFP control, 7-11: GFP-Terminator, 12: GFP-Terminator control, 13-15: Terminator, 16: Terminator control, (control digest 12.09.2012)

Transformation

groES-T

2 Transformations:

- One with a 1:10 dilution of Terminator from ligation,

- another one with a 1:100 dilution of Terminator from ligation

amiC-T

2 Transformations:

- One with a 1:10 dilution of Terminator from ligation,

- another one with a 1:100 dilution of Terminator from ligation

PCR

Gin-RBS

3 reactions:

-One using High Fidelity (HF) Reaction Buffer,

-one using GC-Buffer

-and another one using self-made reaction buffer

Primer used : MS12 + MS13

Template DNA : E. coli C600 chromosomal DNA

13.09.2012

Results

Transformation

- pBAD (11.09.12) --> no colonies

- AmiC-T (11.09.12) --> 2 x 2 colonies

- GroES-T (11.12.09)--> 2 colonies

colony-PCR

AmiC-T & GroES-T (transformation 11.09.12)

parameters: 98°C 5', >>98°C 1', 72°C 1'<<x30, 72°C 5', 4°C

primer MS20 + MS21

1% Agarose gel

M:1kb gene ruler plus, 1:RBS-Gin HF, 2:RBS-Gin GC, 3:RBS-Gin SM (PCR 13.09.2012)

Gel extraction

RBS-Gin (HF) --> 51 ng/µl

RBS-Gin (GC) --> 69 ng/µl

RBS-Gin (SM) --> 56 ng/µl

Ligation

GroES-T & AmiC-T in pSB1K3

Restriction (preparative digest)

GroES (A module)

with SpeI

AmiC (A module)

with SpeI

mRFP-C3 (B module)

with EcoRI and XbaI

CFP-C3 (B module)

with EcoRI and XbaI

Gin-RBS

HF-PCR-Product, GC-PCR-product and SM-PCR-product

with EcoRI and PstI

1% Agarose gel

M:1kb gene ruler plus, 1-4:AmiC-Terminator, 5-6:GroES-Terminator, 7:Scar, 8: control, (colony-PCR 13.09.2012)

14.09.2012

Results

Transformation

AmiC-T: no colonies

GroES-T: no colonies

Restriction

2nd Digestion of A-modules (see digest from yesterday) additionally with EcoRI

Ligation

Gin-RBS with pSB1C3

3 reactions:

one with RBS-Gin HF-PCR-Product

one with RBS-Gin GC-PCR-Product

one with RBS-Gin SM-PCR-Product

Inoculation

Gix-K3 (clone 3 and 4)

P-RBS-C3 (clone 1 and 3)

RBS (BBa_B0030) [clone 1 and 3]

1% Agarose gel

M:1kb gene ruler plus, 1:AmiC, 2:GroES, 3:none, 4:GFP, 5:CFP, 6:mRFP,(digest 13.-14.09.2012)

Gel extraction

GFP

mRFP

1% Agarose gel

M:1kb gene ruler plus, 1:Terminator, (digest 14.09.2012)

Gel extraction

Terminator clone 48

Transformation

RBS-Gin(HF)-pSB1C3

RBS-Gin(GC)-pSB1C3

RBS-Gin(SM)-pSB1C3

17.09.2012

Restriction

AmiC

GroES

CFP

SacB

1% Agarose gel

M:1kb gene ruler plus, 1:AmiC control, 2:AmiC, 3:GroES control, 4:GroES, 5:CFP control, 6:CFP, 7:SacB control, 8:SacB (digest 17.09.2012)

Restriction

CFP-C3

SacB (2nd try)

Resuspend

BBa_B001J

Restreak

RBS-Gin (HF)

RBS-Gin (GC)

RBS-Gin (SM)

DNA isolation

CFP-C3 (Miniprep28.08.12)--> 47,3 ng/µl

Miniprep

GixR pSB1K3 --> 50,5 ng/µl, 144,7 ng/µl

RBS(new)B0030 pSB1A2 --> 726,2 ng/µl, 242,6 ng/µl

P108-RBS pSB1C3 --> 200,5 ng/µl, 177,8 ng/µl

1% Agarose gel

M:1kb gene ruler plus, 1-2:GixR, 3-4:RBS BBa_B0030, 3-4:P108-RBS, (mini prep 17.09.2012)

Transformation

pSB2K3-pBAD & pSB1-A2-TT

1% Agarose gel

CFP-C3 (restriction 2nd try)

SacB-Cs (restriction 2nd try)

M:1kb gene ruler plus, 1:CFP control, 2:CFP, 3:SacB, (digest 17.09.2012)

18.09.2012

Results

Transformation

2x Terminator --> colonies

pBAD --> no colonies

Colony PCR

RBS-Gin

2x Terminator

parameters: 98°C 5', >>98°C 1', 72°C 1'<<x30, 72°C 5', 4°C

primer MS20 + MS21

1% Agarose gel

M:1kb gene ruler plus, 1-2:RBS-Gin HF, 3:RBS-Gin GC, 4:RBS-Gin SM, 5: Scar, 7-10:2xTerminator, 11:control, (colony-pcr 18.09.2012)

Sequencing

SacB

Gel extraction

CFP-C3 E+X

Ligation

am-G: amiC E+S & GFP-A3 E+X

am-C: amiC E+S & CFP-C3 E+X

am-R: amiC E+S & mRFP-C3 E+X

gro-G: groES E+S & GFP-A3 E+X

gro-C: groES E+S & CFP-C3 E+X

gro-R: groES E+S & mRFP-C3 E+X

Transformation

am-G

am-C

am-R

gr-G

gr-C

gr-R

pBAD

19.09.2012

Results

Transformation

am-G --> colonies

am-C --> colonies

am-R --> colonies

gr-G --> colonies

gr-C --> colonies

gr-R --> colonies

pBAD --> no colonies

Colony PCR

RBS-Gin (from 17.09.12)

2x Terminator B0017 (from 17.09.12)

parameters: 98°C 5', >>98°C 1', 72°C 1'<<x30, 72°C 5', 4°C

primer MS20 + MS21

--> Amplification failed

Transformation

pBAD

Microscopy-screening

AmiC-GFP --> fluorescence

GroES-GFP --> fluorescence

AmiC-CFP --> fluorescence

GroES-CFP --> fluorescence

AmiC-mRFP --> fluorescence

GroES-mRFP --> fluorescence

Inoculation

RBS-Gin

TT (B0017)

AmiC-GFP

GroES-GFP

AmiC-CFP

GroES-CFP

AmiC-mRFP

GroES-mRFP

20.09.2012

Miniprep

RBS-Gin

TT (B0017)

AmiC-GFP

GroES-GFP

AmiC-CFP

GroES-CFP

AmiC-mRFP

GroES-mRFP

Restriction (E/P)

TT(B0017)

RBS-Gin

1% Agarose gel

M:1kb gene ruler plus, 1,3,5,7:2xTerminator, 2,4,6,8:2xTerminator control, 9,11,13,15:RBS-Gin, 10,12,14,16:RBS-Gin control, (control digest 20.09.2012)

Restriction

SacB ((XbaI + PstI) & (EcoRI + XbaI)

P-RBS (EcoRI + SpeI) & (SpeI + PstI)

1% Agarose gel

M:1kb gene ruler plus, 1:P-RBS control, 2: P-RBS (E/S), 3: P-RBS (S/P), 4: SacB control, 5: SacB (X/P), 6:SacB (E/X), (digest 20.09.2012)

Inoculation

GroES-GFP

GroES-CFP

GroES-mRFP