- standard electroporation protocol
- used electro competend DH5alpha from NEB
- streaked out on LB-plates with Cam
Team:Bielefeld-CeBiTec/Notebook/Labjournal
Labjournal
2017-04-03 - 2017-04-09
getting positive clones for further work
Investigators: Yannic Kerkhoff
Aim of the experiment: electroporation transformation of BBa_K1416000
Procedure:
getting positive clones for further work
Investigators: Yannic Kerkhoff
Aim of the experiment: electroporation transformation of BBa_KJ36848
Procedure:
- standard electroporation protocol
- used electro competend DH5alpha from NEB
- streaked out on LB-plates with Cam
multiplication of plasmids containing the Biobrick
Investigators: Yannic Kerkhoff
Aim of the experiment: preculture of transformed BBa_K1416000
Procedure:
- standard procedure
- 1,25֬ Cam in 5mL LB
2017-04-10 - 2017-04-16
getting plasmids containing the Biobrick for further experiments
Investigators: Yannic Kerkhoff
Aim of the experiment: plasmid isolation of preculture of BBa_K1416000
Procedure:
- standard protocol
- 517,9 ng/
multiplication of plasmids containing the Biobrick
Investigators: Yannic Kerkhoff
Aim of the experiment: preculture of transformed BBa_J36848
Procedure:
- standard procedure
- 1,25֬ Cam in 5mL LB
getting plasmids containing the Biobrick for further experiments
Investigators: Yannic Kerkhoff
Aim of the experiment: plasmid isolation of preculture of BBa_J36848
Procedure:
- standard protocol
- 231,8 ng/
2017-05-29 - 2017-06-04
getting positive clones for further work
Investigators: Yannic Kerkhoff
Aim of the experiment: heatshock transformation of BBa_E0400
Procedure:
- standard heatshock protocol
- used own produced chemo competend DH5alpha
- streaked out on LB-plates with Amp
2017-06-05 - 2017-06-11
multiplication of plasmids containing the Biobrick
Investigators: Yannic Kerkhoff
Aim of the experiment: preculture of transformed BBa_E0400
Procedure:
- standard procedure
- 5,0֬ Amp in 5mL LB
getting plasmids containing the Biobrick for further experiments
Investigators: Yannic Kerkhoff
Aim of the experiment: plasmid isolation of preculture of BBa_E0400
Procedure:
- standard protocol
- 88,4 ng/
getting positive clones for further work
Investigators: Yannic Kerkhoff
Aim of the experiment: heatshock transformation of BBa_K525998
Procedure:
- standard heatshock protocol
- used own produced chemo competend DH5alpha
- streaked out on LB-plates with Cam
multiplication of plasmids containing the Biobrick
Investigators: Yannic Kerkhoff
Aim of the experiment: preculture of transformed BBa_K525998
Procedure:
- standard procedure
- 1,25֬ Cam in 5mL LB
getting plasmids containing the Biobrick for further experiments
Investigators: Yannic Kerkhoff
Aim of the experiment: plasmid isolation of preculture of BBa_K525998
Procedure:
- standard protocol
- 140,9 ng/
2017-06-12 - 2017-06-18
Assemble the fragments to get the composite Part BBa_P1:GLS1
Investigators: Yannic Kerkhoff
Aim of the experiment: Gibson assembly of F1,F3,F5
Procedure:
- standard Gibson Assembly protocol
To get and purified the plasmid
Investigators: Christina Drake
Aim of the experiment: Plasmidisolation of barnase-plasmid
Procedure:
- protocol from Macherley-Nagel: Plasmid DNA purification, protocol 5: NucleoSpin
- concentration measurement by nanoprop
- sequenzingorder
Duplicate the parts
Investigators: Christina Drake, Denise Kerkhoff
Aim of the experiment: Transformation via Distribution of the parts BBA_J04450, BBa_I746909, BBa_K80800 and BBa_psB1K5
Procedure:
- transformation via electroporation
- plated out: BBa_J04450 on tetracycline, BBa_I74909 and BBa_K808000 on chloramphenicol, BBa_psB1K5 on kanamycin
Duplicate the part
Investigators: Christina Drake, Denise Kerkhoff
Aim of the experiment: Transformation of BBa_psB6A1
Procedure:
- transformation via electroporation
- plated out on amphenicol
Cellgrowth with the plasmids
Investigators: Denise Kerkhoff, Christina Drake
Aim of the experiment: Overnightculture of BBA_J04450, BBa_I746909 and BBa_K808000
Procedure:
- 3 ml LB-medium and at BBA_J04450 3µl tetracycline and atBBa_I746909 and BBa_K808000 0,75 µl chloramphenicol
- inkubation overnight 37°C, 140rpm
To get and purified the plasmid
Investigators: Christina Drake
Aim of the experiment: Plasmidisolation of BBA_J04450, BBa_I746909 and BBa_K80800-plasmids
Procedure:
- protocol from Macherley-Nagel: Plasmid DNA purification, protocol 5: NucleoSpin
- concentration measurement by nanoprop:
- BBA_J04450 26ng/µl and 25,7ng/µl
- BBa_I746909 90,2ng/µl
- 104,3 ng/µl -BBa_K808000 118,3 ng/µl
- and 146,6 ng/µl
- sequenzingorder
2017-06-19 - 2017-06-25
Cellgrowth with the plasmid
Investigators: Denise Kerkhoff
Aim of the experiment: Overnightculture of BBA_psB3K5
Procedure:
- 3 ml LB-medium and 2,5 µl kanamycin
- inkubation overnight 37°C, 140rpm
getting positive clones for further work
Investigators: Yannic Kerkhoff
Aim of the experiment: heatshock transformation of assembled fragments F5,F2,F4
Procedure:
- standard heatshock protocol
- used own produced chemo competend DH5alpha
- streaked out on LB-plates with Cam
multiplication, verification and purification of the needed fragment F2: GFPLinker2
Investigators: Yannic Kerkhoff
Aim of the experiment: Q5-PCR, gel and PCR-cleanUp of F2
Procedure:
- standard Q5-PCR protocol
- template: BBa_E0400
- primer fwd: 17gk
- primer rev: 17gn
- annealing temperature: 58у
- extension time: 50 seconds
- standard PCR-cleanUp protocol
- 125,8 ng/
multiplication, verification and purification of the needed fragment F4: StrepLinker2
Investigators: Yannic Kerkhoff
Aim of the experiment: Q5-PCR, gel and PCR-cleanUp of F4
Procedure:
- standard Q5-PCR protocol
- template: BBa_KJ36848
- primer fwd: 17gp
- primer rev: 17gq
- annealing temperature: 61у
- extension time: 30 seconds
- standard PCR-cleanUp protocol
- 127,0 ng/
multiplication, verification and purification of the needed fragment F5: linearized pSB1C3
Investigators: Yannic Kerkhoff
Aim of the experiment: Q5-PCR, gel and PCR-cleanUp of F5
Procedure:
- standard Q5-PCR protocol
- template: K1416000
- primer fwd: 17gj
- primer rev: 17gl
- annealing temperature: 59у
- extension time: 120 seconds
- standard PCR-cleanUp protocol
- 258,4 ng/
Assemble the fragments to get the composite Part BBa_P2:GLS2
Investigators: Yannic Kerkhoff
Aim of the experiment: Gibson assembly of F2,F4,F5
Procedure:
- standard Gibson Assembly protocol
Screening for positive transformations containing the Biobrick BBa_P2:GLS2
Investigators: Yannic Kerkhoff
Aim of the experiment: GoTaq PCR of seven clones
Procedure:
- standard GoTaq-protocol
- template: colonie pcr clones of GA_P2:GLS2
- primer fwd: Pr姩x_fwd
- primer rev: Suffix_rev
- annealing temperature: 56у
- extension time: 40 seconds
- positive clone 2
multiplication of plasmids containing the Biobrick
Investigators: Yannic Kerkhoff
Aim of the experiment: preculture of the positive clone 2 of BBa_P2:GLS2
Procedure:
- standard procedure
- 1,25֬ Cam in 5mL LB
getting plasmids containing the Biobrick for further experiments
Investigators: Yannic Kerkhoff
Aim of the experiment: plasmid isolation of preculture of BBa_P2:GLS2
Procedure:
- standard protocol
- 208,8 ng/
2017-06-26 - 2017-07-02
Check the sequence
Investigators: Christina Drake
Aim of the experiment: Sequenzingorder barnase
Procedure:
- concentration measurement by nanoprop: 177 ng/µl
- result: sequence was not barnase
PCR clean up of gblock1, gblock2 and pK18mobsacB-backbone
Investigators: Camilla Maerz
Aim of the experiment: Construction of pK18mobsacB_codA_del
Procedure:
- PCR and DNA purification kit
- Nucleo spin PCR and Monarch® PCR & DNA Clean-up protocol
Plasmidisolation and gibson assembly of pSB1C3-PlacUV5_PtNTT2 c30
Investigators: Camilla Maerz
Aim of the experiment: Construction of pSB1C3-PlacUV5_PtNTT2
Procedure:
- Plasmid DNA purification kit
- Nucleo spin plasmid protocol
- Gibson Assembly protocol
- transformation via heat shock protocol in E. coli DH5alpha
Isolate T7RNAP from the chromosome of KRX-e.coli
Investigators: Christina Drake
Aim of the experiment: PCR of T7RNAP from KRX-e.coli
Procedure:
- Q5 High-Fidelity PCR
- annealingtemparatur 64°C, elogationtime 1 min
- 1%-agarose-TAE-gel
- 1kb Marker Geneuler and 5 µl sample with 1 µl 6*Loading Dye
Plated out Barnase from strain collection
Investigators: Christina Drake
Aim of the experiment: Plated out Barnase from strain collection
Procedure:
- solved DNA in 100 µl SOC-medium
- plated out on chloramphenicolplate
- overnightincubation at 37°C
Colony PCR of pK18mobsacB-del_codA
Investigators: Camilla Maerz
Aim of the experiment: Construction of pK18mobsacB_codA_del
Procedure:
- Go Tag (Promega) protocol
- Primer: VR, VF2
- Primer annealing: 56 у
- Elongation: 140 s
2017-07-03 - 2017-07-09
t
Investigators: Christina Drake
Aim of the experiment: Plasmidisolation of Barnase and colonies 1-5 T7RNAP
Procedure:
- protocol from Macherley-Nagel: Plasmid DNA purification, protocol 5: NucleoSpin
- concentration measurement by nanoprop
- Go-Taq-protocol
- annealingtemparatur 58°C, elogationtime 30 s
- 1%-agarose-TAE-gel
- 100bp Marker Geneuler and 5 µl sample with 1 µl 6*Loading Dye
- result: PCR-product could not be barnase
2017-07-10 - 2017-07-16
Biobrick Assembly of 2B1
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- BioBrick Assembly
- RuBisCoTAG mRFP as upstream part, T7-Terminator as downstream part, pSB1A3 as destination plasmid
- transformation via heat shock and DH5α Cells
- used 5µl from the ligation
- plated out on Amp plates and let them grow over night
Check the sequence
Investigators: Christina Drake
Aim of the experiment: Sequenzingorder barnase
Procedure:
- result: sequence was not barnase
- 3 ml LB-medium and 0,75 µl chloramphenicol
- inkubation overnight 37°C, 140rpm
Transformation of T7-Promotor
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- transformation via electroporation of cells with T7-Promotor
Preculture of colonies with T7-Promotor
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- used 5µl LB media and kanamycin
2017-07-17 - 2017-07-23
Isolate the tRNA
Investigators: Christina Drake
Aim of the experiment: PCR of TyrRS-Heidelberg-plasmid
Procedure:
- plasmidisolation with MN protocol 5
- Q5 High-Fidelity PCR
- annealingtemparatur 53°C, elogationtime 20s
- Gibbsonassembly with 5µl backbone and 0.5 µl insert
- transformation via heat shock
- overnight incubation at 37°C
Isolation of T7-Promotor
Investigators: Laura Schlueter
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- Nucleospin Plasmidisolation protocol
- got four products with the concentrations 50.1 ng/µl, 16.3 ng/µl, 24,2 ng/µl and 2.1 ng/µl
Colony PCR with 2B1 Colonies
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
Biobrickassembly of 2B2 to 2B8, B1 and A1
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- BioBrick Assembly
- digest and ligate RuBisCo parts as upstreampart and T7-Terminator/Promotor as downstreampart and pSB1A3 as destination plasmid
- ligate TAG2 and T7-Terminator to 2B2
- ligate TAG111 and T7-Terminator to 2B3
- ligate TAG474 and T7-Terminator to 2B4
- ligate TAG2+TAG111 and T7-Terminator to 2B5
- ligate TAG2+TAG474 and T7-Terminator to 2B6
- ligate TAG111+TAG474 and T7-Terminator to 2B7
- ligate TAG2+TAG111+TAG474 and T7-Terminator to 2B8
- ligate RuBisCo mRFP and T7-Terminator to B1
- ligate Carboxysome and T7-Promotor to A1
- preculture of positive 2B1 colony
Transformation of test devices
Investigators: Camilla Maerz
Aim of the experiment: Interlab study
Procedure:
- dilute test devives (distribution plate 6 & 7) in 10 ddH20
- Transformation
- 1 plasmid from each plate
- transformation via heat shock protocol in E. coli XL1-blue
Transformation of 2B2-2B8, B1 and A1
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
Plasmidisolation of 2B1
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- Nucleospin Plasmidisolation protocol
- got 47 ng/µl and 41 ng/µl
Reverse the insert
Investigators: Christina Drake
Aim of the experiment: PCR of T7GFP
Procedure:
- Q5 High-Fidelity PCR
- Insert: annealingtemparatur 60°C,
- Backbone:elogationtime 30s: annealingtemparatur 60°C, elogationtime 1 min
- 1%-agarose-TAE-gel
- result: PCR didn`t work
Reverse the insert
Investigators: Christina Drake
Aim of the experiment: PCR of T7GFP
Procedure:
- 1%-agarose-TAE-gel
- result: PCR did work
- Gibson Assembly
- transformation via heat shock
Preparation of over-night culture
Investigators: Camilla Maerz
Aim of the experiment: Interlab study
Procedure:
- Over-night culture of negative control, positive control, test device 1-6
- LB-media + Cm were inoculated
- Cultures were incubated over night (37у, 200 rpm)
2017-07-24 - 2017-07-30
Repeat the degestion and transformation from the 18th and 19th july
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
Cellgrowth with the plasmid
Investigators: Christina Drake
Aim of the experiment: Overnightculture of tRNA-psB1C3
Procedure:
- 3 ml LB-medium and 0,75 µl chloramphenicol
- inkubation overnight 37°C, 140rpm
- transformation via heatschock
Cloning of the ori (pSB6A1) in pSB1C3
Investigators: Laura Schlueter
Aim of the experiment: aaRS Plasmid (without aaRS)
Procedure:
- Gibson Assembly Master Mix
- Backbone: 3,28 Ori 1.0: 1,73
- Backbone: 0,32 Ori 1.1: 4,68
- Backbone: 0,90 Ori 3.0: 4,10
- Trafo: Hitzeschock
- not successfull because of the wrong overlapps (try again)
Colony PCR of the Retrafo of pRS (because of mixed culture)
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- Sequencing was not succesfull (maybe mixed colony), so I did a retrafo with the aim of a successful sequencing (incorporation of the aaRS in pSB1C3)
- pRS 3: 1-5
- pRS 4: 1-5
- pRS 5: 1-5
- pRS 7: 1-5
- no positive result (no band at 1000 bp)
Amplification of pSB1C3 for the cloning of the ori in pSB1C3
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- PCR with Q5 High-Fidelity Polymerase Master Mix, Primer jb,jn, 65у
- gelelectrophoresis, 1% Agarose
- band at 2000-2500 bp (supposed to be around 2200 bp)
- Clean up from the gel
- pSB1C3(nur ori): 22,2 ng/
Amplification of pSB1C3 fragments for a 4 part Gibson (see page 4 in the paper-labbook)
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- PCR, Q5 Master Mix
- Primer jj, jn for fragment 2, 65у
- Primer jb, ht for fragment 4, 65у
- gelelectrophoresis, 1% Agarose
- band at 300 (fragment 2, supposed to be around 326 bp)
- band at 1200 (fragment 4, supposed to be around 1233 bp)
- Clean up from the gel
- fragment 2: 18,5 ng/ (overlapp(aaRS)_pSB1C3_overlapp(ori))
- fragment 4: 19,1 ng/ (overlapp(ori)_pSB1C3_overlapp(aaRS))
Colony PCR of 2B2-2B8, B1 and A1
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- GoTaq® G2 PCR
- most have negative results -> create new destination plasmid pSB1A3
Colony PCR of retrafo and more colonies of the pRS
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- GoTaq Master Mix, Primer vr,vf
- 2 strong bands at 400 bp and 600 bp, small bands of pRS3,6 and pRS4,9 at around 1200-1500 bp
- bands of pRS31, pRS32, pRS34, pRS36, pRS39 at around 1200-1500 bp
- GoTaq Master Mix, Primer hq, jk (Gibson Assembly primer) with the colonies pRS31, pRS32, pRS34, pRS36, pRS39
- pRS31, pRS32, pRS39 : stron bands at around 1200 bp
- because of the the two positive colony PCRs (vf-vr, hq-jk) for these probes, the successful integration of the Tyr-aaRS in pSB1C3 seems to be successfull
- pRS31, pRS32, pRS39 send to sequencing
pRS31, pRS32, pRS39 plasmid isolation
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- Macherey-Nagel purification kit
- pRS31: 324,1 ng/
- pRS32: 231,8 ng/
- pRS39: 225,5 ng/
- send to the sequencing
- pRS31, pRS39 have the pSB1C3 with the Tyr-aaRS incorporated (but on position 32, the Arginine (cgt) should be changed to an Leucine (ctg), but it is not. On position 290 there really is a missing Leu, on position 268 the Asparagin is changed to an Arginine)
2017-07-31 - 2017-08-06
plasmid isolation of the positive colonies of the retrafo pRS4,4 (wrong!) and pRS3,12
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- Macherey-Nagel purification kit with each 3 mL culture
- pRS4,4: 44 ng/
- pRS3,12: 68,3 ng/
- not send to sequencing jet
4 part Gibson and Trafo
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- Gibson Assembly Master Mix with 5 ֬ template
- pSB1C3 fragment (2): 18,5 ng/ around 350 bp 2,2
- pSB1C3 fragment (4): 19,1 ng/ around 1300 bp 0,8
- oK1.1 (pMB1 from pSB6A1): 5,8 ng/ around 1300 bp 1,8
- Tyr-aaRS: 68,5 ng/ around 1000 bp 0,2
- Trafo via heatshock
Gibson of the ori in pSB1C3 (pori) and Trafo
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- Gibson Assembly Master Mix with 5 template
- pSB1C3(nur ori): 22,2 ng/ around 2100 bp 1,57
- ok1.0: 5,80 ng/ around 1258 bp 3,43
- Trafo via heatshock
Transfer positive colonies
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- picked and transfered positiv colonies of 2B2, 2B6, 2B7, 2B8 and A1 onto a new plate
- incubate over night
- 2B2 and 2B8 are contaminated with negativ colonies
construct a biobrick
Investigators: Christina Drake
Aim of the experiment: Aquacloning of tRNA and backbone
Procedure:
- transformation via heatschock
construct a biobrick
Investigators: Christina Drake
Aim of the experiment: Gibbsonassembly of barnase and backbone
Procedure:
- transformation via heatschock
- 3 ml LB-medium and 0,75 µl chloramphenicol
- inkubation overnight 37°C, 140rpm
Preculture of 2B6, 2B7 and A1
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- used 3µl LB media
Plasmidisolation
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- Nucleospin Plasmidisolation protocol
- got 67.3 ng/µl of 2B6
- got 32.7 ng/µl of 2B7
- got 51.6 ng/µl of A1
To get and purified the plasmid
Investigators: Christina Drake
Aim of the experiment: Plasmidisolation of barnase-plasmid and tRNA-plasmids
Procedure:
- protocol from Macherley-Nagel: Plasmid DNA purification, protocol 5: NucleoSpin
- concentration measurement by nanoprop
- sequenzingorder
Redo digestion of the destination plasmid
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- analyze the destination plasmid digestion via gelelectrophoresis
- pSB1A3 digestion was not effective
- redo the digestion and analyze it on the gel
- new dgestion was very effective
2017-08-07 - 2017-08-13
Amplification of the backbone (pSB1C3) and insert (Tyr-aaRS)
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- PCR Q5 Polymerase (no Master Mix)
- for 50 reaction
- 10 Reaction Buffer
- 5 2mM dNTPs
- 1 Template
- 0,5 High Fidelity DNA Polymerase
- 10,0 High GC Enhancer
- 18,5 ddest H2O
- 5,0 Primer
- pSB1C3 (from RuBisCo, ncAA team): ht, jk 65у
- aaRS (from Heidelberg) : hq, jk 65у (mistake! should be 58у, redone identically with 58у)
- digestion of the PCR products with Dpn1: 5 CutSmart Reaktionsbuffer and 1 Dpn1 per 50 PCR product, on 37у over night)
- agarose-gelelectrophhoresis, 1% (bands of the right size)
- No further use, because results of the sequencing which show that the integration of the incorporation of the Tyr-aaRS in pSB1C3 was already successful (30.06.2017)
Ligation of 2B2-2B5 and B1
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- Ligation protocol from the BioBrick Assembly
- Variation: incubated 1h at RT instead of 10min
characterisation of T7GFP revers
Investigators: Christina Drake
Aim of the experiment: preparation of KRX-competent cells
Procedure:
- heatschocktransformation of T7GFP and T7GFP revers in KRX
- 1%-agarose-TAE-gel
- result: PCR did work
- Gibson Assembly
- transformation via heat shock
Amplification of the backbone (pRS31) and insert (ori from pSB6A1, oK1.0) for Gibson assembly
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- PCR Q5 Polymerase (protocoll of 07.08.2017)
- pRS31: primer jb, jn 65у
- oK1: primer jl, jc 65у
- digestion with Dpn1 (protocoll of 07.08.2017)
- agarose-gelelectrophhoresis, 1%
- band around 1200 bp (oK1.1) / 2500 bp (pRS31), positive
Gibson Assembly and Trafo of the pRS31 and oK1.0
Investigators: Laura Schlueter
Aim of the experiment: aaRS plasmid
Procedure:
- agarose-gelelectrophhoresis, 1%
- purification from the gel with the Macherey-Nagel purification kit
- oK1.1: 22,5 ng/
- pRS32: 9,5 ng/
- Gibson Assembly Master Mix with:
- 4,1 of oK1.1: around 2480 bp 9,5 ng/
- 0,9 of pRS32: around 1250 bp 22,5 ng/
- Trafo via heatshock
getting positive clones for further work
Investigators: Yannic Kerkhoff
Aim of the experiment: heatshock transformation of assembled fragments F13 and NPA-RS gene synthesis
Procedure:
- standard heatshock protocol
- used own produced chemo competend DH5alpha
- streaked out on LB-plates with Cam
multiplication, verification and purification of the needed fragment F13: linearized ONBY-Part with removal of the ONBY-RS
Investigators: Yannic Kerkhoff
Aim of the experiment: Q5-PCR, gel and PCR-cleanUp of F13
Procedure:
- standard Q5-PCR protocol
- template: K1416000
- primer fwd: 17hl
- primer rev: 17mv
- annealing temperature: 63у
- extension time: 90 seconds
- standard PCR-cleanUp protocol
- 80,6 ng/
Assemble the fragments to get the composite Part BBa_P7:NPA-RS
Investigators: Yannic Kerkhoff
Aim of the experiment: Gibson assembly of F13 and NPA-RS gene synthesis
Procedure:
- standard Gibson Assembly protocol
getting positive clones for further work
Investigators: Yannic Kerkhoff
Aim of the experiment: heatshock transformation of assembled fragments F5,F1,F3
Procedure:
- standard heatshock protocol
- used own produced chemo competend DH5alpha
- streaked out on LB-plates with Cam
multiplication, verification and purification of the needed fragment F1: GFPLinker1
Investigators: Yannic Kerkhoff
Aim of the experiment: Q5-PCR, gel and PCR-cleanUp of F1
Procedure:
- standard Q5-PCR protocol
- template: BBa_E0400
- primer fwd: 17gk
- primer rev: 17gm
- annealing temperature: 58у
- extension time: 50 seconds
- standard PCR-cleanUp protocol
- 15,9 ng/
multiplication, verification and purification of the needed fragment F3: StrepLinker1
Investigators: Yannic Kerkhoff
Aim of the experiment: Q5-PCR, gel and PCR-cleanUp of F3
Procedure:
- standard Q5-PCR protocol
- template: BBa_KJ36848
- primer fwd: 17go
- primer rev: 17gq
- annealing temperature: 61у
- extension time: 30 seconds
- standard PCR-cleanUp protocol
- 17,9 ng/
Biobrickassembly
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
- BioBrick Assembly
- repeat digestion of T7-Terminator downstrampart
- ligate over night
Transformation of new plasmids
Investigators: Maximilian Edich
Aim of the experiment: Biobrick Construction with RuBisCo Parts
Procedure:
Primer annealing preparation
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system - Primer annealing test
Procedure:
- Both Primers (17jh; 17ji) were resuspended in 1x Composite Buffer
- Dilutions: 100 ֍, 10 ֍, 5 ֍, 2.5 ֍, 0.5 ֍
- OD 260 were measured to determine the real concentration
2017-08-14 - 2017-08-20
Screening for positive transformations containing the Biobrick BBa_P2:GLS2
Investigators: Yannic Kerkhoff
Aim of the experiment: GoTaq PCR of 4 clones
Procedure:
- standard GoTaq-protocol
- template: colonie pcr clones of GA_P1:GLS1
- primer fwd: Pr姩x_fwd
- primer rev: Suffix_rev
- annealing temperature: 56у
- extension time: 40 seconds
- positive clone 3
Primer annealing of 17jh & 17ji
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system - Primer annealing test
Procedure:
- Protocol for annealing oligonucleotides (sigmaaldrich)
- Eqimolar Primers were mixed (50 )
- Thermal profile (thermocycler)
- 95 у, 2 min
- Cool to 25 у over 45 min
- Cool to 4 у for temporary storage
Primer annealing of 17jl & 17jm
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system - Primer annealing test
Procedure:
- Both Primers were resuspended in ddH20 to a final concentration of 100 ֍
- HEPES annealing standard protocol
- Aqua annealing standard protocol
- Final volume: 20
- Agarose gel electrophoresis (2%)
- 60 V, 50 min
Native PAGE of annealed primers (17jl & 17jm)
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system - Primer annealing test
Procedure:
- Native DNA PAGE standard protocol
- tested samples:
- HEPES annealing (17jl & 17jm): 100 ֍, 10 ֍, 5 ֍, 2.5 ֍, 1 ֍, 0.5 ֍
- Aqua annealing (17jl & 17jm): 100 ֍, 10 ֍, 5 ֍, 2.5 ֍, 1 ֍, 0.5 ֍
- Variation: ~40 mA
2017-08-21 - 2017-08-27
Native PAGE of annealed primers (17jl & 17jm)
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system - Primer annealing test
Procedure:
- Native DNA PAGE standard protocol
- tested samples:
- HEPES annealing (17jl & 17jm): 100 ֍, 10 ֍, 5 ֍, 2.5 ֍, 1 ֍, 0.5 ֍
- Aqua annealing (17jl & 17jm): 100 ֍, 10 ֍, 5 ֍, 2.5 ֍, 1 ֍, 0.5 ֍
- Variation: 100 V, 1 h
Native PAGE of annealed primers (17jl & 17jm)
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system - Primer annealing test
Procedure:
- Native DNA PAGE standard protocol
- tested samples:
- HEPES annealing (17jl & 17jm): 100 ֍, 10 ֍, 5 ֍, 2.5 ֍, 1 ֍, 0.5 ֍
- Aqua annealing (17jl & 17jm): 100 ֍, 10 ֍, 5 ֍, 2.5 ֍, 1 ֍, 0.5 ֍
- Variation: 60 V, 2 h
Native Page of annealed primers (17jl & 17jm; 17jh & 17ji)
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system - Primer annealing test
Procedure:
- Native DNA PAGE standard protocol
- tested samples:
- HEPES annealing (17jl & 17jm): 0.5 ֍
- Aqua annealing (17jl & 17jm): 0.5 ֍
- Composite Buffer annealing (17jh & 17 jm): 0.5 ֍
- all Primers (ssDNA): 1 ֍
2017-08-28 - 2017-09-03
Native PAGE of annealed primers (HEPES annealing & Composite Buffer annealing) of the same concentration to test if all annealings have the same quality
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system - Primer annealing test
Procedure:
- all samples were diluted to a final concentration of 0.5 ֍
- Native DNA PAGE standard protocol
Restriction digest of control annealings (mutC)
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system
Procedure:
- Restriction Digest (MnlI) of aqua annealing sample: mutC (0.5 ֍)
- 2 MnlI
- 5 CutSmart
- 25 mutC dsDNA
- 18 nuclease-free H2O
- Incubation: 37 у, 1 h
- Inactivation: 20 min., 65 у
- Native DNA PAGE standard protocol
- Tested samples:
- digested mutC sample
- native mutC sample
- ssDNA primers (17jl & 17jm)
Restriction digest of aqua & HEPES annealing
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system
Procedure:
- Restriction Digest (MnlI) of aqua & HEPES annealing sample: mutC (0.5 ֍)
- 2 MnlI
- 5 CutSmart
- 25 mutC dsDNA
- 18 nuclease-free H2O
- Incubation: 37 у, 1 h
- Inactivation: 20 min., 65 у
- Native DNA PAGE standard protocol
- Tested samples:
- digested mutC sample (aqua & HEPES annealing)
- native mutC sample
- ssDNA primers (17jl & 17jm)
Aqua annealing of mutA, mutT, mutG and mutC
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system
Procedure:
- Aqua annealing standard protocol (final concentration: 0.5 ֍)
- mutA: 17jf & 17jg
- mutT: 17jj & 17jk
- mutG: 17jh & 17ji
- mutC: 17jl & 17jm
- final volume of each sample: 50
2017-09-04 - 2017-09-10
Restriction digest of control annealings (mutA, mutT, mutG, mutC) and aqua annealing of oligo2
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system
Procedure:
- Oligo2 annealing
- Aqua annealing standard protocol (final concentration: 0.5 ֍)
- Restricted samples:
- MnlI -> mutC, oligo2
- SapI -> mutG, oligo2
- BsaI -> mutT, oligo2
- EciI -> mutA, oligo2
- Restriction Digest:
- 1 Enzyme
- 5 CutSmart
- 25 mutC dsDNA
- 19 nuclease-free H2O
- Incubation: 37 у, 1 h
- Inactivation: 20 min., 65 у
- Native DNA PAGE standard protocol
2017-09-11 - 2017-09-17
Annealing, restriction digest and native PAGE of all samples
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system
Procedure:
- Aqua annealing standard protocol (final concentration: 0.5 ֍)
- mutA: 17jf & 17jg
- mutT: 17jj & 17jk
- mutG: 17jh & 17ji
- mutC: 17jl & 17jm
- oligo2: olgio2_sense & oligo2_antisense
- final volume of each sample: 50
- Restricted samples:
- MnlI -> mutC, oligo2
- SapI -> mutG, oligo2
- BsaI -> mutT, oligo2
- EciI -> mutA, oligo2
- Restriction Digest:
- 1 Enzyme
- 5 CutSmart
- 25 mutC dsDNA
- 19 nuclease-free H2O
- Incubation: 37 у, 1 h
- Inactivation: 20 min., 65 у
- Native DNA PAGE standard protocol
Annealing, restriction digest and native PAGE of all samples
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system
Procedure:
- Aqua annealing standard protocol (final concentration: 0.5 ֍)
- mutA: 17jf & 17jg
- mutT: 17jj & 17jk
- mutG: 17jh & 17ji
- mutC: 17jl & 17jm
- oligo2: olgio2_sense & oligo2_antisense
- final volume of each sample: 2x50
- Restricted samples:
- MnlI -> mutC
- SapI -> mutG, oligo2
- BsaI -> mutT
- EciI -> mutA
- Restriction Digest:
- 1 Enzyme
- 5 CutSmart
- 25 mutC dsDNA
- 19 nuclease-free H2O
- Incubation: 37 у, 1 h
- Inactivation: 20 min., 65 у
- Native DNA PAGE standard protocol
2017-09-18 - 2017-09-24
-Agarose gel electrophoresis (2%)
Investigators: Agarose, gel, electrophoresis, of, digested, mutA,, mutT,, mutG, &, mutC
Aim of the experiment: CMZ
Procedure:
- 60 V, 40 min
Annealing, restriction digest and native PAGE of all samples
Investigators: Camilla Maerz
Aim of the experiment: M.A.X restriction system
Procedure:
- Aqua annealing standard protocol (final concentration: 0.5 ֍)
- mutA: 17jf & 17jg
- mutT: 17jj & 17jk
- mutG: 17jh & 17ji
- mutC: 17jl & 17jm
- oligo2: olgio2_sense & oligo2_antisense
- final volume of each sample: 2x50
- Restricted samples:
- MnlI -> mutC
- SapI -> mutG, oligo2
- BsaI -> mutT
- EciI -> mutA
- Restriction Digest:
- 1 Enzyme
- 5 CutSmart
- 25 mutC dsDNA
- 19 nuclease-free H2O
- Incubation: 37 у, 1 h
- Inactivation: 20 min., 65 у
- Native DNA PAGE standard protocol
Colony PCR of pSB3K5_mRFP_link_ccdB and pSB1C3_PtNTT2(31-575)-GFP
Investigators: Camilla Maerz
Aim of the experiment: Construction of pSB1C3-PlacUV5_PtNTT2
Procedure:
- PCR
- Go Tag (Promega) protocol
- Primer: VR, VF2
- Danaturation: 56 у
- Elongation: 90 s & 180 s
- Agarose gel electrophoresis (1%)
- 100 V, 30 min
2017-09-25 - 2017-10-01
-Aqua annealing standard protocol (final concentration: 0.5 ֍)
Investigators: Aqua, annealing, of, mutA-1,, mutG-1,, mutC-1,, mutG-1, &, oligo1
Aim of the experiment: ??
Procedure:
- mutA-1: 17iv & 17iw
- mutT-1: 17jb & 17jc
- mutG-1: 17ix & 17iy
- mutC-1: 17jd & 17jc
- oligo1: olgio1_sense & oligo1_antisense
- final volume: 50
2017-10-02 - 2017-10-08
UBP-PCR with TiTaq
Investigators: Camilla Maerz
Aim of the experiment: PCR with UBP
Procedure:
- PCR
- PCR-UBP standard protocol (TiTaq)
- samples:
- Ligation of: mutA, mutT, mutG, mutC and oligo 2 (1 ng/)
- Primer: 17vt & 17vu
- Primer annealing: 56 у
- Elongation: 20 s
- PCR and DNA purification kit (Macherey-Nagel)
- Nucleo spin PCR and Monarch® PCR & DNA Clean-up protocol
- Restriction Digest
- 1 Enzyme
- 5 CutSmart
- 25 mutC dsDNA
- 19 nuclease-free H2O
- Incubation: 37 у, 1 h
- Inactivation: 20 min., 65 у
- Restricted samples:
- MnlI -> mutC
- SapI -> mutG
- BsaI -> mutT
- EciI -> mutA
- EciI, BsaI, SapI, MnlI -> oligo2
- Variation: oligo2 was digested with 0.5 of each enzyme
- Agarose gel electrophoresis (2 %)
- 100 V, 20 min
UBP-PCR with GoTaq G2 and TiTaq
Investigators: Camilla Maerz
Aim of the experiment: PCR with UBP
Procedure:
- PCR with TiTaq:
- PCR-UBP standard protocol (TiTaq)
- samples:
- Ligation of: mutA, mutT, mutG, mutC and oligo 2 (5 ng/)
- Primer: 17 vt & 17 vu
- Primer annealing: 56 у
- Elongation: 20 s
- PCR with GoTaq:
- PCR-UBP standard protocol (TiTaq)
- samples:
- Ligation of: mutA, mutT, mutG and mutC (5 ng/)
- Primer: VR & VF2
- Primer annealing: 56 у
- Elongation: 20 s
- PCR with GoTaq:
- PCR-UBP standard protocol (TiTaq)
- samples:
- Ligation of: mutA, mutT, mutG, mutC and oligo2 (5 ng/)
- Primer: 17 vt & 17 vu
- Primer annealing: 56 у
- Elongation: 20 s
Restriction digest of ligated oligo2
Investigators: Camilla Maerz
Aim of the experiment: PCR with UBP
Procedure:
- Restriction Digest
- 5 CutSmart
- 30 ligated oligo2 DNA
- 2 EcoRV
- filled up to final volume 50 with ddH20
- Incubation: 120 min, 37 у
- Inactivation: 20 min, 65 у
2917-06-14 - 2917-06-20
Duplicate the KRX-e.coli
Investigators: Christina Drake, Denise Kerkhoff
Aim of the experiment: Plated out: KRX-e.coli as glycostocsolution
Procedure:
- plated out on kanamycin
- incubation at 37°C
