Team:NYMU-Taipei/Project/Lab Note
From 2009.igem.org
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- | + | == Experiment of oscillator biobrick parts == | |
- | + | ||
- | = | + | {| border="1" |
+ | | 1 || BBa_C0051 '''cI repressor from E. coli phage lambda (+LVA)''' | ||
+ | |- | ||
+ | | 2 || BBa_K116602 '''CII coding region from λ phage''' | ||
+ | |- | ||
+ | | 3 || BBa_C0040 '''tetracycline repressor from transposon Tn10 (+LVA)''' | ||
+ | |- | ||
+ | | 4 || BBa_C0074 '''penI repressor from Bacillus licheniformis (+LVA)''' | ||
+ | |- | ||
+ | | 5 || BBa_C0072 '''mnt repressor (strong) from Salmonella phage P22 (+LVA)''' | ||
+ | |- | ||
+ | | 6 || BBa_C0073 '''mnt repressor (weak) from Salmonella phage P22 (+LVA)''' | ||
+ | |- | ||
+ | | 7 || BBa_E0040 '''green fluorescent protein''' | ||
+ | |- | ||
+ | | t || BBa_B0015 '''Terminator''' | ||
+ | |- | ||
+ | | A || BBa_R0040 '''TetR repressible promoter ''' | ||
+ | |- | ||
+ | | P || BBa_R0074 '''Promoter (PenI regulated) ''' | ||
+ | |- | ||
+ | | L || BBa_R0010 '''promoter (lacI regulated) ''' | ||
+ | |- | ||
+ | | M || BBa_R0073 '''Promoter (Mnt regulated) ''' | ||
+ | |- | ||
+ | | C || BBa_R0051 '''promoter (lambda cI regulated) ''' | ||
+ | |- | ||
+ | | pCI || BBa_R1051 '''Promoter, Standard (lambda cI regulated)''' | ||
+ | |- | ||
+ | | p22 || BBa_R0053 '''Promoter (p22 cII regulated) ''' | ||
+ | |- | ||
+ | | pLuxR || BBa_R0062 '''Promoter (luxR & HSL regulated -- lux pR) ''' | ||
+ | |- | ||
+ | | pLasR || BBa_R0079 '''Promoter (LasR & PAI regulated) ''' | ||
+ | |- | ||
+ | | E || BBa_K116603 '''pRE promoter from λ phage ''' | ||
- | + | |} | |
- | |||
- | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 07 24 oscillator part.png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | |
+ | 2% agarose, 90V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: BBa_R0051 pCI|287bp (49+238)|238bp|m|= | ||
+ | |2: BBa_C0051 CI lam|988bp (750+238)|238bp|w|= | ||
+ | |3: BBa_C0040 TetR|838bp (660+238)|238bp|w|= | ||
+ | |4: BBa_B0034 RBS|250bp (12+238)|238bp|w|= | ||
+ | |5: BBa_j13002 pTetR|302bp (74+238)|238bp|f|= | ||
+ | |6: BBa_B0015 Term|445bp (129+316)|316bp|w|= | ||
+ | |7: BBa_K116602 CII|532bp (294+238)|238bp|w|= | ||
+ | |8: BBa_K116603 pRE|286bp (48+238)|238bp|w|= | ||
+ | |9: Positive Control BBa_E0240|1114bp (876+238)|238bp|w|= | ||
+ | |10: Negative Control|0bp||w|= | ||
+ | |11: marker 100bp|||n}} }} | ||
- | == | + | == Experiment of oscillator biobrick parts (2)== |
- | + | ||
- | === | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 07 27 oscillator part(2).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= |
- | < | + | 2% agarose, 90V, 30min |
- | + | {{:Team:NYMU-Taipei/GELC|= | |
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: BBa_R0040 pTetR|292bp (54+238)|238bp|w|= | ||
+ | |2: BBa_E0840|1116bp (878+238)|238bp|w|= | ||
+ | |3: CII<Term(from jesse)|669bp (294+8+129+238)|532bp (294+238)|f|= | ||
+ | |4: Positive Control BBa_E0240|1114bp (876+238)|238bp|w|= | ||
+ | |5: Negative Control||Contamination ~300bp|f|= | ||
+ | |6: -|-|-|n|= | ||
+ | |7-8: BBa_B0015 Term (gel extraction)|155bp (129+26)||w|= | ||
+ | |9: marker 100bp|||n}} }} | ||
- | + | == Experiment of oscillator biobrick parts (3)== | |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 07 29 oscillator part(3).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 90V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: CII<Term|669bp (294+8+129+238)|532bp (294+238)|w|= | ||
+ | |2: CI lam<Term|1125bp (750+8+129+238)|988bp (750+238)|w|= | ||
+ | |3: TetR<Term|1035bp (660+8+129+238)|898bp (660+238)|f|= | ||
+ | |4: BBa_R0051 pCI|287bp (49+238)|238bp|m|= | ||
+ | |5: BBa_j13002 pTetR+RBS|312bp (74+238)|238bp|w|= | ||
+ | |6: Positive Control BBa_E0240|1114bp (876+238)|238bp|w|= | ||
+ | |7: Negative Control|0bp|Contamination ~300&700bp,|f|= | ||
+ | |8: -|-|-|n|= | ||
+ | |9-10: BBa_E0840 (Gel extraction)|878bp||w|= | ||
+ | |11: marker 100bp|||n}} }} | ||
+ | 4: Inconclusive. | ||
- | {{:Team:NYMU-Taipei/ | + | == Experiment of oscillator biobrick parts (4)== |
- | | | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 07 31 oscillator part(4).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= |
- | | | + | 2% agarose, 90V, 30min |
- | | | + | {{:Team:NYMU-Taipei/GELC|= |
- | | | + | |0: marker 1kb+100bp|||n|= |
+ | |1: BBa_R0074 pPenI|315bp (77+238)|238bp|w|= | ||
+ | |2-6: BBa_C0074 PenI|739bp (423+316)|316bp|w|= | ||
+ | |7-11: BBa_R0073 pMnt|383bp (67+316)|316bp|m|= | ||
+ | |12-16: BBa_C0072 Mnt (Strong)|604bp (288+316)|316bp|w|= | ||
+ | |17-21: BBa_C0073 Mnt (Weak)|604bp (288+316)|316bp|w|= | ||
+ | |22: Positive Control BBa_E0240|1114bp (876+238)|238bp|w|= | ||
+ | |23: Negative Control|0bp|Contamination|f|= | ||
+ | |24: marker 100bp|||n}} | ||
+ | The result for lanes 7-11 look weird, but it could be because of the gel. A rerun will be done.}} | ||
- | == | + | == Experiment of oscillator biobrick parts (5)== |
- | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 07 31 oscillator part(5).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | |
- | + | 2% agarose, 90V, 30min | |
- | + | {{:Team:NYMU-Taipei/GELC|= | |
- | + | |0: marker 1kb+100bp|||n|= | |
- | + | |1-2: TetR<Term (Gel extraction)|821bp (660+8+129+24)|684bp (660+24)|f|= | |
+ | |4-5: CII<Term (Gel extraction)|455bp (294+8+129+24)|318bp (294+24)|w|= | ||
+ | |7-9: CI<Term (Gel extraction)|911bp (750+8+129+24)|774bp (750+24)|w|= | ||
+ | |10: marker 100bp|||n}} }} | ||
- | == | + | == Experiment of oscillator biobrick parts (6)== |
- | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 03 oscillator part(6).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | |
- | + | 2% agarose, 90V, 30min | |
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: BBa_R0074 pPenI|315bp (77+238)|238bp|w|= | ||
+ | |2: BBa_C0074 PenI|739bp (423+316)|316bp|w|= | ||
+ | |3: BBa_R0073 pMnt|383bp (67+316)|316bp|w|= | ||
+ | |4: BBa_C0072 Mnt (Strong)|604bp (288+316)|316bp|w|= | ||
+ | |5: BBa_C0073 Mnt (Weak)|604bp (288+316)|316bp|w|= | ||
+ | |6: Positive Control BBa_E0240|1114bp (876+238)|238bp|w|= | ||
+ | |7: Negative Control|0bp|Contamination|f|= | ||
+ | |8: marker 100bp|||n}} }} | ||
+ | == Experiment of oscillator biobrick parts (7)== | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 03 oscillator part(7).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 90V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: RBS + CII + Term|687bp |250bp|f|= | ||
+ | |2: RBS + CI lam + Term|1143bp |250bp|f|= | ||
+ | |3: RBS + TetR + Term|1053bp |250bp|f|= | ||
+ | |4: pCI(plate from 090729)|287bp |238bp|m|= | ||
+ | |5: E0840|604bp (288+316)|316bp|w|= | ||
+ | |6: pCI(plasmid from 090730)|287bp |238bp|f|= | ||
+ | |7: Positive Control BBa_E0240|1114bp (876+238)|238bp|w|= | ||
+ | |8: Negative Control|0bp|Contamination~300bp|f|= | ||
+ | |9: marker 1kb+100bp|||n}} }} | ||
- | == | + | == Experiment of oscillator biobrick parts (8)== |
- | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 04 oscillator part(8).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | |
- | + | 2% agarose, 90V, 30min | |
- | + | {{:Team:NYMU-Taipei/GELC|= | |
- | + | |0: marker 1kb+100bp|||n|= | |
- | + | |1: BBa_I13504 r7t|1113bp |250bp|w|= | |
- | + | |2: BBa_I13522 Ar7t|1176bp |292bp|w|= | |
- | + | |3: BBa_I13401 7t|1095bp |958bp|w|= | |
- | + | |4: BBa_R0051 pCI|287bp |238bp|m|= | |
- | + | |5: pTetR<E0240|1176bp |292bp|w|= | |
- | + | |6: PenI<Term|876bp |739bp|f|= | |
- | + | |7: Mnt (Strong)<Term|741bp |604bp|m|= | |
+ | |8: Mnt (Weak)<Term|741bp |604bp|f|= | ||
+ | |9: Positive Control BBa_E0240|1114bp (876+238)|238bp|w|= | ||
+ | |10: Negative Control|0bp|Contamination~300bp|f|= | ||
+ | |11: marker 100bp|||n}} }} | ||
+ | == Experiment of oscillator biobrick parts (9) Gel Extraction == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 04 oscillator part(9).png||c= | ||
+ | 2% agarose, 90V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: B0034+CII+Term r2t|475bp |38bp|f|= | ||
+ | |2: B0034+CII+Term r2t|475bp |38bp|f|= | ||
+ | |3: B0034+CII+Term r2t|475bp |38bp|f|= | ||
+ | |4: B0034+CI lam+Term r1t|931bp |38bp|f|= | ||
+ | |5: B0034+CI lam+Term r1t|931bp |38bp|f|= | ||
+ | |6: B0034+CI lam+Term r1t|931bp |38bp|f|= | ||
+ | |7: B0034+Tet R+Term r3t|841bp |38bp|f|= | ||
+ | |8: B0034+Tet R+Term r3t|841bp |38bp|f|= | ||
+ | |9: B0034+Tet R+Term r3t|841bp |38bp|f|= | ||
+ | |10: marker 100bp|||n}} }} | ||
- | == | + | == Experiment of oscillator biobrick parts (10) (Gel Extraction)== |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 05 oscillator part(10).png||c= | ||
+ | 2% agarose, 90V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: BBa_I13504 r7t|901bp |0bp|w|= | ||
+ | |2: BBa_I13401 7t|881bp |0bp|w|= | ||
+ | |3: PenI+Term|584bp|447bp|f|= | ||
+ | |4: Mnt (Strong)+Term 5t|449bp |312bp|f|= | ||
+ | |5: Mnt (Weak)+Term 6t|449bp |312bp|f|= | ||
+ | |6: TetR+Term 3t|821bp |684bp|f|= | ||
+ | |7: marker 1kb+100bp|||n}} }} | ||
- | + | == Experiment of oscillator biobrick parts (11)== | |
- | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 06 oscillator part(11).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | |
- | + | 2% agarose, 90V, 30min | |
- | + | {{:Team:NYMU-Taipei/GELC|= | |
- | + | |0: marker 1kb+100bp|||n|= | |
- | + | |1: marker 1kb|||n|= | |
- | + | |2: C|287bp |238bp|w|= | |
- | + | |3: M|383bp |316bp|w|= | |
- | + | |4: 3t|1035bp |898bp|f|= | |
+ | |5: 4t|876bp |739bp|f|= | ||
+ | |6: 5t|741bp |604bp|m|= | ||
+ | |7: 6t|741bp |604bp|f|= | ||
+ | |8: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |9: Negative Control |0bp |Contamination~300|f|= | ||
+ | |10: |bp |bp|n|= | ||
+ | |11: |bp |bp|n|= | ||
+ | |12: r<1t|1143bp |250bp|f|= | ||
+ | |13: r<2t|687bp |250bp|f|= | ||
+ | |14: r<7t|1113bp |250bp|f|= | ||
+ | |15: 3<t|1035bp |898bp|f|= | ||
+ | |16: 5<t|741bp |604bp|f|= | ||
+ | |17: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |18: Negative Control |0bp |Contamination~|f|= | ||
+ | |19: marker 1kb|||n|= | ||
+ | |20: marker 100bp|||n}} }} | ||
- | |||
+ | == Experiment of oscillator biobrick parts (12)== | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 11 oscillator part(12).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 90V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Lr7t|1321bp |438bp|f|= | ||
+ | |2: Lr7t|1321bp |438bp|w|= | ||
+ | |3: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |4: r1t|1143bp |250bp|w|= | ||
+ | |5: r1t|1143bp |250bp|w|= | ||
+ | |6: r1t|1143bp |250bp|w|= | ||
+ | |7: r1t|1143bp |250bp|f|= | ||
+ | |8: r1t|1143bp |250bp|w|= | ||
+ | |9: r1t|1143bp |250bp|f|= | ||
+ | |10: r1t|1143bp |250bp|w|= | ||
+ | |11: r1t|1143bp |250bp|w|= | ||
+ | |12: r2t|687bp |250bp|w|= | ||
+ | |13: r2t|687bp |250bp|f|= | ||
+ | |14: r2t|687bp |250bp|w|= | ||
+ | |15: r2t|687bp |250bp|w|= | ||
+ | |16: r2t|687bp |250bp|w|= | ||
+ | |17: r2t|687bp |250bp|w|= | ||
+ | |18: r2t|687bp |250bp|w|= | ||
+ | |19: r2t|687bp |250bp|w|= | ||
+ | |20: r2t|687bp |250bp|w|= | ||
+ | |21: r2t|687bp |250bp|w|= | ||
+ | |22: r2t|687bp |250bp|w|= | ||
+ | |23: Negative Control |0bp ||w|= | ||
+ | |24: marker 1kb+100bp|||n}} }} | ||
- | + | == Experiment of oscillator biobrick parts (13) 2009/08/13== | |
- | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 13 oscillator part(13).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | |
- | + | 2% agarose, 90V, 38min | |
- | + | {{:Team:NYMU-Taipei/GELC|= | |
- | + | |0: marker 1kb+100bp|||n|= | |
- | + | |1: 3t|1035bp |898bp|m|= | |
- | + | |2: 3t|1035bp |898bp|m|= | |
- | + | |3: 3t|1035bp |898bp|f|= | |
- | + | |4: 3t|1035bp |898bp|f|= | |
- | + | |5: 3t|1035bp |898bp|m|= | |
- | + | |6: 4t|876bp |739bp|w|= | |
- | + | |7: 4t|876bp |739bp|w|= | |
- | + | |8: 4t|876bp |739bp|f|= | |
- | + | |9: 4t|876bp |739bp|f|= | |
- | + | |10: 4t|876bp |739bp|w|= | |
- | + | |11: 5t|741bp |604bp|f|= | |
- | + | |12: 5t|741bp |604bp|f|= | |
+ | |13: 5t|741bp |604bp|f|= | ||
+ | |14: 5t|741bp |604bp|f|= | ||
+ | |15: 5t|741bp |604bp|f|= | ||
+ | |16: 6t|741bp |604bp|m|= | ||
+ | |17: 6t|741bp |604bp|m|= | ||
+ | |18: 6t|741bp |604bp|m|= | ||
+ | |19: 6t|741bp |604bp|m|= | ||
+ | |20: 6t|741bp |604bp|m|= | ||
+ | |21: 1t|1125bp |988bp|w|= | ||
+ | |22: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |23: Negative Control |0bp ||w|= | ||
+ | |24: marker 1kb+100bp|||n}} }} | ||
- | + | == Experiment of oscillator biobrick parts (14) (Gel Extraction) 2009/08/13== | |
- | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 13 oscillator part(14).png||c= | |
- | + | 2% agarose, 90V, 36min | |
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: r1t|929bp ||w|= | ||
+ | |2: r1t|929bp ||w|= | ||
+ | |3: marker 1kb+100bp|||n|= | ||
+ | |4: r2t|473bp ||w|= | ||
+ | |5: r2t|473bp ||w}} }} | ||
- | == | + | == Experiment of oscillator biobrick parts (15) 2009/08/15 == |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 15 oscillator part(15).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Ar7t|1176bp |292bp|w|= | ||
+ | |2: Ar7t|1176bp |292bp|w|= | ||
+ | |3: Ar7t|1176bp |292bp|w|= | ||
+ | |4: Ar2t|749bp |292bp|f|= | ||
+ | |5: Pr7t|1199bp |315bp|f|= | ||
+ | |6: Lr7t|1322bp |438bp|w|= | ||
+ | |7: Lr7t|1322bp |438bp|w|= | ||
+ | |8: Lr7t|1322bp |438bp|w|= | ||
+ | |9: Lr7t|1322bp |438bp|w|= | ||
+ | |10: Cr7t|1171bp |287bp|f|= | ||
+ | |11: Cr7t|1171bp |287bp|f|= | ||
+ | |12: Cr7t|1171bp |287bp|f|= | ||
+ | |13: Cr7t|1171bp |287bp|f|= | ||
+ | |14: Er7t|1170bp |286bp|f|= | ||
+ | |15: Er7t|1170bp |286bp|w|= | ||
+ | |16: Er7t|1170bp |286bp|f|= | ||
+ | |17: Er7t|1170bp |286bp|w|= | ||
+ | |18: Er7t|1170bp |286bp|w|= | ||
+ | |19: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |23: Negative Control |0bp ||w|= | ||
+ | |24: marker 1kb+100bp|||n}} }} | ||
- | + | == Experiment of oscillator biobrick parts (16) (Gel Extraction) 2009/08/15== | |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 15 oscillator part(16).png||c= | ||
+ | 2% agarose, 100V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: 3t|821bp |684bp |w|= | ||
+ | |2: 3t|821bp |684bp |w|= | ||
+ | |3: 3t|821bp |684bp |w|= | ||
+ | |4: 4t|584bp |447bp |f|= | ||
+ | |5: 4t|584bp |447bp |f|= | ||
+ | |6: 4t|584bp |447bp |f|= | ||
+ | |7: marker 1kb+100bp|||n}} }} | ||
- | + | == Experiment of oscillator biobrick parts (17) 2009/08/16 == | |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 16 oscillator part(17).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: pH sensor|512bp ||f|= | ||
+ | |2: pH sensor|512bp ||f|= | ||
+ | |3: pH sensor|512bp ||f|= | ||
+ | |4: pH sensor|512bp ||f|= | ||
+ | |5: r3t|1053bp |250bp |f|= | ||
+ | |6: r3t|1053bp |250bp |f|= | ||
+ | |7: r3t|1053bp |250bp |f|= | ||
+ | |8: r3t|1053bp |250bp |w|= | ||
+ | |9: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |10: Negative Control |0bp ||w|= | ||
+ | |11: marker 1kb+100bp|||n}} }} | ||
- | |||
- | === | + | == Experiment of oscillator biobrick parts (18) (digestion) 2009/08/17== |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 17 oscillator part(18).png||c= | ||
+ | 2% agarose, 100V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb|||n|= | ||
+ | |1: marker 100bp|||n|= | ||
+ | |2: Cr7t(XN)|311,2701bp|253bp,2701bp|f|= | ||
+ | |3: Er7t(NP)|36,274,2701bp|253bp,2701bp|w|= | ||
+ | |4: pH Sensor Plasmid #1 Amplify 1-2 (XP)|296,2057bp|1180,2057bp|f|= | ||
+ | |5: pH Sensor Plasmid #1 Amplify 3-4 (XP)|296,2057bp|1180,2057bp|f|= | ||
+ | |6: pH Sensor Plasmid #1 Amplify 1-2 (XN)|2353bp|536,2701bp|f|= | ||
+ | |6: pH Sensor Plasmid #1 Amplify 3-4 (XN)|2353bp|536,2701bp|f|= | ||
+ | |7: marker 1kb+100bp|||n}} | ||
+ | Comments | ||
+ | * Colony's of lanes 4-7 came from the same plate. Because this part was left over from last year, we didn't know if this plasmid contained K116001 or K116002. This gel's digestion results say K116002. | ||
- | + | }} | |
- | + | == Experiment of oscillator biobrick parts (19) (Gel Extraction) 2009/08/17== | |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 17 oscillator part(19).png||c= | ||
+ | 2% agarose, 100V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 100bp|||n|= | ||
+ | |1: marker 1kb|||n|= | ||
+ | |2: Er7t|958bp |74bp |w|= | ||
+ | |3: Er7t|958bp |74bp |w|= | ||
+ | |4: Er7t|958bp |74bp |w|= | ||
+ | |5: Cr7t|959bp |75bp |f|= | ||
+ | |6: Cr7t|959bp |75bp |f|= | ||
+ | |7: Cr7t|959bp |75bp |f|= | ||
+ | |8: marker 1kb|||n|= | ||
+ | |9: marker 100bp|||n}} }} | ||
- | |||
- | === | + | == Experiment of oscillator biobrick parts (20) 2009/08/18 == |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 18 oscillator part(20).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 28min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: AR7t|1175bp |292bp |w|= | ||
+ | |2: AR7t|1175bp |292bp |w|= | ||
+ | |3: PR7t|1198bp |315bp |m|= | ||
+ | |4: PR7t|1198bp |315bp |f|= | ||
+ | |5: CR7t|1170bp |287bp |f|= | ||
+ | |6: CR7t|1170bp |287bp |f|= | ||
+ | |7: pMnt|383bp |316bp |m|= | ||
+ | |8: CI lam|988bp |238bp |m|= | ||
+ | |9: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |10: Negative Control |0bp |contamination~700bp|f|= | ||
+ | |11: marker 1kb+100bp|||n}} }} | ||
- | + | == Experiment of oscillator biobrick parts (21) (Gel Extraction) 2009/08/18== | |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 18 oscillator part(21).png||c= | ||
+ | 2% agarose, 100V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: r3t(XP)|841bp |38bp |w|= | ||
+ | |2: r3t(XP)|841bp |38bp |w|= | ||
+ | |3: r3t(XP)|841bp |38bp |w|= | ||
+ | |4: term(XP)|155bp |445bp |w|= | ||
+ | |5: term(XP)|155bp |445bp |w|= | ||
+ | |6: term(XP)|155bp |445bp |w|= | ||
+ | |7: marker 1kb+100bp|||n}} }} | ||
- | + | == Experiment of oscillator biobrick parts (22) 2009/08/19 == | |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 19 oscillator part(22).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|60s|300s|rp=VR|fp=VF2|polName=pfu|pol=0.5|ddH20=39.5}}|c= | ||
+ | 2% agarose, 100V, 28min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: nhaA|274bp |0bp |w|= | ||
+ | |2: Positive Control Term|445bp |316bp|w|= | ||
+ | |3: Negative Control |0bp ||w|= | ||
+ | |4: marker 1kb+100bp|||n}} | ||
+ | PCR of nhaA using this protocol worked. | ||
- | + | }} | |
- | + | == Experiment of oscillator biobrick parts (23) 2009/08/19 == | |
- | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 19 oscillator part(23).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | |
+ | 2% agarose, 100V, 28min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: 4<t|876bp |739bp |m|= | ||
+ | |2: 4<t|876bp |739bp |m|= | ||
+ | |3: 4<t|876bp |739bp |m|= | ||
+ | |4: 4<t|876bp |739bp |m|= | ||
+ | |5: 5<t|741bp |604bp |f|= | ||
+ | |6: 5<t|741bp |604bp |f|= | ||
+ | |7: 5<t|741bp |604bp |f|= | ||
+ | |8: 5<t|741bp |604bp |f|= | ||
+ | |9: 6<t|741bp |604bp |m|= | ||
+ | |10: 6<t|741bp |604bp |m|= | ||
+ | |11: 6<t|741bp |604bp |m|= | ||
+ | |12: 6<t|741bp |604bp |m|= | ||
+ | |13: M<R7t|1267bp |383bp |f|= | ||
+ | |14: M<R7t|1267bp |383bp |f|= | ||
+ | |15: M<r7t|1267bp |383bp |f|= | ||
+ | |16: M<r7t|1267bp |383bp |f|= | ||
+ | |17: M|383bp |316bp |w|= | ||
+ | |18: P|315bp |238bp |w|= | ||
+ | |19: 1|988bp |238bp |m|= | ||
+ | |20: 5|604bp |316bp |m|= | ||
+ | |21: 6|604bp |316bp |m|= | ||
+ | |22: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |23: Negative Control |0bp |contamination~300,1100bp|f|= | ||
+ | |24: marker 1kb+100bp|||n}} }} | ||
- | + | == Experiment of oscillator biobrick parts (24) 2009/08/20 == | |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 20 oscillator part(24).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 27min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: nhaA -->(l)|512bp |238bp |w|= | ||
+ | |2: A<r2t|749bp |292bp |f|= | ||
+ | |3: E<r3t|1109bp |286bp |f|= | ||
+ | |4: E<r3t|1109bp |286bp |f|= | ||
+ | |5: E<r3t|1109bp |286bp |f|= | ||
+ | |6: 4t|876bp |739bp |f|= | ||
+ | |7: 5t|741bp |604bp |f|= | ||
+ | |8: 6t|741bp |604bp |f|= | ||
+ | |9: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |10: Negative Control |0bp ||w|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
+ | Comments: | ||
+ | * Next time, for the failed ligations, revert back to using old enzymes and redo. Maybe it's something to do with not being familiar enough with the new brands. | ||
+ | * Ligating digested PCR product nhaA(XP) onto an empty pSB1A2 plasmid (obtained from extracting it from digesting E0240(XP)) worked. | ||
+ | }} | ||
- | |||
- | == Experiment | + | == Experiment of oscillator biobrick parts (25) 2009/08/21 == |
- | == | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 21 oscillator part(25).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= |
- | + | 2% agarose, 100V, 28min | |
- | + | {{:Team:NYMU-Taipei/GELC|= | |
- | + | |0: marker 1kb+100bp|||n|= | |
- | + | |1: E<r3t-->(l)|1109bp |286bp |w|= | |
- | + | |2: E<r3t|1109bp |286bp |f|= | |
- | + | |3: E<r3t|1109bp |286bp |f|= | |
- | + | |4: E<r3t|1109bp |286bp |f|= | |
- | + | |5: E<r3t|1109bp |286bp |f|= | |
+ | |6: E<r3t|1109bp |286bp |f|= | ||
+ | |7: E<r3t|1109bp |286bp |f|= | ||
+ | |8: E<r3t|1109bp |286bp |f|= | ||
+ | |9: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |10: Negative Control |0bp |contamination~700,1100,1400|f|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
- | + | Comments: liquid incubation of number 1}} | |
- | + | ||
- | |||
- | |||
- | ==== | + | == Experiment of oscillator biobrick parts (26) 2009/08/22 == |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 22 oscillator part(26).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 28min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: P<r3t|1138bp |315bp |f|= | ||
+ | |2: P<r3t|1138bp |315bp |f|= | ||
+ | |3: P<r3t|1138bp |315bp |f|= | ||
+ | |4: P<r3t|1138bp |315bp |f|= | ||
+ | |5: 4<t|876bp |739bp |f|= | ||
+ | |6: 4<t|876bp |739bp |f|= | ||
+ | |7: 4<t|876bp |739bp |w|= | ||
+ | |8: 4<t-->(4)|876bp |739bp |w|= | ||
+ | |9: Positive Control E0240|1113bp |250bp|w|= | ||
+ | |10: Negative Control |0bp |contamination~700|f|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
+ | Comments: | ||
+ | *4t in lane 5 seems strange. It is not correct,but not fail either. Lane 7 and 8 are correct. They could do liquid incubation. | ||
- | + | *There are no colony on the yesterday's plate Ar2t, so there is no need to do colony PCR. | |
- | + | ||
- | + | ||
- | + | *Ligation&Transformation: Ar7t、Pr7t、Lr7t(33.3uL competent cell each) | |
- | + | ||
- | + | ||
- | + | }} | |
- | + | ||
- | + | ||
- | + | == Experiment of oscillator biobrick parts (27) 2009/08/23 colony PCR== | |
- | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 23 oscillator part(27).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | |
- | |} | + | 2% agarose, 100V, 28min |
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: A<r7t-->(1)|1176bp |292bp |w|= | ||
+ | |2: A<r7t|1176bp |292bp |w|= | ||
+ | |3: P<r7t-->(2)|1199bp |315bp |w|= | ||
+ | |4: P<r7t|1199bp |315bp |w|= | ||
+ | |5: L<r7t-->(3)|1322bp |438bp |w|= | ||
+ | |6: L<r7t|1322bp |438bp |w|= | ||
+ | |7: P<r3t|1138bp |315bp |f|= | ||
+ | |8: P<r3t|1138bp |315bp |f|= | ||
+ | |9: Positive Control E0240|1113bp |250bp|w|= | ||
+ | |10: Negative Control |0bp ||w|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
- | + | Comments: | |
- | + | *all the colonies that are transformed yesterday are all correct. Pr3t is from the checking plate 090821. | |
+ | *haven't done the liquid incubation yet, should I do the liquid? | ||
+ | *Lr7t is green enough to be identified. Ar7t and Pr7t are not sure enough for me to identify. | ||
- | + | *'''r7t''' is BBa_I13504 from Biobrick, not the ligation from r<7t. | |
- | + | *Today's transformation : | |
+ | **Ar<2t | ||
+ | **Ar<7t | ||
+ | *'''Ar''' is BBa_J13002 from Biobrick. | ||
+ | }} | ||
- | + | == Experiment of oscillator biobrick parts (28) 2009/08/23 testing the reheating gel == | |
- | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 23 oscillator part(28).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | |
+ | 2% agarose, 100V, 28min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: r1t|1176bp |292bp |w|= | ||
+ | |2: CI lam|988bp |238bp |m|= | ||
+ | |3: pMnt|1199bp |315bp |w|= | ||
+ | |4: unknown|bp |bp |f|= | ||
+ | |5: unknown|bp |bp |f|= | ||
+ | |6: unknown|bp |bp |f|= | ||
+ | |7: marker 1kb+100bp|||n}} | ||
- | + | Comments: | |
+ | * This gel is made by many pieces of gel and be reheat once. The result seems that this gel could be use to check DNA length, not suitable for gel extraction. | ||
- | + | * CI lam is from the old PCR tube. The result is not that reliable since it is not fresh enough. But the result is strange because it is not success or failure either. | |
- | + | *pMnt seems to be right since that the right marker is upper than th left one, so the length is not sure. | |
- | + | ||
- | + | }} | |
- | + | == Experiment of oscillator biobrick parts (29) 2009/08/26 == | |
- | |} | + | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 26 oscillator part(29).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= |
+ | 2% agarose, 100V, 29min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Pr3t|1138bp |315bp |f|= | ||
+ | |2: Pr3t|1138bp |315bp |m|= | ||
+ | |3: Pr3t|1138bp |315bp |f|= | ||
+ | |4: Pr3t|1138bp |315bp |f|= | ||
+ | |5: Pr3t|1138bp |315bp |f|= | ||
+ | |6: Pr3t|1138bp |315bp |f|= | ||
+ | |7: Pr3t|1138bp |315bp |f|= | ||
+ | |8: Pr3t|1138bp |315bp |f|= | ||
+ | |9: Positive Control E0240|1113bp |250bp|w|= | ||
+ | |10: Negative Control |0bp |Contamination~1400bp|f|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
- | === '' | + | Comments: |
+ | |||
+ | *It is not that correct since those colony have not 100% correct. | ||
+ | *Pr3t in lane 2 seems to be correct in the upper band, while it also has the wrong length band. | ||
+ | |||
+ | |||
+ | }} | ||
+ | == Experiment of oscillator biobrick parts (29) 2009/08/27 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 27 oscillator part(30).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 29min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Pr3t|1138bp |315bp |f|= | ||
+ | |2: Pr3t|1138bp |315bp |f|= | ||
+ | |3: Pr3t|1138bp |315bp |f|= | ||
+ | |4: Pr3t|1138bp |315bp |f|= | ||
+ | |5: Pr3t|1138bp |315bp |f|= | ||
+ | |6: nhaA+ E0240|1396bp |512bp |f|= | ||
+ | |7: nhaA+ E0240|1396bp |512bp |f|= | ||
+ | |8: nhaA+ E0240|1396bp |512bp |f|= | ||
+ | |9: Positive Control E0240|1113bp |250bp|w|= | ||
+ | |10: Negative Control |0bp |Contamination~1400bp|f|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
+ | |||
+ | Comment: | ||
+ | |||
+ | *all of those bands are fail. It means that nhaA+E0240 didn't ligate well. | ||
+ | |||
+ | *DO the ligation again? | ||
+ | |||
+ | |||
+ | |||
+ | }} | ||
+ | |||
+ | == Experiment of oscillator biobrick parts (30) 2009/08/28 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 28 oscillator part(31).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 29min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Pr3t|1138bp |315bp |f|= | ||
+ | |2: Pr3t|1138bp |315bp |f|= | ||
+ | |3: Pr3t|1138bp |315bp |w|= | ||
+ | |4: Pr3t|1138bp |315bp |f|= | ||
+ | |5: Pr3t|1138bp |315bp |f|= | ||
+ | |6: Pr3t|1138bp |315bp |w|= | ||
+ | |7: Ar2t|749bp |292bp |f|= | ||
+ | |8: Ar2t|749bp |292bp |w|= | ||
+ | |9: Positive Control E0240|1113bp |250bp|w|= | ||
+ | |10: Negative Control |0bp ||w|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
+ | |||
+ | Comments: | ||
+ | |||
+ | * It is great progress that we have finally done the ligation of the Ar2t. Doing the liquid this time, including correct one and fail one. | ||
+ | |||
+ | * Pr3t is correct. Doing the liquid culture tomorrow from the checking plate 090828. | ||
+ | |||
+ | |||
+ | }} | ||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (31) 2009/08/31 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 31 oscillator part(32).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 28min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Ar2t<Er7t|1689bp |749bp |f|= | ||
+ | |2: Ar2t<Er7t|1689bp |749bp |f|= | ||
+ | |3: Ar2t<Er7t|1689bp |749bp |f|= | ||
+ | |4: Ar2t<Er7t|1689bp |749bp |f|= | ||
+ | |5: Ar2t<Er7t|1689bp |749bp |f|= | ||
+ | |6: Ar2t<Er7t|1689bp |749bp |f|= | ||
+ | |7: Ar2t<Er7t|1689bp |749bp |f|= | ||
+ | |8: Ar2t<Er7t|1689bp |749bp |f|= | ||
+ | |9: Positive Control E0240|1113bp |250bp|w|= | ||
+ | |10: Negative Control |0bp |Contamination~700bp|f|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
+ | |||
+ | Comments: | ||
+ | |||
+ | *Because the ligation is fail, I restarted from the ligation again. I changed the protocol, which I used 5.5uL inserted DNA instead of using 4uL inserted DNA. | ||
+ | |||
+ | *Since there are still have colony on the plate, we will run colony PCR again with the ligation I did today(L<r7t and Ar2t<Er7t.}} | ||
+ | |||
+ | == Experiment of oscillator biobrick parts (32) Gel Extraction 2009/08/31 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 08 31 oscillator part(33).png||c= | ||
+ | 2% agarose, 100V, 28min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: 4t|584bp |447bp |f|= | ||
+ | |2: 4t|584bp |447bp |f|= | ||
+ | |3: 4t|584bp |447bp |f|= | ||
+ | |4: 4t|584bp |447bp |f|= | ||
+ | |5: r2t|475bp |38bp |w|= | ||
+ | |6: r2t|475bp |38bp |w|= | ||
+ | |7: r2t|475bp |38bp |w|= | ||
+ | |8: r2t|475bp |38bp |w|= | ||
+ | |9: marker 1kb+100bp|||n}} | ||
+ | |||
+ | Comments: | ||
+ | |||
+ | *The failure of 4t is due to the digestion, so we have to digest it again. | ||
+ | |||
+ | *r2t is fine, so we have extract them from the gel.}} | ||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (33) 2009/09/01 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 01 oscillator part(34).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 29in | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Ar2t<Er7t(090830 ligation)|1689bp |749bp |f|= | ||
+ | |2: Ar2t<Er7t(090830 ligation)|1689bp |749bp |f|= | ||
+ | |3: Ar2t<Er7t(090830 ligation)|1689bp |749bp |f|= | ||
+ | |4: Ar2t<Er7t(090830 ligation)|1689bp |749bp |f|= | ||
+ | |5: Ar2t<Er7t(090830 ligation)|1689bp |749bp |f|= | ||
+ | |6: Ar2t<Er7t(090830 ligation)|1689bp |749bp |f|= | ||
+ | |7: Ar2t<Er7t(090830 ligation)|1689bp |749bp |f|= | ||
+ | |8: L<r2t|895bp |438bp |w|= | ||
+ | |9: L<r2t|895bp |438bp |f|= | ||
+ | |10: L<r2t|895bp |438bp |f|= | ||
+ | |11: L<r2t|895bp |438bp |f|= | ||
+ | |12: L<r2t|895bp |438bp |f|= | ||
+ | |13: L<r2t|895bp |438bp |w|= | ||
+ | |14: L<r2t|895bp |438bp |f|= | ||
+ | |15: Ar2t<Er7t(090831 ligation)|1689bp |749bp |w|= | ||
+ | |16: Ar2t<Er7t(090831 ligation)|1689bp |749bp |f|= | ||
+ | |17: Ar2t<Er7t(090831 ligation)|1689bp |749bp |f|= | ||
+ | |18: Ar2t<Er7t(090831 ligation)|1689bp |749bp |w|= | ||
+ | |19: Ar2t<Er7t(090831 ligation)|1689bp |749bp |w|= | ||
+ | |20: Ar2t<Er7t(090831 ligation)|1689bp |749bp |f|= | ||
+ | |21: Ar2t<Er7t(090831 ligation)|1689bp |749bp |m|= | ||
+ | |22: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |23: Negative Control |0bp |contamination~250,1400bp|f|= | ||
+ | |24: marker 1kb+100bp|||n}} | ||
+ | |||
+ | Comments: | ||
+ | |||
+ | * Liquid incubation should be done by the next day. | ||
+ | |||
+ | * I have do the liquid of the 9 and 19. Only 19 is correct. I will do the Digestion and Ligation tomorrow. | ||
+ | }} | ||
+ | |||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (34) Gel Extraction 2009/09/02 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 02 oscillator part(35).png||c= | ||
+ | 2% agarose, 100V, 28min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Ar2tEr7t|1476bp |537bp |w|= | ||
+ | |2: Ar2tEr7t|1476bp |537bp |w|= | ||
+ | |3: Ar2tEr7t|1476bp |537bp |w|= | ||
+ | |4: Ar2t|537bp |80bp |f|= | ||
+ | |5: Ar2t|537bp |80bp |f|= | ||
+ | |6: Ar2t|537bp |80bp |f|= | ||
+ | |7: marker 1kb+100bp|||n}} | ||
+ | |||
+ | Comments: | ||
+ | |||
+ | *The failure of Ar2t is strange, maybe it is that I put too much DNA in the digestion. | ||
+ | |||
+ | *Ar2tEr7t is not digested well, next time we should not put too much DNA. | ||
+ | |||
+ | *concentration measurement before the digestion | ||
+ | |||
+ | }} | ||
+ | |||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (35) 2009/09/03 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 03 oscillator part(36).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|140s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 29min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Er3t<Ar2tEr7t|2567bp |1109bp |w|= | ||
+ | |2: Er3t<Ar2tEr7t|2567bp |1109bp |w|= | ||
+ | |3: Er3t<Ar2tEr7t|2567bp |1109bp |w|= | ||
+ | |4: Er3t<Ar2tEr7t|2567bp |1109bp |w|= | ||
+ | |5: Er3t<Ar2tEr7t|2567bp |1109bp |w|= | ||
+ | |6: Er3t<Ar2tEr7t|2567bp |1109bp |w|= | ||
+ | |7: Er3t<Ar2tEr7t|2567bp |1109bp |m|= | ||
+ | |8: Er3t<Ar2tEr7t|2567bp |1109bp |f|= | ||
+ | |9: Positive Control E0240|1113bp |250bp|w|= | ||
+ | |10: Negative Control |0bp |Contamination~290bp,1300bp,1400bp |f|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
+ | |||
+ | Comments: | ||
+ | |||
+ | *There is a lot of contamination in the negative control. We speculated that it might be due to buffer since that eyelight used the old taq and buffer. | ||
+ | *The length seems to be right, but it is still need to be measured by GFP machine to check if it could be oscillate. | ||
+ | |||
+ | }} | ||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (36) Gel Extraction 2009/09/03 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 03 oscillator part(37).png||c= | ||
+ | 2% agarose, 100V, 28min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Ar2t(8-2)|537bp |80bp |f|= | ||
+ | |2: Ar2t(8-2)|537bp |80bp |f|= | ||
+ | |3: Ar2t(8-2)|537bp |80bp |f|= | ||
+ | |4: Er3t|897bp |74bp |w|= | ||
+ | |5: Er3t|897bp |74bp |w|= | ||
+ | |6: Er3t|897bp |74bp |w|= | ||
+ | |7: -|||n|= | ||
+ | |8: 4t|584bp |447bp |w|= | ||
+ | |9: 4t|584bp |447bp |w|= | ||
+ | |10: 4t|584bp |447bp |w|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
+ | |||
+ | Comments: | ||
+ | |||
+ | *Ar2t still fails. Er3t is the one that we are trying to ligate with Ar2t. | ||
+ | |||
+ | |||
+ | }} | ||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (37) 2009/09/04 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 04 oscillator part(38).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|110s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 29in | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Lr2t<Er7t|1834bp |895bp |f|= | ||
+ | |2: Lr2t<Er7t|1834bp |895bp |f|= | ||
+ | |3: Lr2t<Er7t|1834bp |895bp |f|= | ||
+ | |4: Lr2t<Er7t|1834bp |895bp |f|= | ||
+ | |5: Lr2t<Er7t|1834bp |895bp |w|= | ||
+ | |6: P<r2t|772bp |315bp |f|= | ||
+ | |7: P<r2t|772bp |315bp |w|= | ||
+ | |8: P<r2t|772bp |315bp |f|= | ||
+ | |9: P<r2t|772bp |315bp |w|= | ||
+ | |10: P<r2t|772bp |315bp |f|= | ||
+ | |11: Ar2t<Er3t|1628bp |749bp |f|= | ||
+ | |12: Ar2t<Er3t|1628bp |749bp |f|= | ||
+ | |13: Ar2t<Er3t|1628bp |749bp |w|= | ||
+ | |14: Ar2t<Er3t|1628bp |749bp |f|= | ||
+ | |15: Ar2t<Er3t|1628bp |749bp |f|= | ||
+ | |16: r<4t|816bp |250bp |w|= | ||
+ | |17: r<4t|816bp |250bp |f|= | ||
+ | |18: r<4t|816bp |250bp |w|= | ||
+ | |19: r<4t|816bp |250bp |w|= | ||
+ | |20: r<4t|816bp |250bp |w|= | ||
+ | |21: r<4t|816bp |250bp |w|= | ||
+ | |22: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |23: Negative Control |0bp ||m|= | ||
+ | |24: marker 1kb+100bp|||n}} | ||
+ | |||
+ | Comments | ||
+ | |||
+ | *There is no contamination since I use the old buffer and enzyme. In addition, I change to use new dNTP and I speculated the contamination might be due to new buffer. | ||
+ | |||
+ | *Need to make liquid incubation by using checking plate | ||
+ | |||
+ | }} | ||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (38) Gel Extraction 2009/09/09 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 09 oscillator part(39).png||c= | ||
+ | 2% agarose, 100V, 28min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 100bp|||n|= | ||
+ | |1: marker 1kb|||n|= | ||
+ | |2: r4t|604bp |38bp |w|= | ||
+ | |3: r4t|604bp |38bp |w|= | ||
+ | |4: r4t|604bp |38bp |w|= | ||
+ | |5: -|||n|= | ||
+ | |6: Ar2tEr7t|707bp |?bp |w|= | ||
+ | |7: Er3tAr2tEr7t|707bp|?bp|w|= | ||
+ | |8: marker 1kb|||n|= | ||
+ | |9: marker 100bp|||n|=}} | ||
+ | |||
+ | Comments: | ||
+ | |||
+ | *r4t is correct though it is not digested well enough. | ||
+ | |||
+ | |||
+ | }} | ||
+ | |||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (39) 2009/09/11 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 11 oscillator part(40).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|110s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 28in | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: A<r4t|878bp |292bp |f|= | ||
+ | |2: E<r4t|872bp |286bp |w|= | ||
+ | |3: E<r4t|872bp |286bp |w|= | ||
+ | |4: E<r4t|872bp |286bp |w|= | ||
+ | |5: E<r4t|872bp |286bp |w|= | ||
+ | |6: E<r4t|872bp |286bp |w|= | ||
+ | |7: E<r4t|872bp |286bp |w|= | ||
+ | |8: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |9: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |10: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |11: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |12: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |13: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |14: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |15: Negative Control |0bp ||w|= | ||
+ | |16: marker 1kb+100bp|||n}} | ||
+ | |||
+ | Comments | ||
+ | |||
+ | *It is awful that the plate of Ar4t only have one colony on it. Maybe it is due to the bad digestion of pTet(A). Should the experiment be started from the digestion of pTet or ligation? | ||
+ | |||
+ | *Pr2t<Er7t could do the colony PCR again to check if there are another correct colony. | ||
+ | }} | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (40) 2009/09/15 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 15 oscillator part(41).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|100s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 29in | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |2: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |3: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |4: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |5: Pr2t<Er7t|1712bp |772bp |m|= | ||
+ | |6: A<r4t|878bp |292bp |f|= | ||
+ | |7: A<r4t|878bp |292bp |f|= | ||
+ | |8: A<r4t|878bp |292bp |f|= | ||
+ | |9: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |10: Negative Control |0bp |contamination~700bp|f|= | ||
+ | |11: marker 1kb+100bp|||n}} | ||
+ | |||
+ | |||
+ | Comments: | ||
+ | |||
+ | *Redo the colony PCR again and use more colony to check if there is a correct colony. | ||
+ | *Lane 5 is strange, maybe it is the P<Er7t because the r2t hasn't been ligated correctly. | ||
+ | *Ar4t keeps fail, however there are some small colony we can pick up. | ||
+ | |||
+ | }} | ||
+ | |||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (41) 2009/09/17 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 17 oscillator part(42).png|{{:Team:NYMU-Taipei/PCR|60s|15s|110s|100s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 29in | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: A<r4t|878bp |292bp |w|= | ||
+ | |2: A<r4t|878bp |292bp |w|= | ||
+ | |3: A<r4t|878bp |292bp |w|= | ||
+ | |4: A<r4t|878bp |292bp |w|= | ||
+ | |5: A<r4t|878bp |292bp |w|= | ||
+ | |6: A<r4t|878bp |292bp |w|= | ||
+ | |7: A<r4t|878bp |292bp |w|= | ||
+ | |8: A<r4t|878bp |292bp |w|= | ||
+ | |9: A<r4t|878bp |292bp |w|= | ||
+ | |10: A<r4t|878bp |292bp |w|= | ||
+ | |11: A<r4t|878bp |292bp |w|= | ||
+ | |12: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |13: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |14: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |15: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |16: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |17: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |18: Pr2t<Er7t|1712bp |772bp |w|= | ||
+ | |19: Pr2t<Er7t|1712bp |772bp |m|= | ||
+ | |20: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |21: Pr2t<Er7t|1712bp |772bp |f|= | ||
+ | |22: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |23: Negative Control |0bp |contamination~300bp,700bp|f|= | ||
+ | |24: marker 1kb+100bp|||n}} | ||
+ | |||
+ | |||
+ | Comments: | ||
+ | |||
+ | }} | ||
+ | |||
+ | == Experiment of oscillator biobrick parts (42) 2009/09/18 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 18 oscillator part(43).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|40s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 28in | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: pLuxR|293bp |238bp |w|= | ||
+ | |2: pLuxR|293bp |238bp |w|= | ||
+ | |3: pCI|287bp |238bp |w|= | ||
+ | |4: pCI|287bp |238bp |w|= | ||
+ | |5: p22|292bp |238bp |w|= | ||
+ | |6: p22|292bp |238bp |w|= | ||
+ | |7: pLasR|395bp |238bp |w|= | ||
+ | |8: pLasR|395bp |238bp |w|= | ||
+ | |9: Positive Control Term|445bp |316bp|w|= | ||
+ | |10: Negative Control |0bp |contamination~700bp|f|= | ||
+ | |11: marker 1kb+100bp|||n}}}} | ||
+ | |||
+ | |||
+ | == Experiment of oscillator biobrick parts (43) 2009/09/22 == | ||
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 22 oscillator part(44).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|70s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 28in | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 100bp|||n|= | ||
+ | |1: p22+r7t|1175bp |292bp |m|= | ||
+ | |2: p22+r7t|1175bp |292bp |w|= | ||
+ | |3: p22+r7t|1175bp |292bp |w|= | ||
+ | |4: p22+r7t|1175bp |292bp |w|= | ||
+ | |5: pLuxR+r7t|1176bp |293bp |w|= | ||
+ | |6: pLuxR+r7t|1176bp |293bp |w|= | ||
+ | |7: pLuxR+r7t|1176bp |293bp |w|= | ||
+ | |8: pLuxR+r7t|1176bp |293bp |w|= | ||
+ | |9: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |10: Negative Control |0bp ||w|= | ||
+ | |11: marker 100bp|||n}}}} | ||
- | |||
- | |||
- | |||
- | == | + | == Experiment of oscillator biobrick parts (44) 2009/09/24 == |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 24 oscillator part(45).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 28in | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 100bp|||n|= | ||
+ | |1: pLuxR+r7t|1176bp |293bp |m|= | ||
+ | |2: pLuxR+r7t|1176bp |293bp |w|= | ||
+ | |3: pLuxR+r7t|1176bp |293bp |w|= | ||
+ | |4: pCI+r7t|1170bp |287bp |m|= | ||
+ | |5: pLasR+r7t|1278bp |395bp |w|= | ||
+ | |6: pLasR+r7t|1278bp |395bp |w|= | ||
+ | |7: pLasR+r7t|1278bp |395bp |w|= | ||
+ | |8: pLasR+r7t|1278bp |395bp |w|= | ||
+ | |9: Positive Control E0240|1114bp |238bp|w|= | ||
+ | |10: Negative Control |0bp |contamination~1100bp|w|= | ||
+ | |11: marker 100bp|||n}} | ||
- | + | Comments: | |
- | + | *It is strange that the colony of pCI+r7t is glowing obviously, but the length seems to be wrong. | |
- | + | }} | |
- | |||
- | + | == Experiment of oscillator biobrick parts (45) (Gel Extraction) 2009/09/28== | |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 09 28 oscillator part(46).png||c= | ||
+ | 2% agarose, 100V, 30min | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 1kb+100bp|||n|= | ||
+ | |1: Pr2tEr7t-18|1500bp |560bp |w|= | ||
+ | |2: Pr2tEr7t-18|1500bp |560bp |w|= | ||
+ | |3: Pr2tEr7t-18|1500bp |560bp |w|= | ||
+ | |4: Pr2tEr7t-19|1500bp |560bp |m|= | ||
+ | |5: Pr2tEr7t-19|1500bp |560bp |m|= | ||
+ | |6: Pr2tEr7t-19|1500bp |560bp |m|= | ||
+ | |7: unknown|841bp |38bp |m|= | ||
+ | |8: unknown|841bp |38bp |m|= | ||
+ | |9: unknown|841bp |38bp |m|= | ||
+ | |10: unknown|841bp |38bp |m|= | ||
+ | |11: marker 1kb+100bp|||n}} }} | ||
- | |||
- | |||
- | + | == Experiment of oscillator biobrick parts (46) 2009/10/17 == | |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 10 17 oscillator part(47).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 28in | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 100bp|||n|= | ||
+ | |1: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |2: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |3: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |4: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |5: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |6: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |7: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |8: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |9: Positive Control Lr7t|1321bp |438bp|w|= | ||
+ | |10: Negative Control |0bp |contamination~1100bp|w|= | ||
+ | |11: marker 100bp|||n}}}} | ||
- | |||
- | {{:Team:NYMU-Taipei/ | + | == Experiment of oscillator biobrick parts (47) 2009/10/18 == |
+ | {{:Team:NYMU-Taipei/GEL|NYMU 2009 10 18 oscillator part(48).png|{{:Team:NYMU-Taipei/PCR|60s|15s|20s|80s|300s|rp=VR|fp=VF2}}|c= | ||
+ | 2% agarose, 100V, 30in | ||
+ | {{:Team:NYMU-Taipei/GELC|= | ||
+ | |0: marker 100bp|||n|= | ||
+ | |1: marker 1kb|||n|= | ||
+ | |2: Ar4t<Pr3t|1786bp |878bp |f|= | ||
+ | |3: Ar4t<Pr3t|1786bp |878bp |m|= | ||
+ | |4: Ar4t<Pr3t|1786bp |878bp |f|= | ||
+ | |5: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |6: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |7: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |8: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |9: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |10: Er4t<Pr2t|1414bp |872bp |w|= | ||
+ | |11: Er4t<Pr2t|1414bp |872bp |m|= | ||
+ | |12: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |13: Er4t<Pr2t|1414bp |872bp |f|= | ||
+ | |14: Positive Control Ar7t|1175bp |292bp|w|= | ||
+ | |15: Negative Control |0bp |contamination~1100bp|w|= | ||
+ | |16: Negative Control |0bp |contamination~1100bp|w|= | ||
+ | |17: marker 1kb|||n|= | ||
+ | |18: marker 100bp|||n}}}} |
Latest revision as of 21:54, 21 October 2009
Experiment of oscillator biobrick parts
1 | BBa_C0051 cI repressor from E. coli phage lambda (+LVA) |
2 | BBa_K116602 CII coding region from λ phage |
3 | BBa_C0040 tetracycline repressor from transposon Tn10 (+LVA) |
4 | BBa_C0074 penI repressor from Bacillus licheniformis (+LVA) |
5 | BBa_C0072 mnt repressor (strong) from Salmonella phage P22 (+LVA) |
6 | BBa_C0073 mnt repressor (weak) from Salmonella phage P22 (+LVA) |
7 | BBa_E0040 green fluorescent protein |
t | BBa_B0015 Terminator |
A | BBa_R0040 TetR repressible promoter |
P | BBa_R0074 Promoter (PenI regulated) |
L | BBa_R0010 promoter (lacI regulated) |
M | BBa_R0073 Promoter (Mnt regulated) |
C | BBa_R0051 promoter (lambda cI regulated) |
pCI | BBa_R1051 Promoter, Standard (lambda cI regulated) |
p22 | BBa_R0053 Promoter (p22 cII regulated) |
pLuxR | BBa_R0062 Promoter (luxR & HSL regulated -- lux pR) |
pLasR | BBa_R0079 Promoter (LasR & PAI regulated) |
E | BBa_K116603 pRE promoter from λ phage |
Experiment of oscillator biobrick parts (2)
| 2% agarose, 90V, 30min
|
Experiment of oscillator biobrick parts (3)
| 2% agarose, 90V, 30min
|
4: Inconclusive.
Experiment of oscillator biobrick parts (4)
| 2% agarose, 90V, 30min
The result for lanes 7-11 look weird, but it could be because of the gel. A rerun will be done. |
Experiment of oscillator biobrick parts (5)
| 2% agarose, 90V, 30min
|
Experiment of oscillator biobrick parts (6)
| 2% agarose, 90V, 30min
|
Experiment of oscillator biobrick parts (7)
| 2% agarose, 90V, 30min
|
Experiment of oscillator biobrick parts (8)
| 2% agarose, 90V, 30min
|
Experiment of oscillator biobrick parts (9) Gel Extraction
| 2% agarose, 90V, 30min
|
Experiment of oscillator biobrick parts (10) (Gel Extraction)
| 2% agarose, 90V, 30min
|
Experiment of oscillator biobrick parts (11)
| 2% agarose, 90V, 30min
|
Experiment of oscillator biobrick parts (12)
| 2% agarose, 90V, 30min
|
Experiment of oscillator biobrick parts (13) 2009/08/13
| 2% agarose, 90V, 38min
|
Experiment of oscillator biobrick parts (14) (Gel Extraction) 2009/08/13
| 2% agarose, 90V, 36min
|
Experiment of oscillator biobrick parts (15) 2009/08/15
| 2% agarose, 100V, 30min
|
Experiment of oscillator biobrick parts (16) (Gel Extraction) 2009/08/15
| 2% agarose, 100V, 30min
|
Experiment of oscillator biobrick parts (17) 2009/08/16
| 2% agarose, 100V, 30min
|
Experiment of oscillator biobrick parts (18) (digestion) 2009/08/17
| 2% agarose, 100V, 30min
Comments
|
Experiment of oscillator biobrick parts (19) (Gel Extraction) 2009/08/17
| 2% agarose, 100V, 30min
|
Experiment of oscillator biobrick parts (20) 2009/08/18
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (21) (Gel Extraction) 2009/08/18
| 2% agarose, 100V, 30min
|
Experiment of oscillator biobrick parts (22) 2009/08/19
| 2% agarose, 100V, 28min
PCR of nhaA using this protocol worked. |
Experiment of oscillator biobrick parts (23) 2009/08/19
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (24) 2009/08/20
| 2% agarose, 100V, 27min
Comments:
|
Experiment of oscillator biobrick parts (25) 2009/08/21
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (26) 2009/08/22
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (27) 2009/08/23 colony PCR
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (28) 2009/08/23 testing the reheating gel
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (29) 2009/08/26
| 2% agarose, 100V, 29min
|
Experiment of oscillator biobrick parts (29) 2009/08/27
| 2% agarose, 100V, 29min
|
Experiment of oscillator biobrick parts (30) 2009/08/28
| 2% agarose, 100V, 29min
|
Experiment of oscillator biobrick parts (31) 2009/08/31
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (32) Gel Extraction 2009/08/31
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (33) 2009/09/01
| 2% agarose, 100V, 29in
|
Experiment of oscillator biobrick parts (34) Gel Extraction 2009/09/02
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (35) 2009/09/03
| 2% agarose, 100V, 29min
|
Experiment of oscillator biobrick parts (36) Gel Extraction 2009/09/03
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (37) 2009/09/04
| 2% agarose, 100V, 29in
|
Experiment of oscillator biobrick parts (38) Gel Extraction 2009/09/09
| 2% agarose, 100V, 28min
|
Experiment of oscillator biobrick parts (39) 2009/09/11
| 2% agarose, 100V, 28in
|
Experiment of oscillator biobrick parts (40) 2009/09/15
| 2% agarose, 100V, 29in
Comments:
|
Experiment of oscillator biobrick parts (41) 2009/09/17
| 2% agarose, 100V, 29in
Comments: |
Experiment of oscillator biobrick parts (42) 2009/09/18
| 2% agarose, 100V, 28in
|
Experiment of oscillator biobrick parts (43) 2009/09/22
| 2% agarose, 100V, 28in
|
Experiment of oscillator biobrick parts (44) 2009/09/24
| 2% agarose, 100V, 28in
|
Experiment of oscillator biobrick parts (45) (Gel Extraction) 2009/09/28
| 2% agarose, 100V, 30min
|
Experiment of oscillator biobrick parts (46) 2009/10/17
| 2% agarose, 100V, 28in
|
Experiment of oscillator biobrick parts (47) 2009/10/18
| 2% agarose, 100V, 30in
|