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Team:Wisconsin-Madison/notebook/Sarah
From 2010.igem.org
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| - | =Progress Report 6-3-2010= | + | ==Progress Report 6-3-2010== |
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'''Major Accomplishments''' | '''Major Accomplishments''' | ||
* pBAD's: 18, 33, 35 were successfully made into biobrick vectors | * pBAD's: 18, 33, 35 were successfully made into biobrick vectors | ||
| Line 24: | Line 23: | ||
* Research has been mapped and divided | * Research has been mapped and divided | ||
* ordered parts have either been confirmed or marked as incorrect | * ordered parts have either been confirmed or marked as incorrect | ||
| - | |||
'''Plans for next week''' | '''Plans for next week''' | ||
* Finish encapsulation clones | * Finish encapsulation clones | ||
| Line 31: | Line 29: | ||
* Finnish individual research and have team meeting | * Finnish individual research and have team meeting | ||
* inducible/repressable promotion system | * inducible/repressable promotion system | ||
| - | |||
| - | |||
| - | |||
| - | |||
''Day by Day overview:'' | ''Day by Day overview:'' | ||
| - | |||
'''5-24-2010''' | '''5-24-2010''' | ||
* Lab materials, organization | * Lab materials, organization | ||
| Line 71: | Line 64: | ||
* Planned 4 testing clones of encapsulation | * Planned 4 testing clones of encapsulation | ||
* Encapsulation clones: digestion, extraction, overnight ligation | * Encapsulation clones: digestion, extraction, overnight ligation | ||
| - | + | <br> | |
| - | + | ==Progress Report 6-11-2010== | |
| - | =Progress Report 6-11-2010= | + | |
| - | + | ||
| - | + | ||
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
* 1/2 clones | * 1/2 clones | ||
RcsB:pBAD18BB:DH10b colony PCR | RcsB:pBAD18BB:DH10b colony PCR | ||
| - | |||
[[File: 9.jpg| 400px]] | [[File: 9.jpg| 400px]] | ||
| - | |||
'''Plans for next week''' | '''Plans for next week''' | ||
* Acid survival tests (growth curves and acid dunk) | * Acid survival tests (growth curves and acid dunk) | ||
| Line 89: | Line 77: | ||
* alkaline lysis and digestion of C3 of above colony PCR | * alkaline lysis and digestion of C3 of above colony PCR | ||
| - | |||
'''6-3-2010''' | '''6-3-2010''' | ||
* Got out of Jury Duty | * Got out of Jury Duty | ||
| Line 95: | Line 82: | ||
* Map of LacZ - wrong part | * Map of LacZ - wrong part | ||
* Liquid Cultures | * Liquid Cultures | ||
| - | |||
'''6-4-2010''' | '''6-4-2010''' | ||
* Map (no cut) of pBAD clones | * Map (no cut) of pBAD clones | ||
* encapsulation clones: Miniprep, digestion, gel extraction (wrong) | * encapsulation clones: Miniprep, digestion, gel extraction (wrong) | ||
| - | |||
'''6-7-2010''' | '''6-7-2010''' | ||
* advisor meeting | * advisor meeting | ||
* encapsulation clones to ligation | * encapsulation clones to ligation | ||
| - | |||
'''6-8-2010''' | '''6-8-2010''' | ||
* transformation and plating of encapsulation clones | * transformation and plating of encapsulation clones | ||
| - | |||
'''6-9-2010''' | '''6-9-2010''' | ||
* transformation and plating of encryption clones | * transformation and plating of encryption clones | ||
| - | |||
'''6-10-2010''' | '''6-10-2010''' | ||
* screening of pBAD clones - colony PCR | * screening of pBAD clones - colony PCR | ||
* encapsulation research | * encapsulation research | ||
| - | + | <br> | |
| - | =Progress Report 6-18-2010= | + | ==Progress Report 6-18-2010== |
| - | + | ||
| - | + | ||
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
* Identified and verified next set of parts for cloning | * Identified and verified next set of parts for cloning | ||
| - | |||
'''Plans for next week''' | '''Plans for next week''' | ||
* screen more clones (YgiV and RfaI) | * screen more clones (YgiV and RfaI) | ||
| Line 126: | Line 105: | ||
* pBAD series + RFP | * pBAD series + RFP | ||
* YgiV and RfaI in pBADs | * YgiV and RfaI in pBADs | ||
| - | |||
---- | ---- | ||
'''6/11/10''' | '''6/11/10''' | ||
| Line 132: | Line 110: | ||
* Sequencing rxn of pBADBB [18,33,35] | * Sequencing rxn of pBADBB [18,33,35] | ||
* Planned Map of new ordered parts | * Planned Map of new ordered parts | ||
| - | |||
'''6/14/10''' | '''6/14/10''' | ||
* Mapping of new plates of biobrick vector pBADs | * Mapping of new plates of biobrick vector pBADs | ||
* primer Design of 6 new primers for two well characterized encapsulation genes | * primer Design of 6 new primers for two well characterized encapsulation genes | ||
* Restriction Map of 9 new parts - all correct | * Restriction Map of 9 new parts - all correct | ||
| - | |||
'''6/15/10''' | '''6/15/10''' | ||
* Miniprep of new parts, rcsB clone, and pBADBBs | * Miniprep of new parts, rcsB clone, and pBADBBs | ||
* Restriction map of more parts - ?? | * Restriction map of more parts - ?? | ||
| - | |||
'''6/16/10''' | '''6/16/10''' | ||
* Ligation of RfaI:pBAD35BB | * Ligation of RfaI:pBAD35BB | ||
* Website and Logo | * Website and Logo | ||
| - | |||
'''6/17/10''' | '''6/17/10''' | ||
* Restriction map of iffy parts | * Restriction map of iffy parts | ||
| Line 152: | Line 126: | ||
* Ran mary's gel with 2x concentration of DNA | * Ran mary's gel with 2x concentration of DNA | ||
* ReDigestion of pBAD35BB | * ReDigestion of pBAD35BB | ||
| - | |||
'''6/18/10''' | '''6/18/10''' | ||
* colony PCR of RfaI:pBAD15BB:DH10B x10- fail | * colony PCR of RfaI:pBAD15BB:DH10B x10- fail | ||
* ReDigest and extract pBAD35BB | * ReDigest and extract pBAD35BB | ||
| - | + | <br> | |
| - | =Progress Report 6-25-2010= | + | ==Progress Report 6-25-2010== |
| - | + | ||
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
* Discovered flaw in pBAD35BB: | * Discovered flaw in pBAD35BB: | ||
| Line 168: | Line 140: | ||
** '''Q:''' Do you know anything about a point mutation your lab did or why this is? (DamI methylation?) | ** '''Q:''' Do you know anything about a point mutation your lab did or why this is? (DamI methylation?) | ||
* New and complete planning of cloning, experiments and parts: [https://mywebspace.wisc.edu/sandock/iDIET%20Project.pdf Project Plan] | * New and complete planning of cloning, experiments and parts: [https://mywebspace.wisc.edu/sandock/iDIET%20Project.pdf Project Plan] | ||
| - | |||
| - | |||
| - | |||
| - | |||
---- | ---- | ||
'''6-20-2010''' | '''6-20-2010''' | ||
| Line 177: | Line 145: | ||
** 35 has inactive PstI | ** 35 has inactive PstI | ||
** 33 has inactive extra EcoRI | ** 33 has inactive extra EcoRI | ||
| - | |||
'''6-21-2010''' | '''6-21-2010''' | ||
* Alkaline Lysis and Digestion of RcsB:pBAD18BB - WRONG | * Alkaline Lysis and Digestion of RcsB:pBAD18BB - WRONG | ||
| Line 184: | Line 151: | ||
* confirmation of faulty 35 PstI from sequencing data | * confirmation of faulty 35 PstI from sequencing data | ||
* New digestion protocol uses less reagents | * New digestion protocol uses less reagents | ||
| - | |||
'''6-22-2010''' | '''6-22-2010''' | ||
* pBAD35 - around the world PCR, DpnI digest, PCR clean up, XbaI digest, PCR cleanup, Ligation, transformation, plating | * pBAD35 - around the world PCR, DpnI digest, PCR clean up, XbaI digest, PCR cleanup, Ligation, transformation, plating | ||
* colony PCR of direct genes: wz, wzT, yjb, yjbT | * colony PCR of direct genes: wz, wzT, yjb, yjbT | ||
| - | |||
'''6-23-2010''' | '''6-23-2010''' | ||
* got 3 genes from colony PCR of direct genes (not yjb) | * got 3 genes from colony PCR of direct genes (not yjb) | ||
* pBAD34 - around the world PCR, DpnI digest, PCR clean up, XbaI digest, PCR cleanup, Ligation, transformation, plating | * pBAD34 - around the world PCR, DpnI digest, PCR clean up, XbaI digest, PCR cleanup, Ligation, transformation, plating | ||
* Phussion PCR from colony PCR template | * Phussion PCR from colony PCR template | ||
| - | |||
'''6-24-2010''' | '''6-24-2010''' | ||
* Finished organizing and typing project plan | * Finished organizing and typing project plan | ||
| Line 201: | Line 165: | ||
** [[File:222.jpg]] | ** [[File:222.jpg]] | ||
* Ran PCR off of colony PCR as Template - FAIL (use colony PCR next time) | * Ran PCR off of colony PCR as Template - FAIL (use colony PCR next time) | ||
| - | |||
'''6-25-2010''' | '''6-25-2010''' | ||
* Alkaline lysis of pBAD35BB and pBAD34BB | * Alkaline lysis of pBAD35BB and pBAD34BB | ||
| Line 209: | Line 172: | ||
** [[File:222.jpg]] | ** [[File:222.jpg]] | ||
* Initial digestion of and pBAD34BB - Fail | * Initial digestion of and pBAD34BB - Fail | ||
| - | + | <br> | |
| - | =Progress Report 7-2-2010= | + | ==Progress Report 7-2-2010== |
| - | + | ||
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
* Decided the pBAD vectors were a lost cause | * Decided the pBAD vectors were a lost cause | ||
| Line 218: | Line 180: | ||
* Clones assigned to team | * Clones assigned to team | ||
* Created clones box and updated completed parts | * Created clones box and updated completed parts | ||
| - | |||
'''Plans for next week''' | '''Plans for next week''' | ||
* Clone | * Clone | ||
* New LuxR Rev primer that includes stop codon | * New LuxR Rev primer that includes stop codon | ||
| - | |||
---- | ---- | ||
'''6-28-2010''' | '''6-28-2010''' | ||
* cloning of RcsA downstream of RcsB in iGEM vector pSB1AK3 | * cloning of RcsA downstream of RcsB in iGEM vector pSB1AK3 | ||
| - | |||
'''6-29-2010''' | '''6-29-2010''' | ||
* Successful cloning of RcsB+RcsA - Colony PCR | * Successful cloning of RcsB+RcsA - Colony PCR | ||
| Line 235: | Line 194: | ||
* cloning of YgiV downstream of pLacI+RBS in iGEM vector pSB1AK3 | * cloning of YgiV downstream of pLacI+RBS in iGEM vector pSB1AK3 | ||
* cloning of RfaI downstream of pLacI+RBS in iGEM vector pSB1AK3 | * cloning of RfaI downstream of pLacI+RBS in iGEM vector pSB1AK3 | ||
| - | |||
'''6-30-2010''' | '''6-30-2010''' | ||
* pBAD vectors have given us too much trouble. Time to move on. | * pBAD vectors have given us too much trouble. Time to move on. | ||
| Line 244: | Line 202: | ||
** Correct usage of ribosome binding sites | ** Correct usage of ribosome binding sites | ||
* Ordered and transformed all nessesary parts from registry | * Ordered and transformed all nessesary parts from registry | ||
| - | |||
'''7-1-2010''' | '''7-1-2010''' | ||
* Finished new project plan | * Finished new project plan | ||
| Line 252: | Line 209: | ||
** [[File:plry.jpg|400px]] | ** [[File:plry.jpg|400px]] | ||
* Liquid cultures of transformed parts and successful clones | * Liquid cultures of transformed parts and successful clones | ||
| - | |||
'''7-2-2010''' | '''7-2-2010''' | ||
* Miniprep of 7 Parts from Registry | * Miniprep of 7 Parts from Registry | ||
| Line 258: | Line 214: | ||
* Cloning of I13507 (RBS+mRFP+TT) downstream of R0065 (InducibleRepressiblePromoter) in iGEM vector pSB1A2 | * Cloning of I13507 (RBS+mRFP+TT) downstream of R0065 (InducibleRepressiblePromoter) in iGEM vector pSB1A2 | ||
** for both clonings, backbones cut but inserts were undigested. | ** for both clonings, backbones cut but inserts were undigested. | ||
| - | + | <br> | |
| - | =Progress Report 7-9-2010= | + | ==Progress Report 7-9-2010== |
| - | + | ||
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
* Clone: K200021+C0051 | * Clone: K200021+C0051 | ||
| Line 273: | Line 228: | ||
**[[File:oiue2.jpg|200px]] | **[[File:oiue2.jpg|200px]] | ||
* Sequencing rxn of clones 1 and 2 | * Sequencing rxn of clones 1 and 2 | ||
| - | |||
'''7-6-2010''' | '''7-6-2010''' | ||
* Digestion | * Digestion | ||
* Magnetic Bead cleanup and submission for sequencing | * Magnetic Bead cleanup and submission for sequencing | ||
| - | |||
'''7-7-2010''' | '''7-7-2010''' | ||
* Cloning of C0051 (Repressor and Deg Tag) downstream of K200021(LacI promoter + RBS) in iGEM vector pSB1AK3 | * Cloning of C0051 (Repressor and Deg Tag) downstream of K200021(LacI promoter + RBS) in iGEM vector pSB1AK3 | ||
| - | |||
'''7-8-2010''' | '''7-8-2010''' | ||
* Colony PCR of clone from yesterday | * Colony PCR of clone from yesterday | ||
| Line 287: | Line 239: | ||
* Liquid culture colony#5, colony #6, K112808, I13507 | * Liquid culture colony#5, colony #6, K112808, I13507 | ||
* Went to CS for programing help | * Went to CS for programing help | ||
| - | |||
'''7-9-2010''' | '''7-9-2010''' | ||
* Alkaline Lysis of colony#5, colony#6, K112808, I13507 | * Alkaline Lysis of colony#5, colony#6, K112808, I13507 | ||
| Line 294: | Line 245: | ||
* Kit Miniprep of colony#6 | * Kit Miniprep of colony#6 | ||
* Cloning of above clone in front of B0034(RBS) and B0015(TT) - Digestion, Ligation | * Cloning of above clone in front of B0034(RBS) and B0015(TT) - Digestion, Ligation | ||
| - | + | <br> | |
| - | =Progress Report 7-16-2010= | + | ==Progress Report 7-16-2010== |
| - | + | ||
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
| Line 304: | Line 254: | ||
| - | + | <br> | |
| - | =Progress Report 7-23-2010= | + | ==Progress Report 7-23-2010== |
| - | + | ||
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
| Line 314: | Line 263: | ||
| - | + | <br> | |
| - | =Progress Report 7-30-2010= | + | ==Progress Report 7-30-2010== |
| - | + | ||
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
| Line 324: | Line 272: | ||
---- | ---- | ||
| - | =Progress Report 8-6-2010= | + | <br> |
| - | + | ==Progress Report 8-6-2010== | |
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
| Line 333: | Line 281: | ||
---- | ---- | ||
| - | =Progress Report 8-13-2010= | + | <br> |
| - | + | ==Progress Report 8-13-2010== | |
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
| Line 342: | Line 290: | ||
---- | ---- | ||
| - | =Progress Report 8-20-2010= | + | <br> |
| - | + | ==Progress Report 8-20-2010== | |
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
| Line 351: | Line 299: | ||
---- | ---- | ||
| - | =Progress Report 8-27-2010= | + | <br> |
| - | + | ==Progress Report 8-27-2010== | |
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
'''Plans for next week''' | '''Plans for next week''' | ||
| - | |||
| - | |||
---- | ---- | ||
| - | =Progress Report 9-3-2010= | + | <br> |
| - | + | ==Progress Report 9-3-2010== | |
'''Major Accomplishments''' | '''Major Accomplishments''' | ||
'''Plans for next week''' | '''Plans for next week''' | ||
| - | |||
| - | |||
---- | ---- | ||
Revision as of 02:54, 30 September 2010
Progress Report 6-3-2010
Major Accomplishments
- pBAD's: 18, 33, 35 were successfully made into biobrick vectors
- Primers are done and being ordered
- Lab is organized and a method of labeling and storage is established
- Research has been mapped and divided
- ordered parts have either been confirmed or marked as incorrect
Plans for next week
- Finish encapsulation clones
- Test encapsulation clones (pH and growth curves in testing strain)
- comp cells with either MG1655 or BL21
- Finnish individual research and have team meeting
- inducible/repressable promotion system
Day by Day overview: 5-24-2010
- Lab materials, organization
- Comp Cell overview
- Began Primer Deisgn
- pBAD point mutations
5-25-2010
- began around the world cloning of pBADs up to Digestion overnight
- Primer design
- Redid PCR of pBAD34
5-26-2010
- pBAD 34: digestion to overnight ligation
- pBAD 18,33,35: Ligating to plating transformation
- Finished primer design
5-27-2010
- pBAD34: transformed and plated
- pBAD 18,33,35: picked colonies to screen
- restriction mapping of parts ordered
- Cleaned out fridge and freeze and organized by project (lac v encypt)
5-28-2010
- Alkaline lysis of 23 colonies
- Restriction mapping of pBAD-BB 18, 34, 35 - SUCCESSFUL
- Liquid cultures of pBAD34
- Double digest of ordered parts – Lactose: 3 capsule genes OK
5-29-2010
- Alkaline lysis for screening of pBAD34-BB
6-1-2010
- restriction map of pBAD34-BB – Fail
- inventor of correct vs wrong parts
- planned clones for next day
- research on project
6-2-2010
- Mapped out needed research and assigned to team
- Planned 4 testing clones of encapsulation
- Encapsulation clones: digestion, extraction, overnight ligation
Progress Report 6-11-2010
Major Accomplishments
- 1/2 clones
RcsB:pBAD18BB:DH10b colony PCR
Plans for next week
- Acid survival tests (growth curves and acid dunk)
- pH promoter (RFP and error prone PCR)
- get encapsulation clones
- more encapsulation research
- alkaline lysis and digestion of C3 of above colony PCR
6-3-2010
- Got out of Jury Duty
- Made silent point mutation primers for pBAD33 (extra EcoRI)
- Map of LacZ - wrong part
- Liquid Cultures
6-4-2010
- Map (no cut) of pBAD clones
- encapsulation clones: Miniprep, digestion, gel extraction (wrong)
6-7-2010
- advisor meeting
- encapsulation clones to ligation
6-8-2010
- transformation and plating of encapsulation clones
6-9-2010
- transformation and plating of encryption clones
6-10-2010
- screening of pBAD clones - colony PCR
- encapsulation research
Progress Report 6-18-2010
Major Accomplishments
- Identified and verified next set of parts for cloning
Plans for next week
- screen more clones (YgiV and RfaI)
- pt mutations of 18 and 33
- pH promoter + RFP
- pBAD series + RFP
- YgiV and RfaI in pBADs
6/11/10
- Colony PCR pH promoter+RFP:pBAD35:DH10b
- Sequencing rxn of pBADBB [18,33,35]
- Planned Map of new ordered parts
6/14/10
- Mapping of new plates of biobrick vector pBADs
- primer Design of 6 new primers for two well characterized encapsulation genes
- Restriction Map of 9 new parts - all correct
6/15/10
- Miniprep of new parts, rcsB clone, and pBADBBs
- Restriction map of more parts - ??
6/16/10
- Ligation of RfaI:pBAD35BB
- Website and Logo
6/17/10
- Restriction map of iffy parts
- Tranformation and plating of RfaI:pBAD35BB:DH10b
- PCR, Digestion, cleanup of RFP for pBAD characterization - fail after cleanup
- Ran mary's gel with 2x concentration of DNA
- ReDigestion of pBAD35BB
6/18/10
- colony PCR of RfaI:pBAD15BB:DH10B x10- fail
- ReDigest and extract pBAD35BB
Progress Report 6-25-2010
Major Accomplishments
- Discovered flaw in pBAD35BB:
- PstI cut site in inactive
- Sequencing data shows that the PstI cutsite is missing a single basepair
- Completed new pBAD35BB
- No point mutation is required for pBAD33BB:
- Extra EcoRI cut site in inactive in both the original 33 and our biobrick version
- Q: Do you know anything about a point mutation your lab did or why this is? (DamI methylation?)
- New and complete planning of cloning, experiments and parts: Project Plan
6-20-2010
- EcoRI, XbaI, SpeI, PstI digestion of pBADBB 18, 33, 35
- 35 has inactive PstI
- 33 has inactive extra EcoRI
6-21-2010
- Alkaline Lysis and Digestion of RcsB:pBAD18BB - WRONG
- this is odd: colony PCR said otherwise
- confirmation digestion of 33BB and original and 35 from yesterday
- confirmation of faulty 35 PstI from sequencing data
- New digestion protocol uses less reagents
6-22-2010
- pBAD35 - around the world PCR, DpnI digest, PCR clean up, XbaI digest, PCR cleanup, Ligation, transformation, plating
- colony PCR of direct genes: wz, wzT, yjb, yjbT
6-23-2010
- got 3 genes from colony PCR of direct genes (not yjb)
- pBAD34 - around the world PCR, DpnI digest, PCR clean up, XbaI digest, PCR cleanup, Ligation, transformation, plating
- Phussion PCR from colony PCR template
6-24-2010
- Finished organizing and typing project plan
- Liquid Cultures of pBAD35BB and pBAD34BB
- Initial digestion of pBAD35BB - clones successful
- SpeI cuts clones once and no cuts on originals
- File:222.jpg
- Ran PCR off of colony PCR as Template - FAIL (use colony PCR next time)
6-25-2010
- Alkaline lysis of pBAD35BB and pBAD34BB
- Secondary digestion of pBAD35BB - Successful
- CLONES - BBcutsits=once, KpnI=no cut
- ORIGINAL - KpnI=once
- File:222.jpg
- Initial digestion of and pBAD34BB - Fail
Progress Report 7-2-2010
Major Accomplishments
- Decided the pBAD vectors were a lost cause
- New Project Plan
- 2 clones RcsB+RcsA and pLacI+RBS+YgiV on my first two tries without pBAD vectors
- Clones assigned to team
- Created clones box and updated completed parts
Plans for next week
- Clone
- New LuxR Rev primer that includes stop codon
6-28-2010
- cloning of RcsA downstream of RcsB in iGEM vector pSB1AK3
6-29-2010
- Successful cloning of RcsB+RcsA - Colony PCR
- 400px
- columns 2 and 4 show correct banding for B+A
- columns 1 and 3 show correct banding for B
- caps in PCR were not tight and 5-12 became dehydrated
- cloning of YgiV downstream of pLacI+RBS in iGEM vector pSB1AK3
- cloning of RfaI downstream of pLacI+RBS in iGEM vector pSB1AK3
6-30-2010
- pBAD vectors have given us too much trouble. Time to move on.
- New project plan
- Project Plan
- No pBAD vectors
- Better incorporation of parts offered by registry
- Correct usage of ribosome binding sites
- Ordered and transformed all nessesary parts from registry
7-1-2010
- Finished new project plan
- Colony PCR of cloning from 6/29
- Success - pLacI+RBS+YgiV - bottom ~700bp
- Fail - pLacI+RBS+RfaI - top ~1300bp
- 400px
- Liquid cultures of transformed parts and successful clones
7-2-2010
- Miniprep of 7 Parts from Registry
- Cloning of K112808 (lysis cassette + T) downstream of B0034 (RBS) in iGEM vector pSB1A2
- Cloning of I13507 (RBS+mRFP+TT) downstream of R0065 (InducibleRepressiblePromoter) in iGEM vector pSB1A2
- for both clonings, backbones cut but inserts were undigested.
Progress Report 7-9-2010
Major Accomplishments
- Clone: K200021+C0051
- wrong parts: K112808 and I13507 (both important parts)
- All code for wiki done, just need to fill it in and link to home
Plans for next week
- clone
7-5-2010
- Digestion of K112808 and I13507
- 2nd Proof-Digestion: clones 1 and 2
- Sequencing rxn of clones 1 and 2
7-6-2010
- Digestion
- Magnetic Bead cleanup and submission for sequencing
7-7-2010
- Cloning of C0051 (Repressor and Deg Tag) downstream of K200021(LacI promoter + RBS) in iGEM vector pSB1AK3
7-8-2010
- Colony PCR of clone from yesterday
- 200px
- Band = 825 + 144 = 970
- Liquid culture colony#5, colony #6, K112808, I13507
- Went to CS for programing help
7-9-2010
- Alkaline Lysis of colony#5, colony#6, K112808, I13507
- Double digest of above parts
- 2nd proof-digest of above clones
- Kit Miniprep of colony#6
- Cloning of above clone in front of B0034(RBS) and B0015(TT) - Digestion, Ligation
Progress Report 7-16-2010
Major Accomplishments
Plans for next week
Progress Report 7-23-2010
Major Accomplishments
Plans for next week
Progress Report 7-30-2010
Major Accomplishments
Plans for next week
Progress Report 8-6-2010
Major Accomplishments
Plans for next week
Progress Report 8-13-2010
Major Accomplishments
Plans for next week
Progress Report 8-20-2010
Major Accomplishments
Plans for next week
Progress Report 8-27-2010
Major Accomplishments
Plans for next week
Progress Report 9-3-2010
Major Accomplishments
Plans for next week
