Team:Penn/Notebook
From 2013.igem.org
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<li>21-Jun</li> | <li>21-Jun</li> | ||
<ol> | <ol> | ||
- | <li> | + | <li>troubleshoot plux-luxI pcr</li> |
<li>roubleshoot pdawn-luxI pcr</li> | <li>roubleshoot pdawn-luxI pcr</li> | ||
<li>made pDawn-tetR pcr work</li> | <li>made pDawn-tetR pcr work</li> | ||
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<li>digested t9002 in amp and ptet gfp in amp to identify the correct ligation</li> | <li>digested t9002 in amp and ptet gfp in amp to identify the correct ligation</li> | ||
<li>all of the chosen ptet gfp ligations worked, but let's not use 5 || 13 12. troubleshoot t9002 digest</li> | <li>all of the chosen ptet gfp ligations worked, but let's not use 5 || 13 12. troubleshoot t9002 digest</li> | ||
+ | <li>troubleshoot t9002 digest</li><ol> | ||
+ | <li>check for contamination of something (run uncut sample, sample + buffer, sample + 1 | ||
+ | enzyme, sample + other enzyme, sample + both enzymes)</li> | ||
+ | </ol> | ||
</ol> | </ol> | ||
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<div class="tab-pane" id="tab2"> | <div class="tab-pane" id="tab2"> | ||
- | < | + | <ul> |
+ | <li>1-Jul</li> | ||
+ | <li><ol> | ||
+ | <li>Beautiful Brady Bunch photoshoot</li> | ||
+ | <li>Troubleshooted and Re-tred PCR for user ends for reporter plasmid</li> | ||
+ | <li>Called IDT about pcr assembly – they said Gibson tends to work better, no mutations, all in one tub. If we must PCR assembly – add DMSO, hotstart reaction, anneal at 68-70C (we did this).</li> | ||
+ | <li>Get methylated biobrick sequenced </li> | ||
+ | <li>Only sequence ptet GFP 11, if verified make sure to note on LIMS that we are only using ptet GFP 11 </li> | ||
+ | <li> Check if plux/luxI system is working in liquid cultures – this failed </li><ol> | ||
+ | <li>a. Might be strain competition, need to know growth rates</li> | ||
+ | </ol> | ||
+ | <li>Re-suspend primers for lux amplifier </li> | ||
+ | <li>Mini-prep: e0040, psb1a3, r0062</li> | ||
+ | </ol></li> | ||
+ | |||
+ | |||
+ | <li>2-Jul</li> | ||
+ | <li><ol> | ||
+ | <li>Think about application of mathylation project in e.coli</li> | ||
+ | <li>Ceck if plux/GFP-psb1C3 system is working in liquid cultures</li><ol> | ||
+ | <li>+/- AHL induction at 100nM</li> | ||
+ | <li>Compare with ptetGFP fluorescence, normal LB fluorescence</li> | ||
+ | </ol> | ||
+ | <li>Streak zinc finger 2</li> | ||
+ | <li>Grow up 44251</li> | ||
+ | <li>Transform up R0062</li> | ||
+ | <li>When BstuI arrives</li><ol> | ||
+ | <li>Assay BstuI working</li> | ||
+ | <li>Assay the bvluc and tale1 minipreps in dh5a, dam-, and bl21 cells with msssi and bstuI </li> | ||
+ | <li>Results: BstUI is blocked by methylation, and cells don’t normally methylate</li> | ||
+ | </ol> | ||
+ | <li>Growing up t9002 in chlor and i751250 in amp for fluorescence study</li> | ||
+ | <li>Investigate CHIP or other ways of determining DNA binding domain specificity </li> | ||
+ | </ol></li> | ||
+ | |||
+ | <li>3-Jul</li> | ||
+ | <ol> | ||
+ | <li>Streak zinc finger 2 </li> | ||
+ | <li>Grow up 44251 </li> | ||
+ | <li>Look into lux box being light sensitive </li> | ||
+ | </ol> | ||
+ | |||
+ | <li>4-Jul</li> | ||
+ | <ol> | ||
+ | <li>Mini prep 44251 </li> | ||
+ | <li>Pick ZFP2 colonies to grow up, throw out liquid culture in fridge </li> | ||
+ | </ol> | ||
+ | |||
+ | <li>5-Jul</li> | ||
+ | <ol> | ||
+ | <li>Repeat BstUI assay, taking into account new controls</li> | ||
+ | <li>Suspend the primers in the freezer </li> | ||
+ | <li>We need to check if the origin of replications are compatible before co transformation</li> | ||
+ | <li>Characterize pDawn-mcherry </li> | ||
+ | <li>Practice measuring fluorescence</li> | ||
+ | </ol> | ||
+ | |||
+ | |||
+ | <li>6-Jul</li> | ||
+ | <ol> | ||
+ | <li>troubleshoot ptetGFP user PCR - band was visible but too small to extract</li> | ||
+ | <li>gel extract promoter fragments from USER PCR</li> | ||
+ | <li>re-do USER PCR for: TetR, pTetGFP</li> | ||
+ | <li>Design/check/order (Tale,Cas,ZFP)-flex-REV primers - check fwd primers</li> | ||
+ | </ol> | ||
+ | </ul> | ||
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Revision as of 10:57, 10 July 2013
- 4-Jun
- Learned how to make competent cells, growing up two strains for tomorrow
- Transformed 8 plasmids
- Determined EL222 fusion is risky but still going ahead with it
- Linkers are totally setlled
- Found zinc finger plasmid and updated target sequence
- Learned how to make tetr- mcherry fusion
- Settled on 5 promoters
- 5-Jun
- Learned how to make competent cells, testing them and then making more tomorrow
- Transformed 8 plasmids again
- Made primers to clone the TET-GFP reporter system, the mCherry promoter strength system, ready to order
- Made ultramers for variable promoter blocks (and no target neg controls) – ready to order
- Spilled a lot of iced tea outside, bummer
- Started primers for dna binding machines
- Got a handle on cas9 fusions (pun intended).
- Put awesome pics in dropbox
- 6-Jun
- Clean up dropbox
- Update budget sheet with addgene and cell center orders
- Finish primers for fusion
- Set up plate reader for GFP and mCherry assays
- run minipreps on pdawn, pdawn-mcherry, pet26b
- Grow up mCherry stock
- Wrote Penn iGEM on our plasmid
- 7-Jun
- Transform
- C0012 –amp/chlor (do both)
- M11307 – amp/chlor (do both)
- I13458 – amp/chlor (do both)
- R0010 – amp/chlor (do both)
- R0051 – amp
- K206000 –chlor
- Start the LIMS and file all the strains and DNA we have made/ ordered
- Mini-preped
- I9002
- I13458
- C0051
- Pdawn-mcherry
- Pdawn
- Pet26b
- Dhsa mcherry
- Pdawn dhsa
- Psb1a3
- JM mcherry
- 8-Jun
- Miniprep Addgene stuff + transformations that worked
- Growing up low copy plasmids in 40mLs
- 8-Jun
- Miniprep Addgene stuff + transformations that worked
- Growing up low copy plasmids in 40mLs
- Transformed everything that has failed
- 17-Jun
- Grow up luxI culture and grow up tetR culture
- Sequence all of the minipreps
- Transform t9002 in psb1A3 in NEB10
- Retransform ptetGFP to see if BL21DE3 cells are competent
- Transform r0079, k081015, r0063 in NEB10
- Miniprep psb1k3
- Redo dam gel with more dna
- Figure out second control zfp from addgene
- Figure out how to add luxR binding site to target region
- Order sequencing primers for all addgene minipreps
- Bisulfite converted msssi methylated c0051
- 18-Jun
- The bisulfite conversion was missing a negative control (bisulfite converted but unmethylated c0051) we'll need this to interperet results
- Miniprep c0078, c0079 + make glycerol stocks check same plasmid with our kit
- Order 13420 (second zfp)
- Design a way to make variable promoters more easily varied (for a biobrick so teams can use the reporter plasmid for their own nefarious reasons)
- 19-Jun
- Transform failed transformation
- Make competent DH5a && Dam-
- Figure out methylation assays for promoters
- Miniprep psb1A3 && all the 40mL cultures
- Picked many colonies
- Check pTet-gfp under blue light
- 20-Jun
- run plux-luxI pcr
- run pdawn-luxI pcr
- run pDawn-tetR pcr
- run pet26b-tetR pcr and
- run pDawn-GFP pcr
- run pDawn-mCherry-secretion tag pcr
- Nano drop last nightÕs mini preps to check for accuracy
- Culture amp resistant successful transformations
- Make 5 L LB
- Miniprep all the successful transformations w/ new protocol
- 21-Jun
- troubleshoot plux-luxI pcr
- roubleshoot pdawn-luxI pcr
- made pDawn-tetR pcr work
- troubleshoot pet26b-tetR pcr
- troubleshoot pDawn-GFP pcr
- troubleshoot pDawn-mCherry-secretion tag pcr
- miniprep growing cultures, be sure to pick only the glowing ligations
- ransform the correct t9002 amp ligation - determined from gel
- digested t9002 in amp and ptet gfp in amp to identify the correct ligation
- all of the chosen ptet gfp ligations worked, but let's not use 5 || 13 12. troubleshoot t9002 digest
- troubleshoot t9002 digest
- check for contamination of something (run uncut sample, sample + buffer, sample + 1 enzyme, sample + other enzyme, sample + both enzymes)
- 24-Jun
- Dam-/dh5a v dam methylation + dpnI && dpnII digest
- Digested/ligated/transformed t9002 in amp
- Get methylated biobrick sequenced
- get chlor backbones sequenced
- culture t9002 transformations in liquid media with i751250
- mini prep stuff in the incubator
- figure out the primer issues 8
- Pick t9002 colonies for miniprep
- 26-Jun
- Dam-/dh5a v dam methylation + dpnI && dpnII digest
- Digested/ligated/transformed t9002 in amp
- get chlor backbones sequenced
- culture t9002 transformations in liquid media with i751250
- mini prep stuff in the incubator
- figure out the primer issues
- Pick t9002 colonies for miniprep
- USER Cloning reporter plasmid
- 1-Jul
- Beautiful Brady Bunch photoshoot
- Troubleshooted and Re-tred PCR for user ends for reporter plasmid
- Called IDT about pcr assembly – they said Gibson tends to work better, no mutations, all in one tub. If we must PCR assembly – add DMSO, hotstart reaction, anneal at 68-70C (we did this).
- Get methylated biobrick sequenced
- Only sequence ptet GFP 11, if verified make sure to note on LIMS that we are only using ptet GFP 11
- Check if plux/luxI system is working in liquid cultures – this failed
- a. Might be strain competition, need to know growth rates
- Re-suspend primers for lux amplifier
- Mini-prep: e0040, psb1a3, r0062
- 2-Jul
- Think about application of mathylation project in e.coli
- Ceck if plux/GFP-psb1C3 system is working in liquid cultures
- +/- AHL induction at 100nM
- Compare with ptetGFP fluorescence, normal LB fluorescence
- Streak zinc finger 2
- Grow up 44251
- Transform up R0062
- When BstuI arrives
- Assay BstuI working
- Assay the bvluc and tale1 minipreps in dh5a, dam-, and bl21 cells with msssi and bstuI
- Results: BstUI is blocked by methylation, and cells don’t normally methylate
- Growing up t9002 in chlor and i751250 in amp for fluorescence study
- Investigate CHIP or other ways of determining DNA binding domain specificity
- 3-Jul
- Streak zinc finger 2
- Grow up 44251
- Look into lux box being light sensitive
- 4-Jul
- Mini prep 44251
- Pick ZFP2 colonies to grow up, throw out liquid culture in fridge
- 5-Jul
- Repeat BstUI assay, taking into account new controls
- Suspend the primers in the freezer
- We need to check if the origin of replications are compatible before co transformation
- Characterize pDawn-mcherry
- Practice measuring fluorescence
- 6-Jul
- troubleshoot ptetGFP user PCR - band was visible but too small to extract
- gel extract promoter fragments from USER PCR
- re-do USER PCR for: TetR, pTetGFP
- Design/check/order (Tale,Cas,ZFP)-flex-REV primers - check fwd primers