Team:Penn/Notebook
From 2012.igem.org
(Difference between revisions)
Line 619: | Line 619: | ||
<li>Order AI-2</li> | <li>Order AI-2</li> | ||
<li>Order Crystal Violet Stain</li> | <li>Order Crystal Violet Stain</li> | ||
- | < | + | <li>Plan ClyA experiment in JMOutline</li> |
</ul> | </ul> | ||
</li> | </li> | ||
</ul> | </ul> | ||
<br> | <br> | ||
+ | |||
+ | |||
+ | |||
+ | <p><b>July 30</b></p> | ||
+ | |||
+ | <p>Wet Lab:</p> | ||
+ | <ul> | ||
+ | <li>Avin - Transform pBAD33 and pSB4A5, Inoculate BL21 Intein colonies</li> | ||
+ | <li>Redo the test cuts for pDawn and pDawn-ClyA-RFP with XmaI and ClaI on a 0.7% gel</li> | ||
+ | </ul> | ||
+ | |||
+ | <p>Dry Lab:</p> | ||
+ | <ul> | ||
+ | <li>Avin - Human Practices</li> | ||
+ | <li><ul>Mike - Primers | ||
+ | <li>pET26b-ClyA (IDT) keeping pelB with 6xHis C terminus - use NcoI on forward primer, figure out reverse</li> | ||
+ | <li>pET26b-ClyA (IDT) removing pelB with 6xHis C terminus - use NdeI on forward primer, figure out reverse</li> | ||
+ | <li>pet26b-ClyA+RFP keeping pelB with 6xHis C terminus - use NcoI on forward primer, figure out reverse</li> | ||
+ | <li>pet26B-CLlyA+RFP removing pelB with 6x His C terminus - use NdeI on forward primer, figure out reverse</li> | ||
+ | <li>fix frame shift in pDawn and include 6xHis N terminus - use NdeI on forward primer, figure out reverse</li> | ||
+ | <li>ClyA </li> | ||
+ | <li>mCherry</li> | ||
+ | <li>ClyA-RFP</li> | ||
+ | <li>Cph8 primers - figure out pJT106b primers</li> | ||
+ | </ul> | ||
+ | </li> | ||
+ | </ul> | ||
Revision as of 11:58, 15 September 2012
June 2012 Notebook
Week 1
June 6th
- Set up some lab equipment
- Autoclaved for a while
- Organized biobrick stuff
- Called Vinoo about DNA planning
June 7th
- Transformed Cph8, pLsr, and LuxS
- Placed order with Vinoo
- Developed idea using PGY/PCN system to activate a gene
Week 2
June 11th
Wet Lab
- PCR'd mCherry from NAS157
- Ran 1% Gel and purified product
Dry Lab
- Designed primers for LsR promoter
- Meeting with Dr. Sarkar
June 12th
Wet Lab
- Digested mCherry PCR product with BamHI and NotI
- Column purified mCherry and ligated into NAS152 backbone
- Transformed NAS152-mCherry into DH5alpha
- Poured 25 LB-Kan plates
Dry Lab
- Research more information about bacterial drug delivery system
- More research into biofilm project
June 14th
Wet Lab
- Fill in later....
Dry Lab
- Met with Dr. Goulian, obtained pDawn and pDusk
- Identified inaK as a surface display gene we can use
Week 3
June 18th
Wet Lab
- Miniprep pDawn and pDusk
- Test cut pDawn and pDusk with XmaI, analytical gel was correct
- Prep cut pDawn and pDusk with BamHI and NotI, gel purified
Dry Lab
- Ordered and picked up PCR purification kit from cell center
- Additional orders through cell center
- Designed primers for one of Peter's components (forgot which)
June 20
Wet Lab
- Picked 2 colonies of pDawn-mCherry, innoculated in 5 mL of LB and 50 ug/mL of Kan
- PCR purified fragments (Peter), then ran gel?
Dry Lab
- Researched DARPin binding domains and linkers
- Finalized some biobrick orders
- Finalized synthesis order (minus linker)
Week 4
June 22
Wet Lab
- Ashwin - Repeated miniprep on pDawn and did test cut
- Peter - Miniprepped pet26b and digested with BglII and EcorRI
- Avin - Miniprepped pet26b, made glycerol stock and digested with BamH1 and Not1
Dry Lab
- Avin - Finalized and sent in synthesis order (still awaiting order confirmation)
June 25
Wet Lab
- Ashwin/Avin - Column purification, ligation, and transformation of Pet26b-mCherry
- Peter -run gel of eGFP/plsr ligation
Dry Lab
- Avin - Sent in final gene synthesis order
- Mike - reviewed pDawn protocol, reviewed TetR sequences
- Peter- Order restriction enzymes from cell center
June 26
Wet Lab
- Avin - Picked colonies for Pet26b-mCherry and pJT106b
- Mike/Ashwin - Plated pJT122
Dry Lab
- Everyone - Brainstormed human practices, Wiki design
June 27
Wet Lab:
- Miniprepped pet26b-mCherry and pDawn-mCherry
- Test cut pet26b-mCherry with HindIII and ClaI (picture temporarily saved in MEAM folder of pqiao account), bands looked okay, chose C2 for remainder of experiments and made a glycerol stock, transformed both pet26b-mCherry and pDawn-mCherry into BL21(DE3)- Gold (10 ul cells, ~1ng DNA) Plated 200 ul and 20 ul
- Inoculated colonies for pJT122, pJT106b, PhyB (BBa), PIF3 (BBa), and Cph8 (BBa)
Dry Lab:
- Started exploring possible wiki designs and coding
June 28
Wet Lab:
- Miniprepped pJT122, pJT106b, PhyB, PIF3, Cph8, made glycerol stocks
- Picked colonies for pET26b-mCherry and pDawn-mCherry, innoculated, grew up, then diluted Measured OD along the way
Dry Lab:
- Set up light and dark incubators
June 29
Wet Lab:
- Tested pDawn-mCherry and pET-mCherry, pDawn-mCherry expressed mCherry only after light induction
- Nanodropped pJT122, pJT106b, PhyB, PIF3, Cph8
- Performed digest of pET-26b, eGFP, and plsr
- Spread Biobrick shipment on Amp plates (lsrR, lsrK)
Dry Lab:
- Opened Bio-Rad shipments
July 2012 Notebook
Week 5
July 2
Wet Lab:
- Transformed ho1 and pcyA BioBricks
- Peter: ligations
Dry Lab:
- Contacted labs for JT2 and pPL-PCB
- Worked on Human Practices
July 3
Wet Lab
- Nothing to be done for drug delivery
Dry Lab
- Avin - digital schematic, helped with primers, read human practices bacterial therapy stuff
- Mike - talked to Dan, developed cloning strategy for getting Cph8 into the pDawn backbone, started primer design
July 5
Wet Lab
- Picked colonies of ho1 and pcyA
- Inoculated pDawn-mCherry cells for timecourse
Dry Lab
- worked on primer design/cloning strategy and talked to Dan
- worked on schematic and wiki
- worked on human practices
July 6-7
Wet Lab:
- Took pDawn-mCherry time course
- Sterilized incubator and TC hood
- Moved lab stuff to small room
- Redesigned primers for plsr & egfp
Dry Lab:
- Contacted FDA contacts for human practices
Week 6
July 9
Wet Lab:
- Inoculated 50mL cultures of pDawn-mCherry
- Set up pH meter, picked up JT2
- Organized lab area
- Made bacterial streaks for biobricks
Dry Lab:
- Ordered mammalian cell culture media
- Finalized wiki template
- Worked on cloning steps for cph8
July 10
Wet Lab:
- Did time course for pDawn-mCherry, but since it was from a glycerol stock, saw no growth → will let grow overnight, then dilute in the morning and start a new time course
- Picked colonies from transformed Biobricks and innoculated
- Resuspended ClyA and LuxS IDT DNA and transformed into DH5alpha
- TC/Sterile practice training
Dry Lab:
- Ordered primers for ClyA-RFP, Peters primers
- Worked on wiki
- Emailed Tabor for pJT106b plasmid map
July 11
Wet Lab:
- Recorded BL21 pDawn-mCherry growth curve and calculated doubling time
-
- Miniprepped biobricks
- BBa_K265008 - Ice Nucleation Protein NC
- BBa_K523013 - Plac + INP-EYFP
- BBa_K299810 - B0032 + Invasin
- BBa_K257010 - ClyA + RFP
Dry Lab:
- Worked on biofilm project schematic
- More work on wiki
July 13
Wet Lab:
- Diluted to OD600=0.01 and take 0-8hr time points of pDawn-mCherry fluorescence time course
- Thawed out HEK293T cells
Dry Lab:
- Worked on wiki/schematic
July 17
Wet Lab:
- Re-ligation of pDawn with IDTClyA and ClyA-RFP, Transformation into DH5alpha/XO1blue
- Performed PCR of plsr & gfp w/new primers.
- Picked colonies of T7 and INPNC-DARPin
Dry Lab:
- Designed experiments for ClyA and INPNC-DARPin assays
Week 7
July 16
Wet Lab:
- Transformed INPNC-DARPin and T7 BioBrick
Dry Lab:
- SAAST presentation
- Met with Lazzara lab to discuss DARPin experiments
July 18
Wet Lab:
- Re-inoculated T7 and INPNC-DARPin
- PCR ClyA-RFP, Gel purify PCR ClyA-RFP product
Dry Lab:
- Worked on DARPin assay experiment design
July 19
Wet Lab:
- Trypan Blue Assay
- Digested pDawn-mCherry with BamHI, NotI, pDawn-mCherry with BamHI,Digest pDawn-mCherry with NotI, Digested IDTsmart-ClyA with BamHI, NotI (Gel for Digests showed possible degeneration of NotI enzyme...)
- Ligated pDawn backbone (old) with 1) ClyA and 2) ClyA-RFP and Ligated pDawn backbone (new) with ClyA and ClyA-RFP, as well as pDawn old backbone with H20 and pDawn new backbone with H20 (ligation controls)
- Transformed all of above ligations into DH5alpha
July 23
Wet Lab:
- Ashwin-Design test cuts for pDawn-Clya, pDawn-ClyA+RFP
- Ashwin-Digest pDawn-ClyA+pDawn-ClyA+RFP, Run on gel
- Nikita - Miniprep pDawn culture in Sarkar cold room
- Digest of pET-26b w/ BglII, EcoRI-Peter
- Digest of plsr product w/ BglII, PseI-Peter
- Digest egfp w/ SpeI, EcoRI-Peter
- Ligate & transform pET-26-plsr-GFP-Peter
- Digest INPNC-DARPin
- Avin - Try to rescue 293T cells after CO2 arrives if can’t be rescued, thaw out more 293T
- Transform pET-26b-luxS - Peter
- Avin - pick GAVPO
Dry Lab:
- Ordered AI-2 ASAP-peter
- Nikita - Researched whether ClyA is toxic to E. coli BL21, JT2, DH5 alpha, and whether it is secreted in these strains
- Read Daphne+Dr. Sarkar’s ligation paper
- Avin - Buy:
- DH5 alpha
- 20 kan plates, 10 amp plates
- Cell Counter
- Write out competent cell production protocol-Peter
- Obtained BL21 transformation protocol from daphne/find it-Peter
- Avin - Logo design, human practices
- Ashwin - wiki
July 24
Wet Lab:
- Pick colonies of pDawn-ClyA and pDawn-ClyA+RFP (DH5alpha)
- Avin - Picked 2 colonies (light+dark) of pDawn-ClyA+RFP (BL21), set up pDawn culture experiment, check on HEK293T and passage into 6 well plates if confluent
- Avin - Ran Gel, no DNA
Dry Lab:
- Peter: order the promoter (or figure out an alternative method..)
- Ashwin: wiki
- Avin - Edit/Order primers for HA tag and His tag, design pDawn-ClyA experiments, human practices
- Nikita - Write human practices
Week 8
July 26
Wet Lab:
- Avin - Finish ClyA-RFP time course, collect ClyA supernatant, measure fluorescence of ClyA-RFP triplicates, spin down + pictures if red, Miniprep of DARPin, possible ClyA assay
- Peter- ligation, transformation, plating of ligations, help Avin with ClyA cell lysis experiments
- Transform luxS6-8 into BL21
- Nikita - Miniprep GAVPO and DARPin
Dry Lab:
- Avin - Call IDT at 9am, order blood agar plates, nissl stuff after we do background research
- Ashwin - wiki, research getting recombinant ClyA
- Nikita - Human practices, Nissle research, plan experiments
- Peter
- Complete FDA writeup
- Order ATCC Strains
- Order lss primers
- Order AI-2
- Order Crystal Violet Stain
- Plan ClyA experiment in JMOutline
July 30
Wet Lab:
- Avin - Transform pBAD33 and pSB4A5, Inoculate BL21 Intein colonies
- Redo the test cuts for pDawn and pDawn-ClyA-RFP with XmaI and ClaI on a 0.7% gel
Dry Lab:
- Avin - Human Practices
- Mike - Primers
- pET26b-ClyA (IDT) keeping pelB with 6xHis C terminus - use NcoI on forward primer, figure out reverse
- pET26b-ClyA (IDT) removing pelB with 6xHis C terminus - use NdeI on forward primer, figure out reverse
- pet26b-ClyA+RFP keeping pelB with 6xHis C terminus - use NcoI on forward primer, figure out reverse
- pet26B-CLlyA+RFP removing pelB with 6x His C terminus - use NdeI on forward primer, figure out reverse
- fix frame shift in pDawn and include 6xHis N terminus - use NdeI on forward primer, figure out reverse
- ClyA
- mCherry
- ClyA-RFP
- Cph8 primers - figure out pJT106b primers
Retrieved from "http://2012.igem.org/Team:Penn/Notebook"