Team:Lethbridge/Notebook/Lab Work/Group1

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* C0040 & B0015 were ligated together in pSB1A3 following the Ligation Protocol 1.  
* C0040 & B0015 were ligated together in pSB1A3 following the Ligation Protocol 1.  
* Both ligations were transformed following the Transformation Protocol 1.
* Both ligations were transformed following the Transformation Protocol 1.
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==April 21, 2011==
 
-
==April 23, 2011==
 
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==April 27, 2011==
 
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==April 28, 2011==
 
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* Under Construction
 
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<i>Minipreps of pBAD-rbs-lumazine-dt & K331033-K331035</i>
<i>Minipreps of pBAD-rbs-lumazine-dt & K331033-K331035</i>
* Minipreps of pBAD-rbs-lumazine-dt & K331033-K331035 were made following the Miniprep Protocol (Modified Bench Protocol: QIAprep Spin Miniprep Kit Using Microcentrifuge).
* Minipreps of pBAD-rbs-lumazine-dt & K331033-K331035 were made following the Miniprep Protocol (Modified Bench Protocol: QIAprep Spin Miniprep Kit Using Microcentrifuge).
 +
 +
== June 29th, 2011==
 +
<i>PCR of pBAD-P0440 in pSB1K3 and P0440 was done using PCR protocol </i>
 +
<i>Assembly of R0010 with B0034 in pSB1C3 </i>
 +
<i> Transformation for pBad-RBS and pBad- P0440 into Dh5a E. Coli</i>
 +
== June 30th, 2011==
 +
<i> Ran 1% Agarose Gel from June 29 PCR of pBAD-p0440 and p0440 </i>
 +
 +
 +
=July=
 +
== July 2, 2011==
 +
<i>Picked Colonies and grew overnight </i>
 +
*4 colonies picked from pBad rbs in pSB1T3
 +
*3 colonies picked from pBad-p0440
 +
*picked 3 colonies from 2 plates of pBAD-P0440 in pSB1C3
 +
**1 colony picked from plate A, and 2 colonies from plate B
 +
 +
== July 03,2011==
 +
*None of the 4 colonies of pBAD rbs grew, so they were re-grown in the incubator
 +
*Samples of pBAD-p0440 were mini prepped and stored in team 1 DNA box
 +
*Picked 3 samples of pBad- p0440  in psb1C3 and 3 samples of pBAD p0440 in pSB1K3
 +
 +
== July 05,2011==
 +
<i> PCR out inserts from July 03, of pBAD-P0440</i>
 +
*PCR out inserts from July 03, of pBAD-P0440 samples using prefix and antisense suffix primers  and run on agarose gel at 120V to determine if plasmid contains the correct insert, using po440 as a control. 
 +
 +
== July 06,2011==
 +
<i>Repeated July 05, but only for pBad p0440 (2,4)</i>
 +
 +
== July 7th,  2011==
 +
<i>Assembled I13453 with B0034 and into pSB1K3 with J04500</i>
 +
*Assembly done using Restriction, ligation, and transformation techniques
 +
 +
== July 11th, 2011==
 +
<i>Assembly of pLacI-rbs and Lumazine synthase- dt</i>
 +
<i>Plasmid transfer of Ag43</i>
 +
*Assembled pLacI-rbs and Lumazine synthase- dt into destination plasmid pSB1C3, followed restriction digest, ligation, and transformation procedures. 
 +
*Plasmid Transfer of Ag43 from pSB1C3 to pSB1K3 using cut sites EcoRI and PstI
 +
*Ran a 1% Agarose Gel using 0.5 TAE buffer solution for parts BBa-J04500 in pSB1AK3, R0040, and Lumazine synthase-Dt to confirm sizes. Used Restriction procedure, cutting with EcoRI
 +
 +
== July 13th, 2011==
 +
<i>Assembly of K331033 and K331035</i>
 +
*Did a restriction and Gel Extraction for K331033 cutting at EcoRI and SpeI, K331035 cutting at PstI and XbaI, and pSB1K3 cutting at EcoRI and PstI
 +
*Ran the gel for 80 minutes at 120Volts
 +
*Used Transformation protocol to Transformed XylE, XylF, XylT, XylK, XylQ, into Dh5a E. Coli cells
 +
 +
== July 14, 2011==
 +
<i>Ligation of K331033 to K3310335 into pSB1K3</i>
 +
*Performed a ligation of K331033 to K3310335 into pSB1K3 and transformation of ligated parts into Dh5a E. Coli. Used Transformation and ligation protocols. Plated culture on Kanmycin plates
 +
 +
==July 15th, 2011==
 +
<i> Assembly of pLacI –Rbs in pSB1C3 and Lumazine Dt in pSB1AK3</i>
 +
*Assembly of pLacI –Rbs in pSB1C3 and Lumazine Dt in pSB1AK3 using restriction digest and gel extraction protocols
 +
 +
== July 19th,2011==
 +
<i> Assembly of K346007 and J04500 into destination plasmid pSB1C3</i>
 +
*Assembly of K346007 and J04500 into destination plasmid pSB1C3 parts were restricted, ligated and transformed using appropriate protocols. 
 +
*Results: all of the plates had significant bacterial growth, will repeat experiment using LB instead of SOC during transformation 
 +
 +
== July 20th,2011==
 +
<i>Tried to pre-aliquot restriction</i>
 +
*Created a master-mix from appropriately sized aliquots that can be stored in the -20 freezer.  Two mixes were created in the following volumes:
 +
**16micro liters miliQ H2O
 +
**2.5 micro liters Buffer II
 +
**0.5 micro liters BSA 100X
 +
**0.5 micro liters EcoRI
 +
**0.5 micro liters SpeI
 +
**20 micro liters total restriction mixture
 +
 +
== July 25th, 2011==
 +
<i>A Colony PCR was run for Parts K346007 and J04500 to confirm assemblies</i>
 +
* This was done following the colony PCR protocol
 +
 +
== July 26th,2011==
 +
<i>Picking of colonies</i>
 +
*Cells were picked with parts J04500- K346007 in them, for plasmid extraction by miniprep protocol.  23 colonies were picked in total and placed in 5 ml of lb in test tubes, along with 5micro liters of chloramphenicol was added to each test tube.  Picked colonies were placed in the shaker overnight at 37 degrees Celsius
 +
 +
== July 27th, 2011==
 +
<i>Assembly of following parts:</i>
 +
*K331033 to K331035
 +
**J04500 to Lumazine Synthase Dt
 +
**pBad to P0440
 +
**P0440 to K331033
 +
**Lumazine synthase dt to pBad
 +
*A restriction was done using the restriction protocol following a Gel extraction protocol.  A ligation was performed and contents incubated at room temperature for 30 mins. Controls were run with downstream part being substituted as water.
 +
*Restricted J04500-k346007 with EcoRI, and PstI following restriction protocol, to confirm assembly success, restriction were loaded into a 08% Agarose gel. 23 samples from previous day was loaded into gel. Lanes 16 and 17 showed expected sizes
 +
 +
== July 28th,2011==
 +
<i>Ran a PCR gel for Justin to confirm PCR insert was correct</i>
 +
 +
 +
=August=
 +
== August 1st, 2011==
 +
<i> Three colonies picked for parts J45120 and J45320</i>
 +
*3 colonies picked from plates for J45120 and J45320 and were placed in 5 ml test tubes with LB media and 5 micro liters Amp, and placed in shaker overnight
 +
 
 +
== August 03rd, 2011==
 +
<i>Restriction of:</i>
 +
**pBad-P0440 in pSB1A2
 +
**Lumazine Synthase-dt with pBad in pSB1A2
 +
**K331033 – K331035 in pSB1C3
 +
**P0440 – K331033 in pSB1A2
 +
*Confirmation of assemblies by means of Agarose Gel
 +
*Ran Gel at 80 volts for 2 hours
 +
*Conclusion: parts were verified and appear to have been assembled successfully
 +
 +
== August 4th, 2011==
 +
<i>Restriction by protocol of assembling parts :</i>
 +
**J04500-Lumazine synthase-dt out of pSB1AK3 + pbad-P0440 in psb1AK3
 +
**pBad-P0440 out of pSB1A2 + K331033-K331035 in pSB1C3
 +
**Lumazine synthase-dt-pBad pSB1A2 + p0440-K331033 in psb1A2
 +
*J04500 in pSB1Ak3 + Lumazine-synthase-dt-pBad out of pSB1A2
 +
*P0440-k331033 out of pSB1AK3 + k331035 in pSB1C3
 +
*Ran a TAE agarose Gel
 +
 +
==August 11th, 2011==
 +
<i>Assembly of parts:</i>
 +
*pBad-P0440 + K331033-k331035 in pSB1C3
 +
*Lumazine synthase-Dt-pBad + PlacI in pSB1AK3
 +
*Lumazine synthase in pSB1C3 + Dt in pSB1A2
 +
*PlacI in pSB1AK3 + Lumazine synthase in pSB1C3
 +
*Ran a 1X TAE 1% Agarose Gel at 80Volts for 120 min for Extraction of parts by protocol
 +
 
 +
== August 12th, 2011==
 +
<i>Assembly of J04500 to Enhanced Lumazine synthase and Enhanced Lumazine synthase to Dt</i>
 +
*Followed protocols for Restriction, Gel Extraction, Ligation and Transformation,
 +
*Cut J04500 in pSB1AK3 at SpeI and PstI, Cut Enhanced Lumazine synthase at XbaI and PstI
 +
*Cut Enhanced Lumazine synthase at EcoRI and SpeI, Cut Dt in pSB1AK3 EcoRI and XbaI.
 +
*Samples were run on a 0.9% Agarose gel in 1X TAE at 100Volts
 +
*Results: Colonies grew from the J04500-Enhanced Lumazine synthase and Enhanced Lumazine synthase – Dt in pSB1AK3
 +
 +
== August 13th, 2011==
 +
<i>Assembly of PLacI with Agn43 with Dt</i>
 +
<br>Miniprep:
 +
*Dt in pSB1AK3
 +
*J04500 – Agn43 in pSB1AK3
 +
*K346007(Agn43) in pSB1C3
 +
*J04500-Lumazine synthase – Dt pSB1AK3
 +
Ran a Gel of J04500-Ag43 in pSB1A2, and Agn43 in pAB1C3
 +
Assembly of pBad-P0440 with K331033-K331035
 +
*Picked: pBad-P0440 cells, K331033- K331035 in pSB1C3 cells
 +
**left cells to grow overnight in shaker at 37 degrees Celsius
 +
**Picked 6 colonies from Enhanced Lumazine synthase plates from August 12
 +
 
 +
==August 14th,2011==
 +
<i>Mini-prepped:</i>
 +
*pBad –p0440 in pSB1A2
 +
*K331033-K331035 in pSB1C3
 +
*Enhanced Lumazine synthase
 +
**2 minipreps of plated colonies of pLAcI-Enhanced Lumazine synthase
 +
**4 minipreps of plated colonies of Enhanced Lumazine synthase- Dt
 +
<i>Restricted:</i>
 +
*1) J04500 in pSB1AK3 cut at SpeI and PstI
 +
*2) Enhanced Lumazine syhtase –Dt in pSB1AK3 cut at XbaI and PstI
 +
*3) J04500 –Enhanced Lumazine synthase in pSB1AK3 cut at EcoRI and SpeI
 +
*4) B0017 in pSB1AK3 cut at EcoRI and XbaI
 +
*5) J04500-Lumazine synthase –dt cut at EcoRI and SpeI
 +
*6) pBad- P0440 in pSB1A2 cut at EcoRI and XbaI
 +
*7) pBad- P0440 in pSB1A2 cut at SpeI and PstI
 +
*8) K331033-K331035 Cut at Xba1 and PstI
 +
*Ran a Gel extraction by protocol
 +
<i>The previously numbered restrictions were ligated as follows:</i>
 +
*1+2
 +
*3+4
 +
*5+6
 +
*7+8
 +
*Ligations were incubated and transformed then plated on Ampicillin plates following protocols. 
 +
*A 1X TBE 1% Agarose gel was successfully run at 100volts for 50 minutes to confirm parts
 +
== August 15th, 2011==
 +
<i>Assembly of Antigen 43 with PLacI and Dt</i>
 +
<i>Followed Protocol for a restrictions of :</i>
 +
*1) J04500 in pSB1AK3
 +
*2) Agn43
 +
*3) Agn43
 +
*4)Dt in pSB1AK3
 +
*5) J04500-Agn43
 +
*6) Dt in pSB1AK2
 +
 +
== August 16th, 2011==
 +
<i>Verify parts by running them on an Agarose Gel</i>
 +
 +
== August 17th,2011==
 +
Miniprep protocol was followed for enhanced lumazine synthase in pSB1C3, all 5 ml of culture was used 
 +
Restriction of:
 +
*Enhanced Lumazine synthase dt, J04500 + enhanced lumazine and Enhanced lumazine. 
 +
*Restricted parts were run on a gel to confirm parts.  Gel ran at 80Volts for 90 minutes
 +
*Enhanced lumazine synthase was confirmed,
 +
*J04500-Enhanced lumazine synthase confirmed
 +
*Enhanced Lumazine synthase –Dt  did not confirm
 +
<i>Assembly of J04500-enhanced Lumazine synthase +DT </i>
 +
<i>Did a restriction following protocol of:</i>
 +
*1) J04500 – Enhanced Lumazine synthase out of pSB1AK3  Cut at EcoRI and SpeI
 +
*2) B0017 in pSB1AK3 Cut at EcoRI and XbaI
 +
<b>Ran restricted parts on an Agarose Gel: No DNA was able to be observed outside ladder</b>
 +
 +
== August 18th,2011==
 +
<i>Assembled the complete Lumazine synthase and florescent proteins construct</i>
 +
*Repeat August 17th: Restriction, Gel extraction, Ligation and Transformation
 +
*Did a Restriction following protocol of:
 +
**1) J04500-Enhanced lumazine synthase in pSB1AK3 cut at EcoRI and SpeI
 +
**2) B0017 in pSB1AK3 cut at EcoRI and XbaI
 +
**3) J04500-Lumazine synthase – Dt Cut at EcoRI and SpeI
 +
**4) Dt in pSB1C3 cut at EcoRI and XbaI
 +
*Restrictions were run on an Agarose Gel, only parts 1), and 2) were observed on the Gel
 +
Restrictions and Gel were run again for missing parts; restriction time was decreased; no parts were shown on Gel
 +
 +
== August 20th, 2011==
 +
<i>Assembly of Construct:</i>
 +
*J04500- Lumazine synthase-dt-pBad-P0440- K331033-K331035
 +
*The following protocols were used to assemble this construction:  Restriction, Gel Extraction, Ligation and Transformation
 +
<i>Restriction of:</i>
 +
*1) J04500-Lumazine synthase-dt cut out of pSB1AK3 at EcoRI and SpeI
 +
*2) pBad- P0440-K331033-K331035 in pSB1C3 cut at EcoRI and XbaI
 +
*Restrictions were run on a 1% Agarose 1X TAE Gel for purpose of extraction
 +
*DNA did not show on Gel
 +
 
 +
== August 21st,2011==
 +
<i>Assembly of construct:</i>
 +
*J04500-Lumazine synthase dt-pBad-P0440-K331033-K331035
 +
*Repeated previous day’s work. The parts had been confirmed by sequencing 
 +
*Picked Colonies from plate for parts J04500-Enhanced lumazine synthase in pSB1AK3 and grew overnight in LB for purpose of Glycerol stocks
 +
*Gel of parts worked and a successful Gel extraction was performed.  Extracted parts 1) and 2) from August 20th that were ligated together
 +
*Ligated parts were transformed into Dh5alpha and plated on appropriate antibiotic selected plates
 +
 +
== August 22, 2011==
 +
<i>Picked J04500-Enhanced Lumazine synthase colonies from plated construct</i> 
 +
<b>Assembly of Constructs:</b>
 +
**1) XylE cut at EcoRI and SpeI
 +
**2) S04261 Cut at EcoRI and XbaI
 +
**3)K331007 cut at EcoRi and XbaI in pSB1C3
 +
**4) mms6 cut at EcoRI and SpeI
 +
**5) K3301007 in pSB1C3 cut at SpeI and PstI
 +
**6) mms6 Cut at XbaI and PstI
 +
**7) K331008 in pSB1C3 cut at SpeI an dPstI
 +
**8) mms6 cut at XbaI and PstI
 +
**9) K331009 in pSB1C3 cut at SpeI and PstI
 +
**10) mms6 cut at XbaI and PstI
 +
**11) K331012 in pSB1C3 cut at SpeI and PstI
 +
**12) mms6 cut at XbaI and PstI
 +
**13) S04261 pSB1AK3 cut at EcoRI and XbaI
 +
**14) mms6 cut with EcoRI and SpeI
 +
*Parts were run on an Agarose Gel for Gel extraction
 +
*Gel was successful and a Gel Extraction was performed. 
 +
<i>Following parts were ligated together as per protocol</i>
 +
*1 + 2
 +
* 3 + 4
 +
*5 + 6
 +
* 7 + 6
 +
* 9 + 6
 +
* 11 + 6
 +
*14 + 4
 +
<b> Ligations were transformed via protocol into Dh5 alpha, plated, and left in incubator overnight</b>
 +
 +
*Performed a Concentration of Enhanced lumazine synthase from Sephacryl 400 Chromatography
 +
*Pooled fractions at 35, 36 ,37 
 +
*Vivaspin 20, 3000 mwco reviled with 17.5 ml dd milliQ H20, spun at 4000Xg for 25 minutes
 +
*The column was then washed with 10 ml of sodium phosphate buffer, at 4000Xg for 40 minutes
 +
*7.5ml of Fractions 35,36,37,were loaded onto column and concentrated to 1ml by Centrifuge at 4000XG at 4Degrees Celsius for about an hour in 5 minute increments
 +
*Concentrations to be determined photometrically and concentration must be determined and protein visualized Via SDS page gel
 +
 +
==August  28th, 2011==
 +
<i>Over expression of complete construct</i>
 +
*Overnight culture grown by Justin, 12ml of overnight culture, of E. Coli Dh5alpha J04500-K249002- B0017- I13453-P0040-K331033-K331035, in the pSB1C3 Vector, was inoculated in 4 x 500ml LB flasks, with 500micro liter of Chloramphenicol and grown up to OD600 of 0.0978
 +
 +
== August 29th, 2011==
 +
*Ran SDS page of August 28th, overexpression, SDS sample preparation protocol was followed
 +
*The SDS page was run at 80Volts for 15 mins and 180Volts for 45mins
 +
*Stained in Coomassie blue for 30 mins and distained over night
 +
 +
==August 31, 2011==
 +
<i>Assembly of:</i>
 +
*J04500-Enhanced Lumazine synthase cut out of pSB1AK3 at EcoRI and SpeI ligated to B0015 cut at EcoRI and XbaI in pSB1AK3 
 +
*Ptet-rbs in pSB1A2 cut at SpeI and PStI Ligated to XylE - arginine tag cut at XbaI and PstI.
 +
<i>Followed Restriction, Gel Extraction protocols</i>
 +
**Note: J04500 –Enhanced Lumazine synthase and Xyle – agrinine tag –dt did not Cut out of plasmid.  B0015 in pSB1AK3, and Ptet-rbs in pSB1A2 were found around the right sizes
 +
 +
 +
=September=
 +
== September 3rd, 2011==
 +
<i>Repeated August 31 assembly</i>
 +
 +
== Sept 14th,2011==
 +
<i>Show how effective BamHI is in degrading E.coli DH5α Genomic DNA</i>
 +
*2 overnight cultures were picked in 50 ml flasks with 50micro liters of Ampicillin and were inoculated with BamHI and pLacI from Glycerol stock
 +
*16ml of pLacI from overnight culture were used to inoculate 250ml of Lb with 250micro liters of Ampicillin to bring it to an OD600 of 0.118
 +
*11.2 ml of BamHI overnight culture was used to inoculate 250ml of LB to an OD600 of 0.100
 +
 +
== September 17th, 2011==
 +
<i>Repeat, the August 14th BamHI experiment due to the spectrophotometer being inaccurate</i> 
 +
== September 19th, 2011==
 +
<i>Isolation of genomic DNA from BamHI cells by following the Qiagen Blood and Tissue Kit protocol for isolating genomic DNA of gram-negative bacteria </i>
 +
 +
== September 21, 2011==
 +
<i>Overnight culture of full construct (lumazine synthase – K331033 – K331035, K331033 and K331035) for FRET experiments</i>
 +
*Selected cells were induced with arabinose.
 +
*All cells showed growth after 15 hours in shaker at 37 degrees Celsius.
 +
 +
== September 22, 2011==
 +
<i>Continued work from September 21</i>
 +
*Spun down cells and re-suspended in LB media and checked Optical Density of 1 ml of culture and brought them to 1 OD
 +
*Signs of FRET but nothing confirmed
 +
**Note: This is something we will be working on continuously up until Boston

Latest revision as of 03:32, 29 September 2011





Contents

April

April 1, 2011

Confirmation Gel of I1343, B0034, C0040 & B0015

  • Each of I1343, B0034, C0040 & B0015 were restricted following the Restriction Protocol 4.
  • A gel was made following the 1% Agarose Gel Protocol (100mL).
  • The restrictions were loaded onto the gel with a 1kb ladder and 100bp ladder.
  • The gel ran at 120V for 60 minutes.
  • The gel was then stained in Ethidium Bromide for 10 minutes.
  • Results: The parts were confirmed with the correct sizes.

April 2, 2011

Assembly of I1343 & B0034 and C0040 & B0015

  • Each of I1343, B0034, C0040 & B0015 were restricted following the Restriction Protocol 1 where all odd parts are upstream and even parts are downstream.
  • I1343 & B0034 were ligated together in pSB1A3 following the Ligation Protocol 1.
  • C0040 & B0015 were ligated together in pSB1A3 following the Ligation Protocol 1.
  • Both ligations were transformed following the Transformation Protocol 1.


May

May 18, 201

Transformation of P0440 in pSB1A2 from 2010 Kit Plate

  • 10µL of Milli-Q water and extraction of P0440 in pSB1A2 from the 2010 kit plate (10I) were mixed together.
  • The transformation was done following the Transformation Protocol 1.

May 20, 2011

Miniprep of P0440 in pSB1A2

  • Miniprep of P0440 in pSB1A2 was made following the Miniprep Protocol (Modified Bench Protocol: QIAprep Spin Miniprep Kit).


Assembly of Multiple Parts

  • Each of I13453, P0440, K331033, K331035, K331035, B0015, K249002, B0015, R0010 & B0034 were restricted where all odd parts were upstream and even parts were downstream.
  • I1343 & P0330 were ligated together in pSB1A3 following the Ligation Protocol 1.
  • K331033 & K331035 were ligated together in pSB1A3 following the Ligation Protocol 1.
  • K331035 & B0015 were ligated together in pSB1A3 following the Ligation Protocol 1.
  • K249002 & B0015 were ligated together in pSB1A3 following the Ligation Protocol 1.
  • R0010 & B0034 were ligated together in pSB1A3 following the Ligation Protocol 1.
  • All ligations and a negative control (water) were transformed following the Transformation Protocol 1.
  • Gel

May 26, 2011

Transformation of K325909 in pSB1C3 and K325229 in pSB1C3 from 2011 Kit Plate

  • 10µL of Milli-Q water and extraction of K325909 in pSB1C3 from the 2011 kit plate (17m) were mixed together.
  • 10µL of Milli-Q water and extraction of K325299 in pSB1C3 from the 2011 kit plate (17c) were mixed together.
  • The transformation was done following the Transformation Protocol 1.


June

June 8, 2011

Minipreps of Multiple Parts

  • Minipreps of K331022, K331008, K331024, xylE, K331024, K331007, K331022, K331008 & K331007 were done following the Miniprep Protocol (Modified Bench Protocol: QIAprep Spin Miniprep Kit Using Microcentrifuge).

June 9, 2011

Assembly of pBAD-rbs & lumazine-dt

  • Each of pBAD-rbs & lumazine-dt were restricted following the Restriction Protocol 1
  • pBAD-rbs & lumazine-dt were ligated together in pSB1C3 following the Ligation Protocol 1.
  • The ligation was transformed following the Transformation Protocol 1.

June 10, 2011

Transformation of pBAD-P0440

  • pBAD-P0440 in pSB1K3 was transformed following the Transformation Protocol 1.


Overnight Cultures of pBAD-rbs & lumazine-dt

  • Overnight cultures of pBAD-rbs & lumazine-dt grown following the Overnight Cultures Protocol.

June 11, 2011

Assembly of K331033 & K331035 and R0010 & B0034

  • Each of K331033, K331035, R0010 & B0034 were restricted following the Restriction Protocol 1 where all odd parts are upstream and even parts are downstream.
  • K331033 & K331035 were ligated together in pSB1K3 following the Ligation Protocol 1.
  • R0010 & B0034 were ligated together in pSB1K3 following the Ligation Protocol 1.
  • Both ligations were transformed following the Transformation Protocol 1.

June 12, 2011

Overnight Cultures of K331033-K331035 & R0010-B0034

  • Overnight cultures of K331033-K331035 & R0010-B0034 grown following the Overnight Cultures Protocol.

June 13, 2011

Assembly of Multiple Parts

  • Each of K331033, K331035, R0010, B0034, pBAD-rbs & lumazine-dt were restricted following the Restriction Protocol 1 where all odd parts are upstream and even parts are downstream and with the pSB1K3 destination plasmid.
  • K331033 & K331035 were ligated together in pSB1K3 following the Ligation Protocol 1.
  • R0010 & B0034 were ligated together in pSB1K3 following the Ligation Protocol 1.
  • pBAD-rbs & lumazine-dt were ligated together in pSB1K3 following the Ligation Protocol 1.
  • All ligations were transformed following the Transformation Protocol 1.

June 14, 2011

Minipreps of R0010-B0034 & pBAD-rbs-lumazine-dt

  • Minipreps of R0010-B0034 & pBAD-rbs-lumazine-dt were made following the Miniprep Protocol (Modified Bench Protocol: QIAprep Spin Miniprep Kit).


Overnight Cultures of K331033-K331035 & R0010-B0034

  • Overnight cultures of K331033-K331035 & R0010-B0034 grown following the Overnight Cultures Protocol.

June 15-16, 2011

Assembly of K331033 & K331035 and R0010 & B0034

  • Each of K331033, K331035, R0010 & B0034 were restricted following the Restriction Protocol 1 where all odd parts are upstream and even parts are downstream.
  • K331033 & K331035 were ligated together in pSB1K3 following the Ligation Protocol 1.
  • R0010 & B0034 were ligated together in pSB1K3 following the Ligation Protocol 1.
  • Both ligations were transformed following the Transformation Protocol 1.


Confirmation Gel of pBAD-rbs-lumazine-dt & R0010-B0034

  • Each of pBAD-rbs-lumazine-dt & R0010-B0034 were restricted following the Restriction Protocol 4.
  • A gel was made following the 1% Agarose Gel Protocol (100mL), but 1.5% with 1.50g of Agarose and 100mL of 1x TAE.
  • The restrictions were loaded onto the gel with a 1kb ladder and 100bp ladder.
  • The gel ran at 100V for 60 minutes.
  • The gel was then stained in Ethidium Bromide for 10 minutes.

June 22, 2011

PCR of pBAD-P0440 in pSB1K3

  • pBAD-P0440 was PCRed following the PCR Protocol.

June 23, 2011

Confirmation Gel of pBAD-P0440 (PCR)

  • pBAD-P0440 (PCR) was restricted following the Restriction Protocol 4.
  • A gel was made following the 1% Agarose Gel Protocol (100mL).
  • The restrictions were loaded onto the gel with a 1kb ladder.
  • The gel ran at 100V for 90 minutes.
  • The gel was then stained in Ethidium Bromide for 10 minutes.
  • TABLE? PICTURE?

Overnight Cultures of pBAD-rbs-lumazine-dt & K331033-K331035

  • Overnight cultures of pBAD-rbs-lumazine-dt & K331033-K331035 grown following the Overnight Cultures Protocol.

June 24, 2011

Minipreps of pBAD-rbs-lumazine-dt & K331033-K331035

  • Minipreps of pBAD-rbs-lumazine-dt & K331033-K331035 were made following the Miniprep Protocol (Modified Bench Protocol: QIAprep Spin Miniprep Kit Using Microcentrifuge).

June 29th, 2011

PCR of pBAD-P0440 in pSB1K3 and P0440 was done using PCR protocol Assembly of R0010 with B0034 in pSB1C3 Transformation for pBad-RBS and pBad- P0440 into Dh5a E. Coli

June 30th, 2011

Ran 1% Agarose Gel from June 29 PCR of pBAD-p0440 and p0440


July

July 2, 2011

Picked Colonies and grew overnight

  • 4 colonies picked from pBad rbs in pSB1T3
  • 3 colonies picked from pBad-p0440
  • picked 3 colonies from 2 plates of pBAD-P0440 in pSB1C3
    • 1 colony picked from plate A, and 2 colonies from plate B

July 03,2011

  • None of the 4 colonies of pBAD rbs grew, so they were re-grown in the incubator
  • Samples of pBAD-p0440 were mini prepped and stored in team 1 DNA box
  • Picked 3 samples of pBad- p0440 in psb1C3 and 3 samples of pBAD p0440 in pSB1K3

July 05,2011

PCR out inserts from July 03, of pBAD-P0440

  • PCR out inserts from July 03, of pBAD-P0440 samples using prefix and antisense suffix primers and run on agarose gel at 120V to determine if plasmid contains the correct insert, using po440 as a control.

July 06,2011

Repeated July 05, but only for pBad p0440 (2,4)

July 7th, 2011

Assembled I13453 with B0034 and into pSB1K3 with J04500

  • Assembly done using Restriction, ligation, and transformation techniques

July 11th, 2011

Assembly of pLacI-rbs and Lumazine synthase- dt Plasmid transfer of Ag43

  • Assembled pLacI-rbs and Lumazine synthase- dt into destination plasmid pSB1C3, followed restriction digest, ligation, and transformation procedures.
  • Plasmid Transfer of Ag43 from pSB1C3 to pSB1K3 using cut sites EcoRI and PstI
  • Ran a 1% Agarose Gel using 0.5 TAE buffer solution for parts BBa-J04500 in pSB1AK3, R0040, and Lumazine synthase-Dt to confirm sizes. Used Restriction procedure, cutting with EcoRI

July 13th, 2011

Assembly of K331033 and K331035

  • Did a restriction and Gel Extraction for K331033 cutting at EcoRI and SpeI, K331035 cutting at PstI and XbaI, and pSB1K3 cutting at EcoRI and PstI
  • Ran the gel for 80 minutes at 120Volts
  • Used Transformation protocol to Transformed XylE, XylF, XylT, XylK, XylQ, into Dh5a E. Coli cells

July 14, 2011

Ligation of K331033 to K3310335 into pSB1K3

  • Performed a ligation of K331033 to K3310335 into pSB1K3 and transformation of ligated parts into Dh5a E. Coli. Used Transformation and ligation protocols. Plated culture on Kanmycin plates

July 15th, 2011

Assembly of pLacI –Rbs in pSB1C3 and Lumazine Dt in pSB1AK3

  • Assembly of pLacI –Rbs in pSB1C3 and Lumazine Dt in pSB1AK3 using restriction digest and gel extraction protocols

July 19th,2011

Assembly of K346007 and J04500 into destination plasmid pSB1C3

  • Assembly of K346007 and J04500 into destination plasmid pSB1C3 parts were restricted, ligated and transformed using appropriate protocols.
  • Results: all of the plates had significant bacterial growth, will repeat experiment using LB instead of SOC during transformation

July 20th,2011

Tried to pre-aliquot restriction
  • Created a master-mix from appropriately sized aliquots that can be stored in the -20 freezer. Two mixes were created in the following volumes:
    • 16micro liters miliQ H2O
    • 2.5 micro liters Buffer II
    • 0.5 micro liters BSA 100X
    • 0.5 micro liters EcoRI
    • 0.5 micro liters SpeI
    • 20 micro liters total restriction mixture

July 25th, 2011

A Colony PCR was run for Parts K346007 and J04500 to confirm assemblies

  • This was done following the colony PCR protocol

July 26th,2011

Picking of colonies

  • Cells were picked with parts J04500- K346007 in them, for plasmid extraction by miniprep protocol. 23 colonies were picked in total and placed in 5 ml of lb in test tubes, along with 5micro liters of chloramphenicol was added to each test tube. Picked colonies were placed in the shaker overnight at 37 degrees Celsius

July 27th, 2011

Assembly of following parts:

  • K331033 to K331035
    • J04500 to Lumazine Synthase Dt
    • pBad to P0440
    • P0440 to K331033
    • Lumazine synthase dt to pBad
  • A restriction was done using the restriction protocol following a Gel extraction protocol. A ligation was performed and contents incubated at room temperature for 30 mins. Controls were run with downstream part being substituted as water.
  • Restricted J04500-k346007 with EcoRI, and PstI following restriction protocol, to confirm assembly success, restriction were loaded into a 08% Agarose gel. 23 samples from previous day was loaded into gel. Lanes 16 and 17 showed expected sizes

July 28th,2011

Ran a PCR gel for Justin to confirm PCR insert was correct


August

August 1st, 2011

Three colonies picked for parts J45120 and J45320

  • 3 colonies picked from plates for J45120 and J45320 and were placed in 5 ml test tubes with LB media and 5 micro liters Amp, and placed in shaker overnight

August 03rd, 2011

Restriction of:

    • pBad-P0440 in pSB1A2
    • Lumazine Synthase-dt with pBad in pSB1A2
    • K331033 – K331035 in pSB1C3
    • P0440 – K331033 in pSB1A2
  • Confirmation of assemblies by means of Agarose Gel
  • Ran Gel at 80 volts for 2 hours
  • Conclusion: parts were verified and appear to have been assembled successfully

August 4th, 2011

Restriction by protocol of assembling parts :

    • J04500-Lumazine synthase-dt out of pSB1AK3 + pbad-P0440 in psb1AK3
    • pBad-P0440 out of pSB1A2 + K331033-K331035 in pSB1C3
    • Lumazine synthase-dt-pBad pSB1A2 + p0440-K331033 in psb1A2
  • J04500 in pSB1Ak3 + Lumazine-synthase-dt-pBad out of pSB1A2
  • P0440-k331033 out of pSB1AK3 + k331035 in pSB1C3
  • Ran a TAE agarose Gel

August 11th, 2011

Assembly of parts:

  • pBad-P0440 + K331033-k331035 in pSB1C3
  • Lumazine synthase-Dt-pBad + PlacI in pSB1AK3
  • Lumazine synthase in pSB1C3 + Dt in pSB1A2
  • PlacI in pSB1AK3 + Lumazine synthase in pSB1C3
  • Ran a 1X TAE 1% Agarose Gel at 80Volts for 120 min for Extraction of parts by protocol

August 12th, 2011

Assembly of J04500 to Enhanced Lumazine synthase and Enhanced Lumazine synthase to Dt

  • Followed protocols for Restriction, Gel Extraction, Ligation and Transformation,
  • Cut J04500 in pSB1AK3 at SpeI and PstI, Cut Enhanced Lumazine synthase at XbaI and PstI
  • Cut Enhanced Lumazine synthase at EcoRI and SpeI, Cut Dt in pSB1AK3 EcoRI and XbaI.
  • Samples were run on a 0.9% Agarose gel in 1X TAE at 100Volts
  • Results: Colonies grew from the J04500-Enhanced Lumazine synthase and Enhanced Lumazine synthase – Dt in pSB1AK3

August 13th, 2011

Assembly of PLacI with Agn43 with Dt
Miniprep:

  • Dt in pSB1AK3
  • J04500 – Agn43 in pSB1AK3
  • K346007(Agn43) in pSB1C3
  • J04500-Lumazine synthase – Dt pSB1AK3

Ran a Gel of J04500-Ag43 in pSB1A2, and Agn43 in pAB1C3 Assembly of pBad-P0440 with K331033-K331035

  • Picked: pBad-P0440 cells, K331033- K331035 in pSB1C3 cells
    • left cells to grow overnight in shaker at 37 degrees Celsius
    • Picked 6 colonies from Enhanced Lumazine synthase plates from August 12

August 14th,2011

Mini-prepped:

  • pBad –p0440 in pSB1A2
  • K331033-K331035 in pSB1C3
  • Enhanced Lumazine synthase
    • 2 minipreps of plated colonies of pLAcI-Enhanced Lumazine synthase
    • 4 minipreps of plated colonies of Enhanced Lumazine synthase- Dt

Restricted:

  • 1) J04500 in pSB1AK3 cut at SpeI and PstI
  • 2) Enhanced Lumazine syhtase –Dt in pSB1AK3 cut at XbaI and PstI
  • 3) J04500 –Enhanced Lumazine synthase in pSB1AK3 cut at EcoRI and SpeI
  • 4) B0017 in pSB1AK3 cut at EcoRI and XbaI
  • 5) J04500-Lumazine synthase –dt cut at EcoRI and SpeI
  • 6) pBad- P0440 in pSB1A2 cut at EcoRI and XbaI
  • 7) pBad- P0440 in pSB1A2 cut at SpeI and PstI
  • 8) K331033-K331035 Cut at Xba1 and PstI
  • Ran a Gel extraction by protocol

The previously numbered restrictions were ligated as follows:

  • 1+2
  • 3+4
  • 5+6
  • 7+8
  • Ligations were incubated and transformed then plated on Ampicillin plates following protocols.
  • A 1X TBE 1% Agarose gel was successfully run at 100volts for 50 minutes to confirm parts

August 15th, 2011

Assembly of Antigen 43 with PLacI and Dt Followed Protocol for a restrictions of :

  • 1) J04500 in pSB1AK3
  • 2) Agn43
  • 3) Agn43
  • 4)Dt in pSB1AK3
  • 5) J04500-Agn43
  • 6) Dt in pSB1AK2

August 16th, 2011

Verify parts by running them on an Agarose Gel

August 17th,2011

Miniprep protocol was followed for enhanced lumazine synthase in pSB1C3, all 5 ml of culture was used Restriction of:

  • Enhanced Lumazine synthase dt, J04500 + enhanced lumazine and Enhanced lumazine.
  • Restricted parts were run on a gel to confirm parts. Gel ran at 80Volts for 90 minutes
  • Enhanced lumazine synthase was confirmed,
  • J04500-Enhanced lumazine synthase confirmed
  • Enhanced Lumazine synthase –Dt did not confirm

Assembly of J04500-enhanced Lumazine synthase +DT Did a restriction following protocol of:

  • 1) J04500 – Enhanced Lumazine synthase out of pSB1AK3 Cut at EcoRI and SpeI
  • 2) B0017 in pSB1AK3 Cut at EcoRI and XbaI

Ran restricted parts on an Agarose Gel: No DNA was able to be observed outside ladder

August 18th,2011

Assembled the complete Lumazine synthase and florescent proteins construct

  • Repeat August 17th: Restriction, Gel extraction, Ligation and Transformation
  • Did a Restriction following protocol of:
    • 1) J04500-Enhanced lumazine synthase in pSB1AK3 cut at EcoRI and SpeI
    • 2) B0017 in pSB1AK3 cut at EcoRI and XbaI
    • 3) J04500-Lumazine synthase – Dt Cut at EcoRI and SpeI
    • 4) Dt in pSB1C3 cut at EcoRI and XbaI
  • Restrictions were run on an Agarose Gel, only parts 1), and 2) were observed on the Gel

Restrictions and Gel were run again for missing parts; restriction time was decreased; no parts were shown on Gel

August 20th, 2011

Assembly of Construct:

  • J04500- Lumazine synthase-dt-pBad-P0440- K331033-K331035
  • The following protocols were used to assemble this construction: Restriction, Gel Extraction, Ligation and Transformation

Restriction of:

  • 1) J04500-Lumazine synthase-dt cut out of pSB1AK3 at EcoRI and SpeI
  • 2) pBad- P0440-K331033-K331035 in pSB1C3 cut at EcoRI and XbaI
  • Restrictions were run on a 1% Agarose 1X TAE Gel for purpose of extraction
  • DNA did not show on Gel

August 21st,2011

Assembly of construct:

  • J04500-Lumazine synthase dt-pBad-P0440-K331033-K331035
  • Repeated previous day’s work. The parts had been confirmed by sequencing
  • Picked Colonies from plate for parts J04500-Enhanced lumazine synthase in pSB1AK3 and grew overnight in LB for purpose of Glycerol stocks
  • Gel of parts worked and a successful Gel extraction was performed. Extracted parts 1) and 2) from August 20th that were ligated together
  • Ligated parts were transformed into Dh5alpha and plated on appropriate antibiotic selected plates

August 22, 2011

Picked J04500-Enhanced Lumazine synthase colonies from plated construct Assembly of Constructs:

    • 1) XylE cut at EcoRI and SpeI
**2) S04261 Cut at EcoRI and XbaI 
**3)K331007 cut at EcoRi and XbaI in pSB1C3 
    • 4) mms6 cut at EcoRI and SpeI
    • 5) K3301007 in pSB1C3 cut at SpeI and PstI
    • 6) mms6 Cut at XbaI and PstI
    • 7) K331008 in pSB1C3 cut at SpeI an dPstI
    • 8) mms6 cut at XbaI and PstI
    • 9) K331009 in pSB1C3 cut at SpeI and PstI
    • 10) mms6 cut at XbaI and PstI
    • 11) K331012 in pSB1C3 cut at SpeI and PstI
    • 12) mms6 cut at XbaI and PstI
    • 13) S04261 pSB1AK3 cut at EcoRI and XbaI
    • 14) mms6 cut with EcoRI and SpeI
  • Parts were run on an Agarose Gel for Gel extraction
  • Gel was successful and a Gel Extraction was performed.

Following parts were ligated together as per protocol

  • 1 + 2
  • 3 + 4
  • 5 + 6
  • 7 + 6
  • 9 + 6
  • 11 + 6
  • 14 + 4

Ligations were transformed via protocol into Dh5 alpha, plated, and left in incubator overnight

  • Performed a Concentration of Enhanced lumazine synthase from Sephacryl 400 Chromatography
  • Pooled fractions at 35, 36 ,37
  • Vivaspin 20, 3000 mwco reviled with 17.5 ml dd milliQ H20, spun at 4000Xg for 25 minutes
  • The column was then washed with 10 ml of sodium phosphate buffer, at 4000Xg for 40 minutes
  • 7.5ml of Fractions 35,36,37,were loaded onto column and concentrated to 1ml by Centrifuge at 4000XG at 4Degrees Celsius for about an hour in 5 minute increments
  • Concentrations to be determined photometrically and concentration must be determined and protein visualized Via SDS page gel

August 28th, 2011

Over expression of complete construct

  • Overnight culture grown by Justin, 12ml of overnight culture, of E. Coli Dh5alpha J04500-K249002- B0017- I13453-P0040-K331033-K331035, in the pSB1C3 Vector, was inoculated in 4 x 500ml LB flasks, with 500micro liter of Chloramphenicol and grown up to OD600 of 0.0978

August 29th, 2011

  • Ran SDS page of August 28th, overexpression, SDS sample preparation protocol was followed
  • The SDS page was run at 80Volts for 15 mins and 180Volts for 45mins
  • Stained in Coomassie blue for 30 mins and distained over night

August 31, 2011

Assembly of:

  • J04500-Enhanced Lumazine synthase cut out of pSB1AK3 at EcoRI and SpeI ligated to B0015 cut at EcoRI and XbaI in pSB1AK3
  • Ptet-rbs in pSB1A2 cut at SpeI and PStI Ligated to XylE - arginine tag cut at XbaI and PstI.

Followed Restriction, Gel Extraction protocols

    • Note: J04500 –Enhanced Lumazine synthase and Xyle – agrinine tag –dt did not Cut out of plasmid. B0015 in pSB1AK3, and Ptet-rbs in pSB1A2 were found around the right sizes


September

September 3rd, 2011

Repeated August 31 assembly

Sept 14th,2011

Show how effective BamHI is in degrading E.coli DH5α Genomic DNA

  • 2 overnight cultures were picked in 50 ml flasks with 50micro liters of Ampicillin and were inoculated with BamHI and pLacI from Glycerol stock
  • 16ml of pLacI from overnight culture were used to inoculate 250ml of Lb with 250micro liters of Ampicillin to bring it to an OD600 of 0.118
  • 11.2 ml of BamHI overnight culture was used to inoculate 250ml of LB to an OD600 of 0.100

September 17th, 2011

Repeat, the August 14th BamHI experiment due to the spectrophotometer being inaccurate

September 19th, 2011

Isolation of genomic DNA from BamHI cells by following the Qiagen Blood and Tissue Kit protocol for isolating genomic DNA of gram-negative bacteria

September 21, 2011

Overnight culture of full construct (lumazine synthase – K331033 – K331035, K331033 and K331035) for FRET experiments

  • Selected cells were induced with arabinose.
  • All cells showed growth after 15 hours in shaker at 37 degrees Celsius.

September 22, 2011

Continued work from September 21

  • Spun down cells and re-suspended in LB media and checked Optical Density of 1 ml of culture and brought them to 1 OD
  • Signs of FRET but nothing confirmed
    • Note: This is something we will be working on continuously up until Boston