Team:Michigan/Oil Sands October

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Week 14 - - - - - 10/1/2010 -
Week 15 10/3/2010 10/4/2010 10/5/2010 - 10/7/2010 10/8/2010 - Week 16 - - - - - - 10/16/2010


10/1/2010

Alex

Moved broth cultures 37°C to 4°C -- 1:30pm (19-hr culture) Prepared biofilm assay plate for all pH9 tests - following Alex's biofilm assay protocol

  • plate template:

9-30 plate template.jpg

    • 100 μL/well: 99 μL medium + 1 μL culture
  • stored plate in Lin Lab 4°C -- 2:20pm

Saved data for curves from ph7 plate Read pH7 plate ODs Performed biofilm assay on ph7 plate Started 24-hr kinetic reading for pH9 plate -- ~midnight

Discarded pH7 plate

Processed pH7 plate data

  • uploaded results here

Uploaded pH7 kinetic data here

10/3/10

Alex

Ran CV biofilm assay on pH9 plate, following my protocol

10/4/2010

Marcus and Ben

Performed ligation of Flu operon and pSB1AT3 according to the Ginko Bioworks Ligation protocol, with modifications.

  • Calculated amount from digests to add to ligation for 1:1 and 3:1 insert:vector ratios
    • Amount of DNA in digests:
      • Flu PCR- 29.8 ng/uL x 17 uL= 506.6 ng / 50 uL = 10.132 ng/uL
      • pSB1AT3- 240.5 ng/uL x 5 uL= 1202.5 ng / 50 uL = 24.05 ng/uL
    • Used an online calculator to find moles:
      • Flu PCR- 230.81 fmol/50 uL
      • pSB1AT3- 537.68 fmol/50 uL
      • This gives a molar ratio of 0.4293

1:1 Ligation Mix

  • 4 uL Flu PCR x 10.132 ng/uL= 40.528 ng
  • 1.7 uL pSB1AT3 x 24.05 ng/uL= 40.885 ng
  • 2 uL T4 Buffer
  • 1 uL T4 Ligase
  • 11.3 uL Ultra pure H2O

3:1 Ligation Mix

  • 2 uL Flu PCR x 10.132 ng/uL= 20.264 ng
  • 2.57 uL pSB1AT3 x 24.05 ng/uL= 61.809 ng
  • 2 uL T4 Buffer
  • 1 uL T4 Ligase
  • 12.43 uL Ultra pure H2O

Note that the conversion factor for the 3:1 ligation mixture was applied in reverse, and thus it was actually a 1:3 insert:vector ratio.

Ligation program was the same as used in the Ligation protocol.

10/5/2010

Marcus

Performed transformation according to Pope & Kent (1996).

Transformed Parts

  • Flu/pSB1AT3 1:1 ligation
  • Flu/pSB1AT3 1:3 ligation
  • VP130
  • J61100
  • OmpA
  • Cell only negative control

Procedure

  • 2 uL of DNA was pipetted into PCR tube on ice and transferred to Lin lab
  • Comp cells were thawed on ice and 50 uL was pipetted into each tube with a chilled pipette on ice
    • Cells were pipetted up and down to mix throughly
  • Cells were kept on ice and brought back to ERB
  • Cells were plated directly onto pre-warmed plates with appropriate antibiotics
    • Kevin put plates in incubator several hours before hand

It should be noted that two 200 uL aliquots of cells had to be thawed, and one was labeled "Thawed" and returned to the -80 C. Thawing should be avoided if possible.

Also, made two 5 mL LD1/LD2 co-cultures in M9+Sigma and Acros NAs, pH 7 and pH 9. Also made 2 mL pure cultures at pH 7. All culture tubes were stored in the 30 C. These cultures were made to assay growth, make new stock plates, and determine if colony morphology can be used to distinguish between species in a co-culture.

10/7/2010

Marcus

Ben moved transformation plates to 4 C yesterday, control plates were blank, and all plates except for J61100 appeared to have colonies. The Flu/pSB1AT3 ligation plates had very small colonies, so they were returned to the incubator with the J61100 plate. Also, it could be seen that many colonies on the 1:3 ligation plate appeared red, indicating that the vector had preferentially reformed. This could be because of the ratio, but dephosphorylation treatment should be used in the future for ligations.

OD600's were taken of the Pseudomonas cultures (46 hours)

  • Putida pH 7- 0.157
  • Fluorescens pH 7- 0.129
  • Co-culture pH 7- 0.188
  • Co-culture pH 9- 0.232

Surprisingly, they seem to grow better at pH 9, at least in co-culture. As expected, the co-culture did better than pure cultures. This lends some support towards Alex's biofilm assay results, however, it should still be repeated. Also, plated a serial dilution of the pH 9 co-culture, at 10-5, 10-6, and 10-7 dilutions to determine the conversion factor between OD600 and cell count. Made streak plates of all other cultures, pure cultures for stock, and pH 7 co-culture to determine if colonies could be distinguished. All cultures and plates were returned to the 30oC incubator, without shaking.

10/8/2010

Marcus

Kevin removed the transformation plates which were placed back in the incubator to the 4oC around 1 pm.

The Pope & Kent (1996) appears to be very efficient, as the plates were full of colonies:

5 Transformation Plates.jpg

Next time suspending the cells in water before spreading, or even making dilutions should be tried.

PCR Screening: 8 colonies were picked from each transformation plate except for VP130, and suspended in 50 uL of water on a microplate.

  • Plate Layout
    • Row 1- Flu 1:1
    • Row 2- Flu 1:3
    • Row 3- OmpA
    • Row 4- J61100

The first two rows (Flu 1:1 and 1:3) were PCR'd by adding 1 uL of each sample to a PCR tube with a drop of mineral oil in them. A master mix was made, and 50 uL was added to each tube (should have been 49 uL).

Master Mix (18x)

  • 180 uL 5x Phusion Buffer
  • 18 uL 10 mM dNTPs
  • 45 uL VF2
  • 45 uL VR
  • 9 uL Phusion polymerase
  • 585 uL Ultra pure H2O

PCR Program

  • 1. 95 C for 10 min
  • 2. 95 C for 30 sec
  • 3. 62 C for 30 sec
  • 4. 72 C for 2 min
  • 5. Return to step two 34 times
  • 6. 72 C for 10 min
  • 7. 4 C store

This PCR protocol was constructed from the following sources:

Also- loosened the lids on Pseudomonas liquid cultures to provide air exchange, and returned yesterday's Pseduomonas plates to 30C incubator, without shaking.

10/16/2010

Nick

10-16-10 Psuedomonas Competent Cell Preparation

Protocol - Competent Cell Preparation for Quick Transformation of E. coli

Ben Parker started the overnight cultures and assisted in OD measurement and initial centrifugation steps.

A colony of P. putida and P. fluorescence was picked from LB agar plates (10/6/10) and grown up in an overnight culture in 2ml Amp at 30 C.

The overnight culture was added to 100 ml of LB media and grown at 30C for 4 hours.

Protocol was carried out approximately 20 minutes after the following OD600 was recorded:

Blank - water

P. putida – 0.587

P. Fluorescence – 0.610

One centrifuge tube containing p. putida culture failed during centrifugation at 5000 rpm. The protocol was altered by reducing the speed to 2500 rpm after this point to reduce the chance of failure. The cells are stored in the 4C fridge in room 1239.