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Revision as of 15:45, 16 October 2016


Experiments

Overview of Experiments

1. Production Strains

In order to ensure that the bacteria we are working with are really the ones we want to work with, a 16S rDNA PCR was performed.

As an antibiotic resistance will be used in our later experiments to select transformants, we checked for any native antibiotic resistance against ampicillin, kanamycin, tetracyclin and chloramphenicol in an LB agar plate growth test. It turned out that kanamycin was the only antibiotic, against which none of our strains showed any resistance. For this reason, we decided to use only vectors with kanamycin resistance for our later projects.

After this, we prepared electro competent cells from our strains. All of our strains were grown on LB medium.

2. BioBricks

Our BioBricks were designed using the software SnapGene. The original Genes for our B12 binding proteins, and the torA signal sequence were codon optimized for E. coli.

The DNA containing the Genes were synthesized and friendly provided by IDT Integrated DNA Technologies.

In case of MutB, the length of the gene exceeded the maximum length of 2000 bp from IDT. For this reason, we designed two DNA parts, with a natural occurring HindIII restriction site at both ends. We intended to fuse these both genes by ligation. However, after having diffuculties to fuse the genes by ligation, we decided to fuse them by fusion PCR. In order to multiply the DNA for or cloning experiments, and to equip our genes with restriction sites, PCR was used.

For our purpose, we were searching for a vector with (a) kanamycin resistance and (b) araBAD operon. We thus decided to use the pBAD202 expression system. This vector, however, is equipped with a thioredoxin fusion protein which increases the rate of expression, but prohibits the physiological function of our protein. For this reason, we designed primers for an autarkic synporter protein. In order to test the dependence of the expression system on the B12 export rate, we also decided to use different other vectors.

For vectors ligation, we used a standart ligase reaction, for the pBAD202 expression, which works without ligation but topoisomerase reaction, we followed the manufacturer's protocol.

3. Transformation and Cultivation

For our transformation experiments, we used electroporation for all our self prepared competent cells. For the heat competent E. coli Top10 cells provided with the pBAD202 expression system, we used the manufacturer's heat shock transformation protocol.

For vector multiplication, E. coli cells (Top10 for pBAD202 plasmids, DH5alpha for all other plasmids) were transformed with the constructed plasmids. After the transformation, the cells were cultivated on LB Medium. Transformants were selected, and the respective clones were picked, cultivated in LB medium, and plasmids were extracted.

The Plasmids were then introduced into the production strains: Raoultella planticola ATCC 33531, Shimwellia blattae ATCC 29907, and Salmonella typhimurium TA100.

For the expression experiments, the all cells were cultivated and the expression induced in RM medium under aerobic conditions. As S. blattae is known to produce Vitamin B12 only under anaerobic conditions, the expression was induced under anerobic conditions in RM medium.

The induction was performed using different concentrations of l-arabinose and different induction time spans.

4. Expression Test

To test for the expression of our synporter protein, the cell lysates of the expression cultures we submitted to an SDS-PAGE. From the SDS Gels, Western Blots were performed using anti-Poly-Histidine-tag antibodies.

5. Vitamin B12 Assay

To test the physiological function of our synporter protein, different assays for B12 detection were performed. For the assays, (a) the whole cell filtered medium, and (b) the periplasm fraction of the cells were examined.

The periplasm fraction of the producing cells was gained by ultrazentrifugation.

5.1. Microbial Assay

The microbial B12 assay relies on the growth diameter of the E. coli ATCC 10799 strain on an agar plate, in dependence of the Vitamin B12 (or methionine) concentration in the medium.

For this purpose, agar plates with synthetic Guttman medium (free of B12 and amino acids, 1.5% agarose) were prepared. The E coli detection cells were grown in liquid synthetic Guttman medium supplemented with selected amino acids (no methionine) and Vitmamin B12. Afterwards, the cells were washed with PBS buffer three times, in order to make the cells virtually free of Vitamin B12. The cells were resuspended in PBS buffer, and mixed with warm, liquid Guttman medium (free of B12 and amino acids, 0.8% agarose), and then poured on the prepared agar plates. For the assay, small paper platelets (usually used for antibiotic tests) were placed on the top agar layer, and soaked with differently concentrated calibration solutions of Vitamin B12. The plates were incubated overnight, and the diameters measured after 16 h. From the different diameters, dependent of the Vitamin B12 concentration, a calibration curve was calculated.

In order to determine the B12 content of our medium and periplasm fraction, the assay plates were prepared exactly as described above, and paper platelets were soaked with the respective solution. Comparing to the calibration curve, the diameter indicates the B12 amount.

5.1. Photometric Assay

Protocols

Media

LB Medium

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M9 Minimal Medium

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RM Medium

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Guttman Medium (B12 Assay)

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S. blattae Medium Anaerobic

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Cultivation and Transformation

Cultivation of Escherichia coli, Shimwellia blattae and Salmonella typhimurium TA 100

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Cultivation of Raoultella planticola

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Preparation of Electrocompetent Cells

Material to prepare

  • 2x 5 mL LB
  • 250 mL LB in 1 L Erlenmeyer flask with chicane
  • 500 mL sterile Millipore-H2O at 4 °C
  • 50 mL sterile glycerol (10 % (w/v)) at 4 °C
  • 30 sterile labeled Eppendorf cups at – 20°C or -80 °C
  • 1x sterile GS3 jar at 4 °C
  • 1x Aquatron at 30 °C
  • 1x Sorvall RC6 centrifuge at 4 °C
  • 1x Universal 320R centrifuge at 4 °C
  • 1 L liquid nitrogen

 

Day 1

  • Inoculate 2x 5 mL LB (if required with antibiotics) with your strain of interest, either from cryo culture or from agar plate.
  • Incubate overnight at 37 °C and 150 rpm.

 

Day 2

  • Inoculate 250 mL LB (without antibiotics) with 2 % (5 mL) preculture.
  • Incubate in the Aquatron at 30 °C and 160 rpm until OD600 of 0.5-0.8.
  • Check the culture via microscope for contaminations.

All liquids and containers must be cooled on ice. The major task of cell preparation is the removal of salts. In case of some strains like pLys-strains, the pellets must be resuspended very carefully.

  • Let the cells (OD600 of 0.5-0.8) cool down in ice water for 10-20 min. All further steps are performed under cool conditions.
  • Decant the cells in sterile GS3 jar and centrifuge at 4 °C and 5000 rpm (4230 g) for 5-10 min.
  • Remove supernatant (directly next to the centrifuge or the pellet might resolve) and resuspend the pellet in 250 mL sterile 4 °C ddH2O.
  • Centrifuge the GS3 jar at 4 °C and 5000 rpm (4230 g)for 5-10 min.
  • Remove supernatant (directly next to the centrifuge or the pellet might resolve) and resuspend the pellet in 250 mL sterile 4 °C ddH2O.
  • Centrifuge the GS3 jar at 4 °C and 5000 rpm (4230 g)for 5-10 min.
  • Remove supernatant (directly next to the centrifuge or the pellet might resolve) and resuspend the pellet in 10 mL sterile 4 °C glycerol (10 % (w/v)). Afterwards, transfer the culture into a 50 mL Falcon tube.
  • Centrifuge the Falcon tube at 4 °C and 6200 rpm (4230 g) for 5-10 min.
  • Remove supernatant (directly next to the centrifuge or the pellet might resolve) and resuspend the pellet in 10 mL sterile 4 °C glycerol (10 % (w/v)).
  • Centrifuge the Falcon tube at 4 °C and 6200 rpm (4230 g) for 5-10 min.
  • Remove supernatant (directly next to the centrifuge or the pellet might resolve) and resuspend the pellet in 500 µL sterile 4 °C glycerol (10 % (w/v)).
  • Aliquot the cells into the Eppendorf cups (40 µL per Eppendorf cup). While aliquoting, filled Eppendorf cups must be frozen directly in liquid nitrogen.
  • Store the filled Eppendorf cups in a cryobox at -80 °C.
Transformation Electroporation of Electrocompetent Cells
  • Mix 50-200 ng plasmid DNA with 40 µL of competent cells (always defrost on ice!). Transfer attempt into precooled electroporation cuvette. Incubate on ice for 10 min.
  • Important: DNA must be salt free! Use either directly in ddH2O eluted plasmids, or (e.g. directly after ligation) desalt the DNA for 30 min on a Millipore filter (MF Membrane Filters).
  • Electroporation: 2500 V for 2 mm cuvettes (1250 V for 1 mm cuvettes), 25 µF, 200 Ω, discharging time should be 3-5 msec. Contacts of the electroporation cuvette must be dry. Remove all air bubbles before electroporation.
  • Immediately add 960 µL liquid LB (or, if available, SOC medium for a higher transformation efficiency) into the cuvette and transfer the content into a 2 ml Eppendorf cup.
  • Incubate at 37 °C and 150 rpm for 1 h. Fix tube in horizontal position with tape.
  • Plate 100 µL of 10-3 to 10-6 dilutions on plates with selection pressure
  • Incubate at 37 °C overnight.
Heat Shock Transformation of Heat Competent Cells

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PCR and Cloning

Entry 1

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ENtry 2

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Entry 3

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Entry 4

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Analytic Tests

Agarose Gel Electrophoresis

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SDS Polyacrylamid Gel Electrophoresis

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Western Blot

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Microbial B12 Plate Assay

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Contact


iGEM Team Göttingen 2016
Institut für Mikrobiologie
und Genetik
AG Prof. Dr. Rolf Daniel
Grisebachstr. 8
37077 Göttingen

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