Difference between revisions of "Team:Calgary/BetaOxidation"

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Revision as of 07:02, 31 October 2017

Header

Beta Oxidation

Beta-Oxidation Pathway


Aim

The objective of our project was to genetically engineer E. coli to produce PHB from volatile fatty acids (VFAs) found in human fecal waste. VFAs (acetic acid, propionic acid, butyric acid, and lactic acid) serve as a precursors for the synthesis of PHB (Reyhanitash, 2017).

In order to synthesize PHB from fatty acids found in human fecal waste, we manipulated the fatty acid beta-oxidation pathway within E. coli. By designing a construct that contains the gene phaJ, encoding for an enoyl-CoA hydratase that converts the enoyl-CoA from the beta-oxidation cycle into (R)-hydroxybutyrate (Lu, 2003). Our construct also includes the gene phaC, encoding for the PHA synthase, which converts the (R)-hydroxyacyl-CoA into polyhydroxybutyrate(PHB). To our advantage, this pathway not only uses VFAs, but can also use undigested long-chain fatty acids in human fecal waste, thus maximizing the substrates available for PHB synthesis.


Volatile fatty acids & beta-oxidation pathway


Genetic construct

Beta-Oxidation Construct

Figure 1: Genetic construct for phaCJ, including the ribosomal binding sites (BBa_B0034) and the phaJ and phaC genes


Results

The O/Ns were grown in the respective media for ~24 hours. The flasks containing different media was inoculated with the O/Ns after adjusting the OD600. The composition of each of the replicate in the flasks is shown below:

Glucose (Positive control) pET29B in BL21 (Negative control)
  • 10 ml O/Ns in LB+Kan
  • 7 ml 20% Glucose
  • 100 uL MgSO4
  • 5 uL CaCl2
  • 10 ml M9 salts
  • 5 uL 1M IPTG
  • 20 ml dH2O
  • 10 ml O/Ns in LB+Kan
  • "Syn poo" fermented supernatant
  • 100 uL MgSO4
  • 5 uL CaCl2
  • 10 ml M9 salts
  • 5 uL 1M IPTG
Fermented "syn poo" supernatant Pure VFAs
  • 10 ml O/Ns in LB+Kan
  • 10 ml "Syn poo" fermented supernatant
  • 100 uL MgSO4
  • 5 uL CaCl2
  • 10 ml M9 salts
  • 5 uL 1M IPTG
  • 23 ml dH2O
  • 10 ml O/Ns in LB+Kan
  • VFAs
    • 410 uL propionic acid
    • 118 uL acetic acid
    • 55 uL butyric acid
  • 100 uL MgSO4
  • 5 uL CaCl2
  • 10 ml M9 salts
  • 5 uL 1M IPTG
  • 30 ml dH2O

The OD600 readings of .....???? were taken and recorded:

Condition OD600 of replicate 1 OD600 of replicate 2 OD600 of replicate 3
pET29b in BL21 (Negative control) 0.571 0.531 0.487
Glucose (Positive control) 0.190 0.195 0.139
Pure VFAs 0.140 0.134 0.146
Fermented "syn poo" supernatant 0.135 0.107 0.144

After spinning down the culture in flasks, the cells were resuspended in 1x PBS. The OD600 readings were taken:

Condition OD600 of replicate 1 OD600 of replicate 2 OD600 of replicate 3
pET29b in BL21 (Negative control) 2.659 2.001 2.899
Glucose (Positive control) 1.934 1.887 1.919
Pure VFAs 0.510 0.571 0.532
Fermented "syn poo" supernatant 2.533 2.559 2.349



Works Cited

Rose, C., Parker, A., Jefferson, B. & Cartmell, E. (2015). The characterization of feces and urine: a review of the literature to informed advanced treatment technology. Critical Reviews in Environmental Science Technology. 45: 1827-1879.