P(3HB) is the most common polyhydroxyalkanoate, which is a group of fully biodegradable polymers with properties similar to those of petroleum-based plastics. It can be produced in a variety of microorganisms, and its synthesis as a compound for energy storage in vivo has been extensively studied [1]. P(3HB) accumulates inside cells, and has been reported to occupy up to 90% (w/w) of the dry cell mass in certain species [2]. However, P(3HB) has yet to become integrated into the plastics market on Earth due to high costs of both fermentation and purification [3]. This summer, we focused on making the production, extraction, and use of P(3HB) more feasible on a lunar or Martian base.

(1) Increasing P(3HB) Yield

Increasing the yield of P(3HB) from a cell culture would decrease the time needed to complete the plastic production and extraction process by making smaller cultures more efficient. We have used the phaCAB operon from Ralstonia eutropha H16 that encodes the three genes required for P(3HB) production: PhaA, PhaB, and PhaC. Previous iGEM teams (Tokyo Tech 2012 and Imperial 2013) were able to successfully produce P(3HB) in vivo using BioBricks that encode these three genes. The pathway for P(3HB) production is as follows. First, 3-ketothiolase, encoded by PhaA, combines two molecules of acetyl-CoA to form acetoacetyl-CoA. This is then reduced by acetoacetyl-CoA reductase, encoded by PhaB, to form (R)-3-hydroxybutyl-CoA. This is then polymerized by PHA synthase, encoded by PhaC, forming poly-3-hydroxybuterate.

To increase the yield of P(3HB), we looked for a way to increase the amount of acetyl-coA, the precursor molecule to P(3HB) formation. Acetyl-CoA is composed of an acetyl group bound to coenzyme A. Coenzyme A consists of a beta-mercaptoethylamine group linked to pantothenic acid. On the Tokyo Tech 2012 iGEM team’s wiki, their results showed that adding pantothenic acid into their culture media led to increased yields of P(3HB). Therefore, we decided to increase the production of coenzyme A, which would then allow the cells to synthesize greater amounts of P(3HB).

Coenzyme A biosynthesis is a five-step process that is primarily regulated by the first enzyme in the pathway, pantothenate kinase (encoded by the gene PanK, which is also called CoaA) [4]. Pantothenate kinase stringently controls amount of coenzyme A produced in E. coli because the pantothenate kinase produced by E. coli is significantly inhibited by coenzyme A and its thioesters (such as acetyl-coA). Therefore, since we wanted to increase coenzyme A synthesis, we had to find a way to get around this negative feedback inhibition. Fortunately, the pantothenate kinase made in Staphylococcus aureus does not experience feedback inhibition from coenzyme A or its thioesters [5]. Indeed, this allows S. aureus to accumulate high levels of coenzyme A. We ordered the S. aureus pantothenate kinase sequence from IDT and inserted into the backbone PSB1C3 in front of the phaCAB operon designed by the Tokyo Tech iGEM team in 2012 with the hybrid promoter designed by the Imperial College iGEM team in 2013. The results section below shows that inserting the gene for pantothenate kinase allows for higher levels of P(3HB) production in E. coli.

(2) Facilitating P(3HB) Extraction

Since bacteria that naturally synthesize P(3HB) use the plastic as an energy storage mechanism, the plastic is produced inside the cell and stays there. Currently, the isolation of P(3HB) from the cells and culture media is one of the main bottlenecks in the P(3HB) production process – and the main source of its high cost of approximately $4-6 USD [6]. Traditional isolation methods include the use of large amounts of chemicals that can be hazardous to human health and the environment, such as chloroform and sodium hypochlorite, or other problems such as large volumes of waste water produced or impurities in the polymers [6]. Since one of our team’s goals has been to reduce up-mass of materials on space flights, we wanted to minimize the amounts of harmful (and heavy) chemicals that would need to be brought up as payload to extract the P(3HB).

We accomplished this by introducing a lysis device into the PSB1C3 plasmid that contained the phaCAB operon and the gene for pantothenate kinase. The lysis device was developed by the 2008 Berkeley iGEM team. The device contains T7 phage antiholin under a weak promoter, and T7 phage holin and endolysin inducible under (L)-arabinose. This lysis device was not reported to kill entire populations of E. coli, and we saw this as an advantage for a continuous plastic-production system. We would be able to cause part of the population to lyse and release its P(3HB) into the media. The rest of the population would continue growing and producing plastic. The plastic can be recovered from the media by causing the granules to aggregate, and then requiring lower amounts of solvents and less time to complete the purification process [7]. The results section below demonstrates the success of the lysis system and compares the efficiency of the recovery methods with and without the release of the P(3HB) into the media.

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Protocols

Device construction. Parts for this project were obtained from the 2015 Distribution Plates, ordered from the Registry, or synthesized by IDT. BioBricks assembly was used to construct the devices.

Transforming bacteria. Chemically competent DH5-alpha E. coli cells from New England Biolabs were used for all parts of this project. Plates containing successful transformants were stored at 4C.

Growing Plastic. Transformed cells were inoculated into Terrific Broth (TB) medium supplemented with chloramphenicol and shaken at 37C for 72 hours.

Extracting Plastic Powder. Liquid cultures of P(3HB) were pelleted by centrifugation at five-minute cycles at 4,000xg at 4C. The tubes with pellets were then placed at -80C for at least one hour, and then rushed down to the lyophilizer, where they were allowed to freeze dry for at least 24 hours. The freeze-dried pellets were then ground up and re-suspended in a 6-10% (v/v) sodium hypochlorite solution. This reaction is exothermic and significant pressure can build up; we had an unfortunate incident wherein the Eppendorf tubes all popped open in the incubator after only a few minutes. To avoid this, we then started to use 15mL Falcon tubes since the tops could be better secured. The first 20 minutes of reaction were carried out at room temperature with the lids only attached lightly to allow air to escape. Then, the lids were tightened and the tubes were shaken at 37C for an hour, with the air pressure being released every five to ten minutes. The samples were then centrifuged at 4,000xg at 4C for five minutes, the supernatant was discarded, and then the samples were re-suspended in 70% (v/v) ethanol. The samples were centrifuged at the same settings again, the supernatant was discarded, and they were re-suspended once more in distilled water. The samples were centrifuged one last time, the supernatant was poured off, and then the remaining water was allowed to evaporate overnight at 40-60C. The final mass of the plastic was then measured. This protocol was adapted from Hahn et al [8]. .

Extracting Plastic Sheets.

Liquid cultures of P(3HB) were pelleted by centrifugation at five-minute cycles at 4,000xg at 4C. The tubes with pellets were then placed at -80C for at least one hour, and then rushed down to the lyophilizer, where they were allowed to freeze dry for at least 24 hours. The freeze-dried pellets were then ground up and added to a sealable glass container of chloroform. We used half as much chloroform as media in the original culture (100mL chloroform if we had cells growing in 200 mL TB media). The contents of the container were stirred for 24 hours and then filtered into a flask using a mixed cellulose acetate filter. At this point, the P(3HB) and lipids from cells are dissolved in chloroform is in the flask. This solution was allowed to evaporate slightly, and then was dropped into a container of methanol. At this point, the plastic precipitates out, and the methanol dissolves the remaining lipids and non-polar cell particles. This solution is then filtered using a glass fiber filter to let the methanol and lipids through, and keep the P(3HB) in the filter. The filter was then changed to a different flask, and chloroform was added to the filter to bring the plastic through. The contents of the flask were poured into a glass petri dish and the chloroform was allowed to evaporate, leaving a plastic sheet at the bottom of the petri dish.

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References

[1] Anderson, A. J. and Dawes, E. A. Occurrence, Metabolism, Metabolic Role, and Industrial Uses of Bacterial Polyhydroxyalkanoates. Microbiological Reviews 54 (4), 1990. 450 – 472.

[2] Madison, L. L. and Huisman, G. W. Metabolic Engineering of Poly(3-Hydroxyalkanoates): From DNA to Plastic. Microbiol Mol Biol Rev 63 (1), 1999. 21 – 53.

[3] Kunasundari, B. and Sudesh, K. Isolation and recovery of microbial polyhydroxyalkanoates. eXPRESS Polymer Letters 5 (7), 2011. 620 – 634.

[4] Leonardi, R. et al. Coenzyme A: Back in action. Progress in Lipid Research 44, 2005. 125 – 153.

[5] Leonardi, R. et al. A Pantothenate Kinase from Staphylococcus aureus Refractory to Feedback Regulation by Coenzyme A. The Journal of Biological Chemistry 280, 2005. 3312 – 3322.

[6] Jacquel, N. et al. Isolation and purification of bacterial poly(3-hydroxyalkanoates). Biochemical Engineering Journal 39 (1), 2008. 15 – 27.

[7] Rahman, A. et al. Secretion of polyhydroxybuterate in Escherichia coli using a synthetic biological engineering approach. Journal of Biological Engineering 7 (24), 2013.

[8] Hahn, S. K. et al. Recovery and Characterization of Poly(3-Hydroxybutyric Acid) Synthesized in Alcaligenes eutrophus and Recombinant Escherichia coli. Applied and Environmental Microbiology 61 (1), 1995. 34 – 39.