Difference between revisions of "Part:BBa K5325002"
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PLA depolymerases can be categorized into 2 types: Type I (proteases) - specific to cleave poly L-lactic acid (PLLA) - and Type II (lipases/cutinases/esterases) - preferentially cleave poly D-lactic acid (PDLA), with BBa_K5325002 matching the description of Type II as the original protein is an esterase with a preference towards cleaving poly(D,L)-lactate over strictly PLLA or PDLA<sup>[1,2]</sup>. While the mechanism of how PLA depolymerase binds to and hydrolyze PLA is still unknown, PLA depolymerase hydrolysis activity is known to increase as temperature approaches the hydrolysis temperature of PLA (>50 °C). | PLA depolymerases can be categorized into 2 types: Type I (proteases) - specific to cleave poly L-lactic acid (PLLA) - and Type II (lipases/cutinases/esterases) - preferentially cleave poly D-lactic acid (PDLA), with BBa_K5325002 matching the description of Type II as the original protein is an esterase with a preference towards cleaving poly(D,L)-lactate over strictly PLLA or PDLA<sup>[1,2]</sup>. While the mechanism of how PLA depolymerase binds to and hydrolyze PLA is still unknown, PLA depolymerase hydrolysis activity is known to increase as temperature approaches the hydrolysis temperature of PLA (>50 °C). | ||
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| + | ===Parts Preparation=== | ||
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| + | The four parts BBa_K5325000, BBa_K5325001, BBa_K5325002, and BBa_K5325003 were each assembled into different pRL814 vectors so that only 1 part out of 4 will be in a vector. All parts’ expressions in the pRL814 were controlled by the lac repressor and operon system. Afterwards, the assembled vectors were each transformed into <i>E. coli</i>, and the transformed <i>E. coli</i> are then conjugated with <i>S. oneidensis</i> so that the final result are 4 different <i>S. oneidensis</i> strains and each strain carrying one of the four above-mentioned parts. | ||
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| + | </p> | ||
===SDS-PAGE and Western Blot Results=== | ===SDS-PAGE and Western Blot Results=== | ||
Latest revision as of 08:09, 2 October 2024
RPA1511_plaA
An extracellular polylactic acid (PLA) depolymerase taken from Rhodopseudomonas palustris. able to digest PLA into oligomers and lactic acid monomers.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal NgoMIV site found at 70
- 1000INCOMPATIBLE WITH RFC[1000]Illegal SapI.rc site found at 820
Contents
NOTE: As the four parts BBa_K5325000, BBa_K5325001, BBa_K5325002, and BBa_K5325003 were experimented at the same time, experimental methods, results, and figures shown in the four parts' pages will be identical to one another.
Usage and Biology
Poly lactic acid (PLA) depolymerases have been found naturally in several microorganisms and they are able to facilitate digestion of the biopolymer PLA, producing oligomer chains and lactate monomers. This makes the protein a promising option for the clean up of PLA waste in the environment, which is not quite as biodegradable as the plastic was advertised to be and is still capable of persisting and polluting natural habitats. With that in mind, our team designed this part as a candidate for a PLA depolymerase part, originating from Rhodopseudomonas palustris (R. palustris) to allow an engineered bacteria with the part to cleave PLA to its oligomers and monomers, which can then be metabolized by the bacteria.
PLA depolymerases can be categorized into 2 types: Type I (proteases) - specific to cleave poly L-lactic acid (PLLA) - and Type II (lipases/cutinases/esterases) - preferentially cleave poly D-lactic acid (PDLA), with BBa_K5325002 matching the description of Type II as the original protein is an esterase with a preference towards cleaving poly(D,L)-lactate over strictly PLLA or PDLA[1,2]. While the mechanism of how PLA depolymerase binds to and hydrolyze PLA is still unknown, PLA depolymerase hydrolysis activity is known to increase as temperature approaches the hydrolysis temperature of PLA (>50 °C).
Parts Preparation
The four parts BBa_K5325000, BBa_K5325001, BBa_K5325002, and BBa_K5325003 were each assembled into different pRL814 vectors so that only 1 part out of 4 will be in a vector. All parts’ expressions in the pRL814 were controlled by the lac repressor and operon system. Afterwards, the assembled vectors were each transformed into E. coli, and the transformed E. coli are then conjugated with S. oneidensis so that the final result are 4 different S. oneidensis strains and each strain carrying one of the four above-mentioned parts.
SDS-PAGE and Western Blot Results
Five S. oneidensis strains that contained empty pRL814 vector, BBa_K5325000, BBa_K5325001, BBa_K5325002, and BBa_K5325003, respectively, were incubated overnight with 100μM IPTG at 30°C before being diluted to OD600nm=1. The resulting dilution was mixed with 0.5 μL of 1 M DTT and was incubated at 95°C for 10 minutes, spun down, and ran through a SDS-PAGE gel. Collected SDS-PAGE gel was then visualized using Western Blot with anti-FLAG antibodies to highlight the proteins of interest in the gel. The Western blot result is shown in Figure 1, which showed the resulting protein band size of RPA at 25-30 kDa. While this is below the predicted size of 34 kDa from RPA1511, the resulting band was considered to be within the expected range for the part BBa_K5325002[2].
Cell Lysate and Cell Supernatant HPLC Analysis
Five S. oneidensis strains with empty pRL814 vector, BBa_K5325000, BBa_K5325001, BBa_K5325002, and BBa_K5325003, respectively, were grown in LB broth cultures overnight before each culture had the supernatant and cells separated into different new LB broth media. All cells were lysed using the freeze-thaw method in which the cell cultures were subjected to cooling to -20 °C for 30 minutes before being heated to 37 °C for 3 times consecutively. Supernatant cultures and cell lysate cultures for all strains were incubated with low-molecular weight PLA beads and 100μM IPTG at 37 °C and 0.5 mL from supernatant culture and cell lysate each were taken after 24 hours for 5 days. Day 5 culture samples for supernatants and cell lysates of S. oneidensis were analyzed with HPLC for acetate and lactate concentrations. Lactate and acetic acid concentrations in Day 5 sample for the supernatant and cell lysate cultures of S. oneidensis containing the four parts and empty vector are shown in Figure 2 and Figure 3, respectively.
In Figure 2, the supernatants' HPLC result does not show any lactate content for all four parts. As the part was expected to cleave PLA to produce the monomer lactic acid, the result shown here indicate that the part was likely non-functional in the extracellular space. Abundance of acetate in all supernatant samples were likely a result of S. oneidensis metabolism in LB broth cultures, indicating that cells were growing and thus all the cells in the respective samples should have been able to express the parts. On the other hand, in Figure 3, the cell lysates' HPLC result for RPA indicated that the sample have the most lactate out of all samples in the treatment group. However, the amount of lactate produced in the negative control pRL814 empty vector was higher than that of ABO, which should have not been the case as the cell lysate negative control had no way of generating lactate in the LB media. Due to this result, a solid conclusion for the activity of the part BBa_K5325002 in the cell lysate samples cannot be made.
OD600 Analysis
The 5 S. oneidensis strains mentioned previously were grown in M5 minimum broth media supplemented with 200μM Lactate: one set with PLA and the other without PLA as the negative control, and each set having 3 replicates. All replicates were incubated at 30 °C with 100μM IPTG, and OD600 results were taken over the course of 6 days. As the parts were not transported out of the engineered bacteria due to the lack of a Sec system signal sequence, once the broth cultures enter their death phase on day 3, cells will burst open and release their contents, enabling the cytosolic PLA depolymerases to degrade PLA and the remaining cells to metabolize the produced lactate oligomers and monomers to persist longer than cells in cultures with no PLA. The cultures' longevity was predicted to be shown through a higher average OD600 relative to that of cultures with no PLA.
From the result of parametric t-test for paired samples, the strain with RPA (BBa_K5325002) did not show a statistically significant difference between the OD600 values of cultures with PLA and cultures without PLA at all time points. From this result, it is likely that the cytosolic part BBa_K5325002 is not active in the cell.
Possible Improved Parts
We have designed new parts with an N-terminus PelB signal sequence for periplasmic secretion and a C-terminus His tag for more affordable extraction columns. However, as of September 16th 2024, these new parts have not been successfully transformed into E. coli and thus cannot be tested for expression and activity.
References
1. Kawai, F., Nakadai, K., et al. (2011). Different enantioselectivity of two types of poly(lactic acid) depolymerases toward poly(l-lactic acid) and poly(d-lactic acid). Polym. Degrad. Stab. 96(7):1342-1348.
2. Hajighasemi, M., Nocek, B.P., et al. (2016). Biochemical and Structural Insights into Enzymatic Depolymerization of Polylactic Acid and Other Polyesters by Microbial Carboxylesterases. Biomacromolecules. 17(6):2027-2039