PAR_Ble_SP7_FAST-PETase_Ter

This composite part have: PAR promoter, the bleomycin/zeocin resistance sequence, signal peptide, the Fast-PETase, and the terminator. Designed to express and secrete Fast-PETase in Chlamydomonas reinhardtii, utilizing pJP32 backbone.

Sequence and Features

Introduction to the Mhetygua Project

The Mhetygua project, initiated for the IGEM Global 2023 edition, represents a pioneering endeavor to combat the pressing issue of microplastic pollution. Spearheaded by a dedicated group of students, the project titled "MHETYGUÁ: algae as devices for the degradation of aquatic pollutants" seeks to harness the potential of algae, specifically Chlamydomonas reinhardtii, as a bio-tool for microplastic degradation. Beyond the scientific pursuit, the project embodies a broader vision of fostering environmental awareness and education, aiming to catalyze a shift towards sustainable practices and a reduced plastic footprint in the Latin American region.

Commentary on the Genetic Circuit Construction: Circuit Number 1

The genetic circuit, labeled as Circuit Number 1, is meticulously designed to achieve the expression and secretion of the enzyme Fast-PETase in the microalgae Chlamydomonas reinhardtii. The construction of this circuit involves several key components:

1. PAR Promoter: Serving as the starting point of the circuit, the PAR promoter is chosen for its light-inducible properties, allowing for the modulation of gene expression based on light availability. This promoter is known for its efficacy in Chlamydomonas reinhardtii, making it an ideal choice for initiating the transcription of downstream genes.
2. Bleomycin/Zeocin Resistance Sequence: This sequence confers resistance to the antibiotics bleomycin and zeocin. By incorporating this resistance gene, it becomes feasible to select for algal cells that have successfully integrated the genetic circuit, ensuring the propagation of the desired trait.
3. Signal Peptide: A crucial component for ensuring the secretion of the enzyme, the signal peptide directs the synthesized Fast-PETase protein to the secretory pathway, facilitating its release into the external environment.
4. Fast-PETase: The central player of the circuit, Fast-PETase is an enzyme engineered for enhanced plastic degradation capabilities. Once expressed and secreted, this enzyme acts on microplastics, breaking them down into less harmful byproducts.
5. Terminator: Concluding the circuit, the terminator sequence ensures the proper end of transcription, providing stability and efficiency to the overall genetic expression process.

The entire circuit is integrated into the pJP32 backbone, a vector known for its compatibility with Chlamydomonas reinhardtii. This choice of backbone further ensures the successful integration and expression of the circuit within the algal cells.

Mhetyguá Parts

Mhetyguá Parts

PAR Promoter

We chose the PAR promoter because it is a promoter sequence commonly used in Chlamydomonas reinhardtii for the expression of transgenes. The promoter in question is light-inducible, and its activity is modulated by the availability of light-harvesting complexes, specifically the phycobilisome complex. PAR is relatively strong, and its expression can be adjusted by changing the intensity and duration of light exposure. This promoter is a combination of the HSP70A (upstream) and RBCS2 promoters; no heat shock is required as a transcription activator. Several characteristics of this promoter suggest its usefulness as a tool to enhance transgene expression in this alga. It can, by itself, confer high inducibility to a transgene.

Reference: Schroda, M., Blöcker, D., & Beck, C. F. (2000). The HSP70A promoter as a tool for the improved expression of transgenes in Chlamydomonas. Plant Journal, 21(2), 121-131. <a href="https://doi.org/10.1046/j.1365-313x.2000.00652.x">https://doi.org/10.1046/j.1365-313x.2000.00652.x</a>

Ble Resistance Gene

The bleomycin resistance gene confers resistance to the antibiotic bleomycin and zeocin. In the context of Chlamydomonas reinhardtii the bleomycin resistance of cells harboring the Sh ble gene is attributed to the action of the bleomycin-binding protein. This protein binds to bleomycin, sequestering it and preventing it from exerting its antibiotic effect on the cell. This resistance mechanism is particularly useful in genetic engineering experiments. By introducing the Sh ble gene alongside other genes of interest into Chlamydomonas reinhardtii, researchers can easily select for cells that have taken up the foreign DNA by exposing them to bleomycin. Only the cells that have incorporated the Sh ble gene (and by extension, the other genes of interest) will survive, allowing for efficient selection.

Reference: Gatignol, A., Durand, H., & Tiraby, G. (1988). Bleomycin resistance conferred by a drug‐binding protein. FEBS Letters, 230.

SP7 Signal Peptide

For the constructs expressed in Chlamydomonas reinhardtii, we used the signal peptide SP7 which has been recently characterized in a paper by João Molino. SP7 is a novel protein identified in the flagella of Chlamydomonas reinhardtii. The flagella are whip-like appendages that protrude from the cell body and are vital for motility and sensory functions. Which confers an interesting capacity to secrete recombinant proteins.

Reference: Molino JVD, de Carvalho JCM, Mayfield SP (2018) Comparison of secretory signal peptides for heterologous protein expression in microalgae: Expanding the secretion portfolio for Chlamydomonas reinhardtii. PLoS ONE 13(2): e0192433. <a href="https://doi.org/10.1371/journal.pone.0192433">https://doi.org/10.1371/journal.pone.0192433</a>

FAST-PETase Enzyme

FAST-PETase is derived from the original sequence of the PETase enzyme, with several modifications introduced through directed evolution. The FAST-PETase sequence is approximately 590 amino acids in length and consists of several domains, including a signal peptide sequence for secretion (twin-arginine translocation (Tat) signal peptide), a catalytic domain, and a carbohydrate-binding module. The catalytic domain is responsible for breaking the ester bonds in PET, while the carbohydrate-binding module helps anchor the enzyme to the plastic surface. Directed mutations have enhanced the enzyme's ability to bind to PET and break it down into its components more quickly. Therefore, we chose FAST-PETase because it is capable of breaking down PET at a faster rate than the original PETase enzyme.

Reference: Lu, H., Diaz, D.J., Czarnecki, N.J. et al. Machine learning-aided engineering of hydrolases for PET depolymerization. Nature 604, 662–667 (2022). <a href="https://doi.org/10.1038/s41586-022-04599-z">https://doi.org/10.1038/s415 Continue