PART COLLECTION
Best part collection - a toolkit to functionalise BC with proteins
During the making of our project, we discovered that bacterial cellulose (BC) is an incredibly versatile material with a lot of applications. Because we are firm believers in collaborative science, we have developed a toolkit to further utilise this material. The goal of this part collection is to give future iGEM teams -or other researchers- a head start when developing new applications for BC.
This part collection consists of 11 (C3-13) composite parts, which are made up from twenty-two basic parts. Central to this part collection are the basic parts dCBD and cipA, the two cellulose binding domains (CBDs) investigated during this project. These parts are obtained from previous iGEM teams and adapted/applied in our toolkit (BBa_K1321340 and BBa_K4380000). dCBD is a family one CBD, which utilises disulphide bonds and aromatic residues for binding, and generally only binds to crystalline cellulose1. cipA is a family three CBD, which binds to both crystalline and amorphous cellulose using a large beta-strand framework2.
Other basic parts (B4 - B12) in this collection are reporter proteins, such as GFP, or functional proteins that we have used to modify the BC properties, such as HFBI to increase hydrophobicity, or to add properties, such as Cry3Aa to confer toxicity to beetle species. The basic parts B13-B22 are parts we used to correctly express our proteins, such as linker sequences and genes that make up our expression plasmids.
The first two composite parts in this collection are the two expression plasmids we used in our project, one for Escherichia coli and one for Saccharomyces cerevisiae. We decided to work with two different organisms to facilitate both ex situ and in situ protein functionalisation approaches. Proteins produced by E. coli can be purified using their His-tag and combined with BC after harvesting. Proteins produced by S. cerevisiae are secreted into the culture medium through their signal peptide and are incorporated into the BC while it grows. The remaining eleven composite parts are coding sequences ready to be inserted into these plasmids. This allows for quick and easy expression of these proteins. We highly encourage any future iGEM teams to expand upon this toolbox by adding more protein sequences to the toolbox that allow for different BC properties.
Composite parts
| Nr. | Name | Nickname | Used in | Description | Relevance |
|---|---|---|---|---|---|
| C1 | BBa_259CTPBX | pBCD5_KanR | E. coli | Plasmid backbone containing a T7 expression system, bicistronic design element, a kanamycin resistance gene, and a p15A origin of replication. | This plasmid backbone can be used to express proteins in E. coli strains that have a T7 polymerase on their genome, such as the NiCo21 (DE3) strain that was used in this project. Additionally, the empty vector may also be used to validate transformation protocols. |
| C2 | BBa_250N9BLI | plasmid_CEN-ARS_KanMX | S. cerevisiae | Plasmid backbone no coding sequence for a functional protein. Contains the CEN/ARS ori and KanMX marker. | This plasmid backbone can be used to express proteins in S. cerevisiae. Additionally, the empty vector may also be used to validate transformation protocols and act as a control. |
| C3 | BBa_25OFBAY0 | cipA_sfGFP | E. coli | Coding sequence for the expression of the cipA-sfGFP fusion protein in E. coli. Contains a His-tag for purification purposes. | The cipA-sfGFP fusion protein was used to validate the binding affinity of the cipA domain to BC by measuring the strength of the fluorescent signal after treating BC with protein solution followed by a washing step. |
| C4 | BBa_25SRDDT7 | mUkG1_cipA_AGA2 | S. cerevisiae | Coding sequence for the expression of the mUkG1-cipA fusion protein in S. cerevisiae. Contains a AGA2 signal peptide for secretion. | The mUkG1-cipA fusion protein was used to validate the binding affinity of the cipA domain to BC by measuring the strength of the fluorescent signal after treating BC with protein solution followed by a washing step. |
| C5 | BBa_25258K5R | mUkG1_dCBD_AGA2 | S. cerevisiae | Coding sequence for the expression of the mUkG1-dCBD fusion protein in S. cerevisiae. Contains a AGA2 signal peptide for secretion. | The mUkG1-dCBD fusion protein was used to validate the binding affinity of the cipA domain to BC by measuring the strength of the fluorescent signal after treating BC with protein solution followed by a washing step. |
| C6 | BBa_25MVPDX0 | Spycatcher003_sfGFP_6xHis | E. coli | Coding sequence for the expression of the Spycatcher003-sfGFP fusion protein in E. coli. The spycatcher003 domain may be used to link the sfGFP to proteins containing the Spytag003 peptide. Contains a His-tag for purification purposes. | The Spycatcher003-sfGFP fusion protein was used to validate and quantify the presence of the other fusion proteins produced by S. cerevisiae. Because these proteins all had a Spytag003 domain, this part could be covalently attached to them, which allowed for quantification of the sfGFP fluorescent signal. |
| C7 | BBa_25N5WL5K | cipA_Cry3Aa | E. coli | Coding sequence for the expression of the cipA-Cry3Aa fusion protein in E. coli. Contains a His-tag for purification purposes. | The cipA-Cry3Aa fusion protein was used to make BC toxic to Coleoptera. The protein was immobilised on the seed coating which caused starvation effects, indicative of reduced feeding behaviour, in mealworms (Alphitobius diaperinus). This marks the first step towards using our seed coatings as a more sustainable alternative to classical pesticides. |
| C8 | BBa_258PB1SY | HFBI_cipA_AGA2 | S. cerevisiae | Coding sequence for the expression of the HFBI-cipA fusion protein in S. cerevisiae. Contains a AGA2 signal peptide for secretion. | The HFBI-cipA fusion protein can be used to increase the hydrophobicity of BC. This can be advantageous for the delayed germination of seeds. |
| C9 | BBa_25M93E07 | HFBI_dCBD_AGA2 | S. cerevisiae | Coding sequence for the expression of the HFBI-dCBD fusion protein in S. cerevisiae. Contains a AGA2 signal peptide for secretion. | The HFBI-dCBD fusion protein can be used to increase the hydrophobicity of BC. This can be advantageous for the delayed germination of seeds. |
| C10 | BBa_25JO5U5D | CBH1_cipA_AGA2 | S. cerevisiae | Coding sequence for the expression of the CBH1-cipA fusion protein in S. cerevisiae. Contains a AGA2 signal peptide for secretion. | The CBH1-cipA fusion protein has a cellulase-like effect on BC. This means that the biodegradability of the material will be improved, which can speed up the release of active compounds contained in the coating. |
| C11 | BBa_25FPHHHE | CBH1_dCBD_AGA2 | S. cerevisiae | Coding sequence for the expression of the CBH1-dCBD fusion protein in S. cerevisiae. Contains a AGA2 signal peptide for secretion. | The CBH1-dCBD fusion protein has a cellulase-like effect on BC. This means that the biodegradability of the material will be improved, which can speed up the release of active compounds contained in the coating. |
| C12 | BBa_25WDECJ3 | AmilCPblue_dCBD_AGA2 | S. cerevisiae | Coding sequence for the expression of the AmilCPblue-dCBD fusion protein in S. cerevisiae. Contains a AGA2 signal peptide for secretion. | The AmilCPblue-dCBD fusion protein can stain the BC matrix with a blue colour, allowing us to change the colour of our seed coatings. From our human practices, we learned that colour is a very important factor for farmers, because a uniform colour signifies a high quality product. |
| C13 | BBa_25FS93QF | AmilGFPyellow_dCBD_AGA2 | S. cerevisiae | Coding sequence for the expression of the AmilGFPyellow-dCBD fusion protein in S. cerevisiae. Contains a AGA2 signal peptide for secretion. | The AmilGFPyellow-dCBD fusion protein can stain the BC matrix with a yellow colour, allowing us to change the colour of our seed coatings. From our human practices, we learned that colour is a very important factor for farmers, because a uniform colour signifies a high quality product. |
Basic parts
| Nr. | Name | Nickname | Used in | Description | Relevance |
|---|---|---|---|---|---|
| B1 | BBa_K1321340 | dCBD | E. coli | Synthetic double cellulose binding domain. Contains two domains from Trichoderma reesei cellobiohydrolases, spaced by a linker sequence. | dCBD is a CBD belonging to family 1 of the CBDs. In this project, it was used to fuse several active proteins that were produced in S. cerevisiae to the surface of BC to change the material properties. |
| B2 | BBa_25B74R7S | cipA | E. coli | Cellulose binding domain from Clostridium thermocellum. | cipA is a CBD belonging to family 3 of the CBDs. In this project it was used to fuse several active proteins that were produced in S. cerevisiae or E. coli to the surface of BC to change the material properties. This version of cipA is codon optimised for expression in E. coli. |
| B3 | BBa_257HMYMW | cipA | S. cerevisiae | Cellulose binding domain from Clostridium thermocellum. | cipA is a CBD belonging to family 3 of the CBDs. In this project it was used to fuse several active proteins that were produced in S. cerevisiae or E. coli to the surface of BC to change the material properties. This version of cipA is codon optimised for expression in S. cerevisiae. |
| B4 | BBa_25G620IT | sfGFP | E. coli | Superfolder green fluorescent protein. | Superfolder GFP is a variant of the GFP molecule that performs much better than its wild type variant when fused to a different protein domain. Whereas the wild type might have trouble correctly folding when fused to poorly folded polypeptides, sfGFP does not share these struggles, making it a popular choice in fusion protein production. In this project it was fused to cipA and Spycatcher003 to validate and quantify CBD binding affinity. |
| B5 | BBa_25VKT7TL | mUkG1 | S. cerevisiae | Monomeric variant of Umikinoko-Green fluorescent protein. | mUkG1 is a green fluorescent protein derived from a soft coral. This fluorophore has been reported to perform much better in yeast than traditional GFP variants. For that reason, this protein was chosen to act as a reporter in our CBD yeast toolkit. |
| B6 | BBa_250L082D | Spytag003 | E. coli | Can undergo protein-protein interactions with its Spycatcher003 counterpart to form a covalent bond. | This part was fused to cellulose-binding fusion proteins produced by S. cerevisiae. This allowed for detection and quantification of these proteins using Spytag003’s counterpart, Spycatcher003, fused to an sfGFP molecule. |
| B7 | BBa_25A7C85Z | Spycatcher003 | E. coli | Can undergo protein-protein interactions with its Spytag300 counterpart to form a covalent bond. | This part was fused to an sfGFP molecule. This allowed for detection and quantification of cellulose-binding fusion proteins produced by S. cerevisiae, as these were fused to Spycatcher003’s counterpart, Spytag003. |
| B8 | BBa_2544O00E | Cry3Aa | E. coli | Insecticidal protein from Bacillus thuringiensis. | The bt protein Cry3Aa is naturally produced by Bacillus thuringiensis subsp. tenebrionis and is toxic to members of the order Coleoptera. In this project, it was investigated to be used as a biological control to protect seeds from pest insects. |
| B9 | BBa_254BBZE3 | AmilCPblue | S. cerevisiae | Blue chromoprotein. | AmilCPblue was fused to a cellulose binding domain to change the colour of the BC matrix. Although this is purely an aesthetic change, we have found this to be a very important factor for our customers. |
| B10 | BBa_2538H5OR | AmilGFPyellow | S. cerevisiae | Yellow chromoprotein. | AmilGFPyellow was fused to a cellulose binding domain to change the colour of the BC matrix. Although this is purely an aesthetic change, we have found this to be a very important factor for our customers. |
| B11 | BBa_25INM0JW | HFBI | S. cerevisiae | Class II hydrophobin 1 (HFBI) is a small hydrophibic protein derived from Trichoderma reesei. | HFBI was fused to a cellulose binding domain to make BC more hydrophobic, which can be useful for delayed germination purposes. |
| B12 | BBa_25L5H7E5 | CBH1 | S. cerevisiae | Exocellobiohydrolases 1 (CBH1) can catalyse the hydrolysis of 1,4-beta-D-glucosidic bonds in cellulose to release the disaccharide cellobiose, improving the biodegradability. | CBH1 was fused to a cellulose binding domain to increase the biodegradability of BC. Increasing the biodegradability allows for faster release of embedded compounds. |
| B13 | BBa_K1614000 | T7 promoter | E. coli | Promoter from T7 bacteriophage. Very strong promoter, often used for protein expression. | The T7 promoter was used to produce heterologous proteins in E. coli. Because it is controlled by a separate DNA-polymerase than the rest of the genome -which itself is placed under the control of an inducible promoter- it is possible to achieve very high protein titres. |
| B14 | BBa_25KVSR5Q | BCD5 | E. coli | Bicistronic design element. Facilitates binding of the ribosomes to the RNA, and thus protein production. | Bicistronic design elements greatly improve protein production when compared to monocistronic design elements. It was used to achieve high protein titres. |
| B15 | BBa_25X9RPLK | Synthetic terminator | E. coli | Synthetic terminator consisting of a stem-loop and a T-stretch. | This terminator was used to arrest transcription of the coding sequences on our production plasmid in E. coli. |
| B16 | BBa_25U4ZG1K | p15A_ORI | E. coli | Medium copy origin of replication. | The p15A_ORI ensures replication of the plasmid alongside the genome. Plasmids with a p15A_ORI have a range of about 20-30 copies per cell. |
| B17 | BBa_258UIRIC | NeoR/KanR | E. coli | Gene that confers antibiotic resistance to neomycin and kanamycin. | This gene makes bacteria immune to neomycin and kanamycin. This allows for selection of cells that have successfully integrated the plasmid, and ensures the plasmid is not lost over time. |
| B18 | BBa_25ZYLAYB | NEOKAN_promoter | E. coli | Constitutive promoter to continually express the NeoR/KanR gene. | This strong constitutive promoter was used to ensure that the antibiotic resistance gene was always active. |
| B19 | BBa_2563QDP3 | (GGGGS)3 linker | S. cerevisiae | Flexible linker designed for fusion proteins. | This linker was used to separate protein domains in a fusion protein, ensuring that their function is not affected by steric hindrance. |
| B20 | BBa_25BVPI08 | GSTG linker | E. coli | Short, rigid linker designed for fusion proteins. | This linker is used to separate protein domains in a fusion protein, ensuring that their function is not affected by steric hindrance. |
| B21 | BBa_K3033006 | 6xHIS | E. coli | Protein tag consisting of six histidine residues. | The 6xHIS-tag was used for protein purification. |
| B22 | BBa_25DJZF34 | AGA2 | S. cerevisiae | The AGA2 signal peptide is used for protein secretion in yeast. | AGA2 was fused to all fusion proteins produced in S. cerevisiae to allow for protein secretion into the medium. |
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