Difference between revisions of "Part:BBa K5117042"
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<b>Main purpose of use:</b> Immobilization of PpBglB on the spore crust of <i>B. subtilis</i> (spore surface display) | <b>Main purpose of use:</b> Immobilization of PpBglB on the spore crust of <i>B. subtilis</i> (spore surface display) | ||
− | <b> | + | <b>Potential application:</b> Degradation of cellobiose |
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− | <html><center><img src="https://static.igem.wiki/teams/5117/parts-registry/spore-display/ppbglb/ppbglb-l2-part.png" style="width: | + | <html><center><img src="https://static.igem.wiki/teams/5117/parts-registry/spore-display/ppbglb/ppbglb-l2-part.png" style="width: 20%; height: auto;"></center></html> |
<p class="image_caption"><center> <font size="1"><b> Fig. 1: Agarose gel electrophoresis: PCR of PpBglB-L2. </b> Oligonucleotides for amplification can be found on the <html><a href="https://2024.igem.wiki/tu-dresden/experiments">Experiments</a></html> page. The correct PCR product has a size of 1421 bp. 1 kb Plus DNA Ladder (NEB) served as marker (M). The PCR product was purified by gel extraction resulting in a DNA concentration of 190.5 ng/µl. </font></center></p> | <p class="image_caption"><center> <font size="1"><b> Fig. 1: Agarose gel electrophoresis: PCR of PpBglB-L2. </b> Oligonucleotides for amplification can be found on the <html><a href="https://2024.igem.wiki/tu-dresden/experiments">Experiments</a></html> page. The correct PCR product has a size of 1421 bp. 1 kb Plus DNA Ladder (NEB) served as marker (M). The PCR product was purified by gel extraction resulting in a DNA concentration of 190.5 ng/µl. </font></center></p> | ||
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+ | <img src="https://static.igem.wiki/teams/5117/parts-registry/spore-display/ppbglb/ppbglb-l2-ecoli.png" alt="Image 1"> | ||
+ | </div> | ||
+ | <div class="image-container image2"> | ||
+ | <img src="https://static.igem.wiki/teams/5117/parts-registry/spore-display/ppbglb/ppbglb-spore-ecoli-control.png" alt="Image 2"> | ||
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<p class="image_caption"><center> <font size="1"><b> Fig. 4: Agarose gel electrophoresis: Insert amplification of P<sub><i>cotYZ</i></sub>-PpBglB-L2-<i>cotY</i>-B0014 by Colony PCR of transformed <i>E. coli</i> DH10β cells. </b> | <p class="image_caption"><center> <font size="1"><b> Fig. 4: Agarose gel electrophoresis: Insert amplification of P<sub><i>cotYZ</i></sub>-PpBglB-L2-<i>cotY</i>-B0014 by Colony PCR of transformed <i>E. coli</i> DH10β cells. </b> | ||
− | Oligonucleotides for amplification can be found on the <html><a href="https://2024.igem.wiki/tu-dresden/experiments">Experiments</a></html> page. Numbers 1-8 correspond to chosen colonies. The correct PCR product has a size of 2329 bp. The negative control displayed no bands. 1 kb Plus DNA Ladder (NEB) served as marker (M). | + | Oligonucleotides for amplification can be found on the <html><a href="https://2024.igem.wiki/tu-dresden/experiments">Experiments</a></html> page. Numbers 1-8 correspond to chosen colonies. The correct PCR product has a size of 2329 bp. The negative control displayed no bands. 1 kb Plus DNA Ladder (NEB) served as marker (M). Colonies 4 and 8 were verified by sequencing, but no correct insert sequence was found. </font></center></p> |
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− | <!-- Uncomment this to enable Functional Parameter display | + | <!-- Uncomment this to enable Functional Parameter display |
===Functional Parameters=== | ===Functional Parameters=== | ||
− | <partinfo>BBa_K5117042 parameters</partinfo> | + | <partinfo>BBa_K5117042 parameters</partinfo><!-- --> |
Latest revision as of 05:47, 2 October 2024
PcotYZ-BsRBS-PpBglB-L2-CotY-B0014
This part serves as transcriptional unit composed of:
- promoter PcotYZ of Bacillus subtilis (BBa_K5117021)
- ribosome binding site of Bacillus subtilis (BBa_K5117000)
- bglB gene of Paenibacillus polymyxa encoding a β-glucosidase (EC 3.2.1.21),
- cotY gene of Bacillus subtilis (BBa_K5117022)
- bidirectional terminator B0014 (BBa_B0014)
Biosafety level: S1
Target organism: Bacillus subtilis
Main purpose of use: Immobilization of PpBglB on the spore crust of B. subtilis (spore surface display)
Potential application: Degradation of cellobiose
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 1627
- 1000COMPATIBLE WITH RFC[1000]
Enzyme characterization according to literature
The characterization of the enzyme included in this composite part can be found on the basic part page (BBa_K5117030) of the enzyme.
Construct design
For compatibility with the BioBrick RFC[10] standard, the restriction sites EcoRI, XbaI, SpeI, PstI and NotI were removed from the coding sequence (CDS). To make the part compatible with the Type IIS standard, BsaI and SapI sites were removed as well. This was achieved by codon exchange using the codon usage table of Bacillus subtilis (Codon Usage Database Kazusa).
To express target genes only under sporulation, the sporulation-dependent promoter PcotYZ of B. subtilis was chosen. In previous studies, this promoter has so far provided the highest activity for spore surface display (Bartels et al. 2018, unpublished data of Elif Öztel). The promoter was followed by the ribosome binding site (RBS) for the host B. subtilis with a 7 bp spacer.
To anchor the target enzyme on the spore surface, it was fused to the N-terminus of the anchor protein CotY. This anchor is located in the crust, the outermost spore layer, and has been shown to be well suited for protein immobilization (McKenney et al. 2013, Bartels et al. 2018, Lin et al. 2020).
Moreover, different linkers between the fused target enzyme and anchor protein were analyzed, as these proteins may affect the folding and stability of each other and, eventually, lead to misfolding and reduced activity. Whereas flexible linkers promote the movement of joined proteins and are usually composed of small amino acids (e.g. Gly, Ser, Thr), rigid linkers are usually applied to maintain a fixed distance between the domains (Chen et al. 2013).
Within the framework of the TU Dresden iGEM 2024 Team, three linkers have been tested: 1) A short flexible GA linker (L1) encoding the small amino acids Gly and Ala, 2) A long flexible linker (GGGGS)4 (L2) which is one of the most common flexible linkers consisting of Gly and Ser residues and 3) A rigid linker GGGEAAAKGGG (L3) in which the EAAAK motif results in the formation of an alpha helix providing high stability (Chen et al. 2013).
The composite part documented in this page contains the long flexible linker (GGGGS)4.
Following the CDS of cotY, a spacer consisting of 10 bp of the natural genome sequence downstream from the cotYZ operon was inserted. This creates space before the terminator and ensures that the ribosome is able to read the full length of the CDS. The construct ends with the terminator B0014, a bidirectional terminator consisting of B0012 and B0011.
The entire construct was flanked with the BioBrick prefix and suffix, allowing for cloning via the BioBrick assembly standard and restriction-ligation-cloning. The vector pBS1C from the Bacillus BioBrickBox was used as an integrative plasmid backbone enabling genomic integration into the amyE locus of B. subtilis (Radeck et al. 2013).
Construction of spore display plasmids
First, all biological parts including the enzyme candidate (Fig. 1) as well as the promoter PcotYZ, the terminator B0014 and the anchor gene cotY (Fig. 2) were amplified by PCR and purified using the HiYield® PCR Clean-up/Gel Extraction Kit (SLG, Germany). The RBS was added by oligonucleotides. The plasmid pSB1C3-PpBglB generated in the subcloning phase served as template for PCR of the enzyme candidate (see BBa_K5117018). The linker was added by oligonucleotides. The promoter and anchor gene were amplified from genomic DNA of B. subtilis W168 and the terminator from a plasmid provided by the laboratory collection of Prof. Thorsten Mascher (General Microbiology, TU Dresden).
The composite part was subsequently assembled via Overlap PCR by complementary overhangs, which were designed and added by oligonucleotides (Fig. 3).
Afterwards, the Overlap PCR product was cloned into the vector backbone pBS1C enabling genome integration into the amyE locus in B. subtilis (Radeck et al. 2013). For that purpose, the insert as well as pBS1C were digested with EcoRI and PstI and purified by PCR clean up (DNA concentration: 31.9 ng/µl and 25 ng/µl respectively) using the HiYield® PCR Clean-up/Gel Extraction Kit (SLG, Germany).
After ligation, the plasmid was transformed into chemically competent E. coli DH10β cells and transformants were selected by ampicillin resistance (100 μg/ml ampicillin) encoded on the vector backbone. As the vector was purified via PCR clean up, the vector backbone might re-ligate with the original RFP insert, but colonies with re-ligated plasmids appear pink on the plate and can therefore be distinguished from correct transformants.
The negative control containing no DNA showed no growth. The positive control containing pBS1C resulted in a pink bacterial lawn. The re-ligation control containing the digested vector pBS1C led to growth of approximately 400 pink and 20 white colonies. The transformation with the spore display plasmid pBS1C-PcotYZ-PpBglB-L2-cotY-B0014 resulted in ≈ 300-400 colonies, both pink and white ones.
White colonies transformed with the spore display plasmid were analyzed by Colony PCR and agarose gel electrophoresis (Fig. 4). Colonies with a band at the correct size of the insert were chosen for plasmid isolation according to the HiYield® Plasmid Mini DNA Kit (SLG, Germany) and verified via sequencing by Microsynth Seqlab GmbH. After testing multiple colonies, however, no correct insert sequence was found. Consequently, the spore display plasmid pBS1C-PcotYZ-PpBglB-L2-cotY-B0014 was not constructed and could not be characterized in subsequent assays.
References
Bartels J., López Castellanos S., Radeck J., Mascher T. (2018): Sporobeads: The utilization of the Bacillus subtilis endospore crust as a protein display platform. ACS synthetic biology 7(2), 452-461. https://doi.org/10.1021/acssynbio.7b00285
Chen X., Zaro J. L., Shen, W. C. (2013): Fusion protein linkers: property, design and functionality. Advanced drug delivery reviews 65(10), 1357-1369. https://doi.org/10.1016/j.addr.2012.09.039
McKenney P. T., Driks A., Eichenberger P. (2013): The Bacillus subtilis endospore: assembly and functions of the multilayered coat. Nature Reviews Microbiology 11 (1), 33–44. https://doi.org/10.1038/nrmicro2921
Lin P., Yuan H., Du J., Liu K., Liu H., Wang T. (2020): Progress in research and application development of surface display technology using Bacillus subtilis spores. Applied microbiology and biotechnology 104 (6), 2319–2331. https://doi.org/10.1007/s00253-020-10348-x
Öztel, E. & Mascher T. (2024): unpublished data.
Radeck J., Kraft K., Bartels J., Cikovic T., Dürr F., Emenegger J., Kelterborn S., Sauer C., Fritz G., Gebhard S., Mascher T. (2013): The Bacillus BioBrick Box: generation and evaluation of essential genetic building blocks for standardized work with Bacillus subtilis. Journal of biological engineering 7, 1-17. https://doi.org/10.1186/1754-1611-7-29
Vellanoweth R. L. & Rabinowitz J. C. (1992): The influence of ribosome‐binding‐site elements on translational efficiency in Bacillus subtilis and Escherichia coli in vivo. Molecular microbiology 6(9), 1105-1114. https://doi.org/10.1111/j.1365-2958.1992.tb01548.x