Difference between revisions of "Part:BBa K5246045"

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The holdfast synthesis (<i>hfs</i>) genes include those encoding predicted glycosyltransferases, carbohydrate modification factors, and components of a wzy-type polysaccharide assembly pathway. [4][5][6]
 
The holdfast synthesis (<i>hfs</i>) genes include those encoding predicted glycosyltransferases, carbohydrate modification factors, and components of a wzy-type polysaccharide assembly pathway. [4][5][6]
  
<B>-->Full functional project operon assembly with this part and full operon characterization can be found in composite part <html><a href="https://parts.igem.org/Part:BBa_K5246046" target="_blank">BBa_K5246046</a></html>.</B>
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<HTML><p><B>-->Full functional project operon assembly with this part and full operon characterization can be found in composite part <a href="https://parts.igem.org/Part:BBa_K5246046" target="_blank">BBa_K5246046</a></B></p></html>
  
 
===Sequence and Features===
 
===Sequence and Features===
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All of the proteins composing this system are responsible for polysaccharide polymerization and export. Since the system's proteins are found in the membrane, we concluded that using a low-copy plasmid would decrease the probability of inclusion body formation. Their formation would diminish the functionality of our system, as the proteins would not allow the polysaccharide to be exported outside the bacteria.
 
All of the proteins composing this system are responsible for polysaccharide polymerization and export. Since the system's proteins are found in the membrane, we concluded that using a low-copy plasmid would decrease the probability of inclusion body formation. Their formation would diminish the functionality of our system, as the proteins would not allow the polysaccharide to be exported outside the bacteria.
  
To assemble specifically this part into <html><a href="https://parts.igem.org/Part:BBa_K5246046">BBa_K5246046</a></html> to then further assemble the holdfast synthesis pathway in <i> E. coli </i>, we had to assemble this part first into a backbone of pACYC-Duet-1 containing other composite part genes: <html><a href="https://parts.igem.org/Part:BBa_K5246045">BBa_K52460465/a></html>. We designed a strategy to maximize the success of plasmid assembly by first assembling plasmids with 3 genes (part:<html><a href="https://parts.igem.org/Part:BBa_K5246045">BBa_K52460465/a></html>) and, after verifying the sequences, integrating 3 left genes into that backbone (Fig. 1). In this way, we prevented Golden Gate assembly errors by trying to construct plasmids from 8 or more fragments.
+
To assemble specifically this part into <html><a href="https://parts.igem.org/Part:BBa_K5246046" target="_blank">BBa_K5246046</a></html> to then further assemble the holdfast synthesis pathway in <i> E. coli </i>, we had to assemble this part first into a backbone of pACYC-Duet-1 containing other composite part genes: <html><a href="https://parts.igem.org/Part:BBa_K5246044" target="_blank">BBa_K5246044</a></html>. We designed a strategy to maximize the success of plasmid assembly by first assembling plasmids with 3 genes (part:<html><a href="https://parts.igem.org/Part:BBa_K5246044" target="_blank">BBa_K5246044</a></html>) and, after verifying the sequences, integrating 3 left genes into that backbone (Fig. 1). In this way, we prevented Golden Gate assembly errors by trying to construct plasmids from 8 or more fragments.
  
 
<html>
 
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The <html><a href="https://parts.igem.org/Part:BBa_K5246045">BBa_K52460465/a></html> assembly was done using Golden Gate assembly with IIS AarI restriction enzyme sites introduced during PCR amplification. The backbone of pACYC-Duet-1 (Novagen) and fragments were amplified using Phusion Plus DNA polymerase, as the genome of <i> C. crescentus </i> has a high GC% content making the appearance of non-specific products during PCR amplification more common and primer design more challenging (Fig. 2). Since hfsA gene had an AarI RE site directly in the gene, this site was domesticated during side directed mutagenesis.
+
The <html><a href="https://parts.igem.org/Part:BBa_K5246045" target="_blank">BBa_K52460465</a></html> assembly was done using Golden Gate assembly with IIS AarI restriction enzyme sites introduced during PCR amplification. The backbone of pACYC-Duet-1 (Novagen) and fragments were amplified using Phusion Plus DNA polymerase, as the genome of <i> C. crescentus </i> has a high GC% content making the appearance of non-specific products during PCR amplification more common and primer design more challenging (Fig. 2). Since hfsA gene had an AarI RE site directly in the gene, this site was domesticated during side directed mutagenesis.
  
  
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       <figure>
 
       <figure>
 
         <div class="center">
 
         <div class="center">
           <img src="https://static.igem.wiki/teams/5246/webp/engineering/cb2-genes-genome.webp" style="width:350px;">
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           <img src="https://static.igem.wiki/teams/5246/results/creation-of-an-efficient-vector-system-for-holdfast-production-in-e-coli/pcr-from-genome-cb2.webp" style="width:350px;">
 
         </div>
 
         </div>
         <figcaption><center><b> Fig. 2. </b> Plasmid construction strategy. Plasmids are constructed in two rounds, cloning 3 genes at a time. Verified by colony PCR, restriction digestion analysis, and Nanopore sequencing </center></figcaption>
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         <figcaption><center><b> Fig. 2. </b> PCR amplification of target genes from the genome after purification  of C. crescentus CB2 </center></figcaption>
 
       </figure>
 
       </figure>
 
</html>
 
</html>
  
Due to the high amount of non-specific products, the fragments were gel-purified. Vectors and fragments composing this operon were mixed in equimolar amounts with GG reaction components and incubated as described in the <html><a href=" https://2024.igem.wiki/vilnius-lithuania/experiments/">protocol</a>. The reaction was later transformed into <i>E. coli</i> Mach1 (Thermo Scientific) competent cells. The assembly was then confirmed with restriction digest analysis (Fig. 3), and positive colonies were sequenced.  
+
Due to the high amount of non-specific products, the fragments were gel-purified. Vectors and fragments composing this operon were mixed in equimolar amounts with GG reaction components and incubated as described in the <html><a href=" https://2024.igem.wiki/vilnius-lithuania/experiments/" target="_blank">protocol</a>. The reaction was later transformed into <i>E. coli</i> Mach1 (Thermo Scientific) competent cells. The assembly was then confirmed with restriction digest analysis (Fig. 3), and positive colonies were sequenced.  
  
 
<html>
 
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</html>
 
</html>
  
After acquiring sequence-verified clones, we further cloned the 3 remaining genes: <html><a href="https://parts.igem.org/Part:BBa_K5246006">hfsF</a></html>,<html><a href="https://parts.igem.org/Part:BBa_K5246003">hfsC</a></html>, <html><a href="https://parts.igem.org/Part:BBa_K5246009#Bioinformatic_analysis">hfsI</a></html>, this was done the same way as the first 3 genes. After transformation into <I> E. coli </i>, obtained colonies were once again screened with cPCR (Fig. 4) and restriction digestion analysis (Fig. 5). After choosing positive colonies full plasmids with hfsA-hfsB-hfsD-hfsF-hfsC-hfsI were once again sequenced
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After acquiring sequence-verified clones, we further cloned the 3 remaining genes: <html><a href="https://parts.igem.org/Part:BBa_K5246006" target="_blank">hfsF</a></html>,<html><a href="https://parts.igem.org/Part:BBa_K5246003" target="_blank">hfsC</a></html>, <html><a href="https://parts.igem.org/Part:BBa_K5246009" target="_blank">hfsI</a></html>, this was done the same way as the first 3 genes. After transformation into <I> E. coli </i>, obtained colonies were once again screened with cPCR (Fig. 4) and restriction digestion analysis (Fig. 5). After choosing positive colonies full plasmids with hfsA-hfsB-hfsD-hfsF-hfsC-hfsI were once again sequenced and <b>fully characterized as a composite part <html><a href="https://parts.igem.org/Part:BBa_K5246046" target="_blank">BBa_K5246046</a></html></B>.
  
 
<html>
 
<html>
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       </figure>
 
       </figure>
 
</html>
 
</html>
 
<B>-->Full operon characterization can be found in composite part <html><a href="https://parts.igem.org/Part:BBa_K5246046" target="_blank">BBa_K5246046</a></html>.</B>
 
  
 
===References===
 
===References===

Latest revision as of 19:36, 29 September 2024


C.Crescentus CB2/CB2A hfsF-hfsC-hfsI Part of polysaccharide export apparatus

Introduction

Vilnius-Lithuania iGEM 2024 project Synhesion aspires to create biodegradable and environmentally friendly adhesives. We were inspired by bacteria, which naturally produce adhesives made from polysaccharides. Two bacteria from aquatic environments - C. crescentus and H. baltica - harness 12 protein synthesis pathways to produce sugars, anchoring them to the surfaces. We aimed to transfer the polysaccharide synthesis pathway to industrially used E. coli bacteria to produce adhesives. Our team concomitantly focused on creating a novel E. coli strain for more efficient production of adhesives.

This is a part of the complete holdfast polymerization and export apparatus BBa_K5246046 used in Vilnius-Lithuania iGEM 2024 project "Synhesion" https://2024.igem.wiki/vilnius-lithuania/. This part can also be used separately for polysaccharide export, but this feature needs more detailed characterization.

Usage and Biology

Caulobacter crescentus is a common freshwater gram-negative oligotrophic bacterium of the clade Caulobacterales. Its distinguishing feature is its dual lifestyle. Initially, C. crescentus daughter cells are in a “swarmer” cell phase, which has a flagellum, enabling them to perform chemotaxis. After the motile phase, they differentiate into “stalked” cells. This phase features a tubular stalk with an adhesive structure called a holdfast, allowing them to adhere to surfaces and perform cell division. [1][2]

Caulobacterales synthesize a polysaccharide-based adhesin known as holdfast at one of their cell poles, enabling tight attachment to external surfaces. It is established that holdfast consists of repeating identical units composed of multiple monomers. Current literature agrees that in Caulobacter crescentus, these units form tetrads composed of glucose, an unidentified monosaccharide (either N-mannosamine uronic acid or xylose), N-acetylglucosamine, and N-glucosamine. These units are polymerized and exported to the outer membrane of the cell, where they function as anchors, securing the bacterium to a surface[3][4]. The C. crescentus holdfast is produced via a polysaccharide synthesis and export pathway similar to the group I capsular polysaccharide synthesis Wzy/Wzx-dependent pathway in Escherichia coli. The holdfast synthesis (hfs) genes include those encoding predicted glycosyltransferases, carbohydrate modification factors, and components of a wzy-type polysaccharide assembly pathway. [4][5][6]

-->Full functional project operon assembly with this part and full operon characterization can be found in composite part BBa_K5246046

Sequence and Features


Assembly Compatibility:
  • 10
    INCOMPATIBLE WITH RFC[10]
    Illegal XbaI site found at 2813
    Illegal PstI site found at 1121
    Illegal PstI site found at 2620
  • 12
    INCOMPATIBLE WITH RFC[12]
    Illegal PstI site found at 1121
    Illegal PstI site found at 2620
    Illegal NotI site found at 2293
  • 21
    INCOMPATIBLE WITH RFC[21]
    Illegal BglII site found at 2039
    Illegal BglII site found at 2411
    Illegal BglII site found at 2816
    Illegal BglII site found at 3872
    Illegal BamHI site found at 181
    Illegal XhoI site found at 3286
  • 23
    INCOMPATIBLE WITH RFC[23]
    Illegal XbaI site found at 2813
    Illegal PstI site found at 1121
    Illegal PstI site found at 2620
  • 25
    INCOMPATIBLE WITH RFC[25]
    Illegal XbaI site found at 2813
    Illegal PstI site found at 1121
    Illegal PstI site found at 2620
    Illegal NgoMIV site found at 431
    Illegal NgoMIV site found at 539
    Illegal NgoMIV site found at 821
    Illegal NgoMIV site found at 878
    Illegal NgoMIV site found at 922
    Illegal NgoMIV site found at 953
    Illegal NgoMIV site found at 1177
    Illegal AgeI site found at 239
    Illegal AgeI site found at 3066
  • 1000
    COMPATIBLE WITH RFC[1000]

Experimental characterization

Part cloning

All of the proteins composing this system are responsible for polysaccharide polymerization and export. Since the system's proteins are found in the membrane, we concluded that using a low-copy plasmid would decrease the probability of inclusion body formation. Their formation would diminish the functionality of our system, as the proteins would not allow the polysaccharide to be exported outside the bacteria.

To assemble specifically this part into BBa_K5246046 to then further assemble the holdfast synthesis pathway in E. coli , we had to assemble this part first into a backbone of pACYC-Duet-1 containing other composite part genes: BBa_K5246044. We designed a strategy to maximize the success of plasmid assembly by first assembling plasmids with 3 genes (part:BBa_K5246044) and, after verifying the sequences, integrating 3 left genes into that backbone (Fig. 1). In this way, we prevented Golden Gate assembly errors by trying to construct plasmids from 8 or more fragments.

Fig. 1. Plasmid construction strategy. Plasmids are constructed in two rounds, cloning 3 genes at a time. Verified by colony PCR, restriction digestion analysis, and Nanopore sequencing


The BBa_K52460465 assembly was done using Golden Gate assembly with IIS AarI restriction enzyme sites introduced during PCR amplification. The backbone of pACYC-Duet-1 (Novagen) and fragments were amplified using Phusion Plus DNA polymerase, as the genome of C. crescentus has a high GC% content making the appearance of non-specific products during PCR amplification more common and primer design more challenging (Fig. 2). Since hfsA gene had an AarI RE site directly in the gene, this site was domesticated during side directed mutagenesis.


Fig. 2. PCR amplification of target genes from the genome after purification of C. crescentus CB2

Due to the high amount of non-specific products, the fragments were gel-purified. Vectors and fragments composing this operon were mixed in equimolar amounts with GG reaction components and incubated as described in the protocol. The reaction was later transformed into E. coli Mach1 (Thermo Scientific) competent cells. The assembly was then confirmed with restriction digest analysis (Fig. 3), and positive colonies were sequenced.

Fig. 3. Restriction digest analysis of C. crescentus CB2 pACYC-hfsA-hfsB-hfsD. On the left - expected in silico profile of restriction digest with EcoRI and ScaI, on the right - digested plasmids - 1-6 colonies, M - molecular weight ladder, GeneRuler DNA Ladder Mix (Thermo Scientific)

After acquiring sequence-verified clones, we further cloned the 3 remaining genes: hfsF,hfsC, hfsI, this was done the same way as the first 3 genes. After transformation into E. coli , obtained colonies were once again screened with cPCR (Fig. 4) and restriction digestion analysis (Fig. 5). After choosing positive colonies full plasmids with hfsA-hfsB-hfsD-hfsF-hfsC-hfsI were once again sequenced and fully characterized as a composite part BBa_K5246046.

Fig. 4. cPCR of C. crescentus CB2 hfsA-hfsB-hfsD-hfsC-hfsI Golden Gate assembly into pACYC-Duet-1. Expected product length - ~1.5kb. -C - negative control, 1-15 - different colonies, M - molecular weight ladder, GeneRuler DNA Ladder Mix (Thermo Scientific).

Fig. 5. Restriction digest analysis of C. crescentus CB2 pACYC-hfsA-hfsB-hfsD-hfsF-hfsC-hfsI. On the left - expected in silico profile of restriction digest with EcoRI, HindIII and XhoI, on the right - digested plasmids - 5,8,10,12,13 positive cPCR colonies, M - molecular weight ladder, GeneRuler DNA Ladder Mix (Thermo Scientific).

References

1. Hendrickson, H., & Lawrence, J. G. (2000). Mutational bias suggests that replication termination occurs near the dif site, not at Ter sites. FEMS Microbiology Reviews, 24(2), 177–183. https://doi.org/10.1111/j.1574-6976.2000.tb00539.x
2. Andrews, S. C., Robinson, A. K., & Rodríguez-Quiñones, F. (2004). Bacterial iron homeostasis. Journal of Bacteriology, 186(5), 1438–1447. https://doi.org/10.1128/jb.186.5.1438-1447.2004
3.Rabah, A., & Hanchi, S. (2023). Experimental and modeling study of the rheological and thermophysical properties of molybdenum disulfide-based nanofluids. Journal of Molecular Liquids, 384, 123335. https://doi.org/10.1016/j.molliq.2023.123335
4. Boutte, C. C., & Crosson, S. (2009). Bacterial lifestyle shapes stringent response activation. Journal of Bacteriology, 191(9), 2904-2912. https://doi.org/10.1128/jb.01003-08
5. Mackie, J., Liu, Y. C., & DiBartolo, G. (2019). The C-terminal region of the Caulobacter crescentus CtrA protein inhibits stalk synthesis during the G1-to-S transition. mBio, 10(2), e02273-18. https://doi.org/10.1128/mbio.02273-18
6.Thanbichler, M., & Shapiro, L. (2003). MipZ, a spatial regulator coordinating chromosome segregation with cell division in Caulobacter. Journal of Bacteriology, 185(4), 1432-1442. https://doi.org/10.1128/jb.185.4.1432-1442.2003