Difference between revisions of "Part:BBa K3904405"
 
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<partinfo>BBa_K3904405 short</partinfo>
  
  
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[[File:T--Vilnius-Lithuania--amebyeLogo dark.png|right|100px|AmeBye]]
 
[[File:T--Vilnius-Lithuania--amebyeLogo dark.png|right|100px|AmeBye]]
  
Vilnius-Lithuania iGEM 2021 project [https://2021.igem.org/Team:Vilnius-Lithuania <b>AmeBye</b>]looks at amebiasis holistically and comprehensively, therefor target <i>E. histolytica</i> from several angles: prevention and diagnostics. As a tool to prevent amebiasis, the team created probiotics capable of naringenin biosynthesis. For the diagnostic part, the project includes a rapid, point of care, user-friendly diagnostic test identifying extraintestinal amebiasis. The main components of this test are aptamers, specific to the <i>E. histolytica</i> secreted proteins. These single-stranded DNA sequences fold into tertiary structures for particular fit with target proteins.
+
Vilnius-Lithuania iGEM 2021 project [https://2021.igem.org/Team:Vilnius-Lithuania <b>AmeBye</b>]looks at amebiasis holistically and comprehensively, therefore target <i>E. histolytica</i> from several angles: prevention and diagnostics. Our team's preventive solution consists of probiotics engineered to produce naringenin - an antiprotozoal compound. Two strains of genetically modified microorganisms were chosen as the main chassis - world-renowned <i>Lactobacillus casei</i> BL23 (<i>Lactobacillus paracasei</i>) and <i>Escherichia coli</i>  Nissle 1917. Furthermore, the team made specific gene deletions to enhance naringenin production and adapted a novel toxin-antitoxin system to prevent GMO spreads into the environment. The diagnostic part includes a rapid, point of care, user-friendly diagnostic test identifying extraintestinal amebiasis. The main components of this test are aptamers specific to the <i>E. histolytica</i> secreted proteins. These single-stranded DNA sequences fold into tertiary structures for particular fit with target proteins.
  
 
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=Usage and Biology=
 
=Usage and Biology=
  
CRISPR-Cas9 is a versatile genome-editing technique. In our approach to editing <i>E. coli</i> Nissle 1917 genome, we have used two plasmid based system enabling to combine of Lambda Red recombination and CRISPR-Cas9 as counterselection tools - [https://www.addgene.org/62225/ pCas] and [https://www.addgene.org/62226/ pTarget].  
+
CRISPR-Cas9 is a versatile genome-editing technique. In our approach to editing <i>E. coli</i> Nissle 1917 genome, we have used two plasmid based system enabling to combine of Lambda Red recombination and CRISPR-Cas9 as counterselection tools encoded in [https://www.addgene.org/62225/ pCas] and [https://www.addgene.org/62226/ pTarget].  
  
 
==Mechanism of genome editing==
 
==Mechanism of genome editing==
  
pCas plasmid is used for Cas9, Lambda Red system expression, and plasmid curing of pTarget. Cas9 - the RNA-guided endonuclease - is expressed constitutively, while the expression of Lambda Red genes (Gam, Exo, Beta) is under the control of arabinose inducible promoter araBp. pTarget plasmid caries constitutively expressed single-guide RNA (sgRNA). This RNA molecule, as and in nature, is composed of two central parts: CRISPR RNA (crRNA) and trans-activating crispr RNA(tracrRNA). crRNA is 17-20 nt length RNA sequence complementary to the targeted DNA adjacent to the protospacer adjacent motif (PAM) and tracrRNA is the scaffold for the Cas (in this case Cas9) nuclease binding to guide RNA and forming the ribonucleoprotein complex (1). In nature those two parts exist as two separate RNA molecules and tracrRNA participates in pre-crRNA maturation(2), however, in laboratory experiments they are usually combined into one single-guide RNA (sgRNA) obviating additional processing of pre-crRNA. As both pCas and pTarget plasmids are in a cell, Cas9 nuclease and sgRNA are able to form ribonucleoprotein complex and perform a double-strand break in the chosen part of the DNA. However, if arabinose has been added to the cell culture and a double-stranded DNA repair template is present in the cell, the Lambda Red system performs homologous recombination. If this process is unsuccessful, the Cas9-sgRNA complex will cause a double-strand break and will cause cell death (3). This is employed as a counterselection in order to avoid the additional antibiotic as selection marker usage.
+
[[File:T--Vilnius-Lithuania--crisprcas92.png|right|500px|CRISPRCas9]]
 +
 
 +
pCas plasmid is used for Cas9, Lambda Red system expression, and plasmid curing of pTarget. Cas9 - the RNA-guided endonuclease - is expressed constitutively, while the expression of Lambda Red genes (Gam, Exo, Beta) is under the control of arabinose inducible promoter araBp. pTarget plasmid caries constitutively expressed single-guide RNA (sgRNA). This RNA molecule, as and in nature, is composed of 17-20 nt length guide RNA (gRNA) sequence complementary to the targeted DNA adjacent to the protospacer adjacent motif (PAM) present at the 3' end, and the scaffold for the Cas9 nuclease binding to sgRNA and forming the ribonucleoprotein complex (1). Although in nature sgRNA exists as two separate RNA molecules, in laboratory experiments they are usually combined into one single-guide RNA (sgRNA) obviating additional maturation steps. As both pCas and pTarget plasmids are in a cell, Cas9 nuclease and sgRNA are able to form ribonucleoprotein complex, scan DNA for PAM sequences and perform a double-strand break in a part of the DNA which is complementary to the gRNA and adjacent to the PAM sequence - NGG. However, if arabinose has been added to the cell culture and a double-stranded DNA repair template is present in the cell, the Lambda Red system performs homologous recombination. If this process is unsuccessful, the Cas9-sgRNA complex will cause a double-strand break and will cause cell death (2). This is employed as a counterselection in order to avoid the additional antibiotic as selection marker usage.
 +
 
 +
 
 +
 
 +
<b>Table 1.</b> sgRNA collection for <i>E. coli</i> Nissle 1917 genome editing.
 +
 
 +
{| class="wikitable"
 +
|-
 +
|ackA-specific sgRNA
 +
|[https://parts.igem.org/Part:BBa_K3904401 BBa_K3904401]
 +
|-
 +
||pta-specific sgRNA
 +
|[https://parts.igem.org/Part:BBa_K3904402 BBa_K3904402]
 +
|-
 +
|colicin-specific sgRNA
 +
|[https://parts.igem.org/Part:BBa_K3904405 BBa_K3904405]
 +
|-
 +
|nupG-specific sgRNA
 +
|[https://parts.igem.org/Part:BBa_K3904426 BBa_K3904426]
 +
|}
 +
 
 +
 
 +
 
 +
<b>Table 2.</b> Parts collection for genomic insertion into <i>E. Coli</i> Nissle 1917 <i>colicin</i> gene.
 +
 
 +
{| class="wikitable"
 +
|-
 +
|<b>Short description</b>
 +
|<b>Part number</b>
 +
|-
 +
|colicin-specific sgRNA
 +
|[https://parts.igem.org/Part:BBa_K3904405 BBa_K3904405]
 +
|-
 +
|Forward primer to generate a right homology arm of <i>colicin</i> gene
 +
|[https://parts.igem.org/Part:BBa_K3904411 BBa_K3904411]
 +
|-
 +
|Reverse primer to generate right homology arm of <i>colicin</i> gene
 +
|[https://parts.igem.org/Part:BBa_K3904410 BBa_K3904410]
 +
|}
 +
 
 +
==colicin-specific sgRNA importance to our project==
 +
 
 +
Particularly in our project, we needed to insert the metabolic pathway for naringenin production into the genomes of our target probiotic strains. We have chosen two genomic sites for genomic insertions, which would do not harm or negatively affect our probiotic bacteria growth or overall performance - a putative colicin-encoding and <i>nupG</i> genes. We have inserted sfGFP encoding gene under the control of constitutive slpA promoter into these sequences. SfGFP fluorescence was significantly higher in samples with insertion in <i>nupG</i>, however, this case also demonstrated higher fluorescence fluctuations in comparison with putative colicin samples.
 +
 
 +
[[File:T--Vilnius-Lithuania--positioning.png|center|500px|CRISPRCas9]]
 +
 
 +
<b>Fig. 1.</b> Transcriptional activity comparison of GFP transcription from its constructs insertion in <i>nupG</i> or <i>colicin</i> genes.
 +
 
 +
 
 +
 
 +
 
 +
==Genome editing efficiency==
 +
 
 +
GFP insertion into <i>colicin</i> gene with this sgRNA have be  have achieved with 89 % efficiency (fig. 2).
 +
 
 +
[[File:T--Vilnius-Lithuania--GFP-colicin.png|left|500px|CRISPRCas9]]
 +
 
 +
<b>Fig. 2.</b>  GFP insertion into <i>colicin</i> gene results. Here are represented with XbaI digested cPCR products from chosen transformant colonies. If insertion is successful, 1 kbp and 148 bp products are expected. L - GeneRuler 1 bkp Ladder, 1 - negative control (wild type <i>E. coli</i> Nissle 1917),  2 - <i>colicin</i> wild type, 3 - <i>colicin</i>-GFP mutant, 4 - <i>colicin</i>-GFP mutant, 5 - <i>colicin</i>-GFP mutant, 6 - <i>colicin</i>-GFP mutant, 7 - <i>colicin</i>-GFP mutant, 8 - <i>colicin</i>-GFP mutant, 9 - <i>colicin</i>-GFP mutant, 10 - <i>colicin</i>-GFP mutant.
 +
 
 +
 
 +
 
 +
 
  
==tracrRNA==
 
  
tracrRNA and crRNA together guides the nuclease Cas9 to the target of any DNA sequence, known as a protospacer, with a protospacer-adjacent motif (PAM) present at the 3′ end. In this process tracrRNA serves as a scaffold for binding Cas9 endonuclease (3).
 
  
  
Line 34: Line 95:
 
   <li>Doudna, J. A., & Charpentier, E. (2014). The new frontier of genome engineering with CRISPR-Cas9. Science, 346(6213).</li>
 
   <li>Doudna, J. A., & Charpentier, E. (2014). The new frontier of genome engineering with CRISPR-Cas9. Science, 346(6213).</li>
 
   <li>Mali, P., Yang, L., Esvelt, K. M., Aach, J., Guell, M., DiCarlo, J. E., Norville, J. E., & Church, G. M. (2013). RNA-guided human genome engineering via Cas9. Science (New York, N.Y.), 339(6121), 823–826.</li>
 
   <li>Mali, P., Yang, L., Esvelt, K. M., Aach, J., Guell, M., DiCarlo, J. E., Norville, J. E., & Church, G. M. (2013). RNA-guided human genome engineering via Cas9. Science (New York, N.Y.), 339(6121), 823–826.</li>
  <li>Jiang, Y., Chen, B., Duan, C., Sun, B., Yang, J., & Yang, S. (2015). Multigene editing in the Escherichia coli genome via the CRISPR-Cas9 system. Applied and environmental microbiology, 81(7), 2506-2514.</li>
 
  <li></li>
 
  <li></li>
 
 
</ol>   
 
</ol>   
  
 
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Latest revision as of 01:35, 22 October 2021


colicin-specific sgRNA


Introduction

AmeBye

Vilnius-Lithuania iGEM 2021 project AmeByelooks at amebiasis holistically and comprehensively, therefore target E. histolytica from several angles: prevention and diagnostics. Our team's preventive solution consists of probiotics engineered to produce naringenin - an antiprotozoal compound. Two strains of genetically modified microorganisms were chosen as the main chassis - world-renowned Lactobacillus casei BL23 (Lactobacillus paracasei) and Escherichia coli Nissle 1917. Furthermore, the team made specific gene deletions to enhance naringenin production and adapted a novel toxin-antitoxin system to prevent GMO spreads into the environment. The diagnostic part includes a rapid, point of care, user-friendly diagnostic test identifying extraintestinal amebiasis. The main components of this test are aptamers specific to the E. histolytica secreted proteins. These single-stranded DNA sequences fold into tertiary structures for particular fit with target proteins.

Usage and Biology

CRISPR-Cas9 is a versatile genome-editing technique. In our approach to editing E. coli Nissle 1917 genome, we have used two plasmid based system enabling to combine of Lambda Red recombination and CRISPR-Cas9 as counterselection tools encoded in pCas and pTarget.

Mechanism of genome editing

CRISPRCas9

pCas plasmid is used for Cas9, Lambda Red system expression, and plasmid curing of pTarget. Cas9 - the RNA-guided endonuclease - is expressed constitutively, while the expression of Lambda Red genes (Gam, Exo, Beta) is under the control of arabinose inducible promoter araBp. pTarget plasmid caries constitutively expressed single-guide RNA (sgRNA). This RNA molecule, as and in nature, is composed of 17-20 nt length guide RNA (gRNA) sequence complementary to the targeted DNA adjacent to the protospacer adjacent motif (PAM) present at the 3' end, and the scaffold for the Cas9 nuclease binding to sgRNA and forming the ribonucleoprotein complex (1). Although in nature sgRNA exists as two separate RNA molecules, in laboratory experiments they are usually combined into one single-guide RNA (sgRNA) obviating additional maturation steps. As both pCas and pTarget plasmids are in a cell, Cas9 nuclease and sgRNA are able to form ribonucleoprotein complex, scan DNA for PAM sequences and perform a double-strand break in a part of the DNA which is complementary to the gRNA and adjacent to the PAM sequence - NGG. However, if arabinose has been added to the cell culture and a double-stranded DNA repair template is present in the cell, the Lambda Red system performs homologous recombination. If this process is unsuccessful, the Cas9-sgRNA complex will cause a double-strand break and will cause cell death (2). This is employed as a counterselection in order to avoid the additional antibiotic as selection marker usage.


Table 1. sgRNA collection for E. coli Nissle 1917 genome editing.

ackA-specific sgRNA BBa_K3904401
pta-specific sgRNA BBa_K3904402
colicin-specific sgRNA BBa_K3904405
nupG-specific sgRNA BBa_K3904426


Table 2. Parts collection for genomic insertion into E. Coli Nissle 1917 colicin gene.

Short description Part number
colicin-specific sgRNA BBa_K3904405
Forward primer to generate a right homology arm of colicin gene BBa_K3904411
Reverse primer to generate right homology arm of colicin gene BBa_K3904410

colicin-specific sgRNA importance to our project

Particularly in our project, we needed to insert the metabolic pathway for naringenin production into the genomes of our target probiotic strains. We have chosen two genomic sites for genomic insertions, which would do not harm or negatively affect our probiotic bacteria growth or overall performance - a putative colicin-encoding and nupG genes. We have inserted sfGFP encoding gene under the control of constitutive slpA promoter into these sequences. SfGFP fluorescence was significantly higher in samples with insertion in nupG, however, this case also demonstrated higher fluorescence fluctuations in comparison with putative colicin samples.

CRISPRCas9

Fig. 1. Transcriptional activity comparison of GFP transcription from its constructs insertion in nupG or colicin genes.



Genome editing efficiency

GFP insertion into colicin gene with this sgRNA have be have achieved with 89 % efficiency (fig. 2).

CRISPRCas9

Fig. 2. GFP insertion into colicin gene results. Here are represented with XbaI digested cPCR products from chosen transformant colonies. If insertion is successful, 1 kbp and 148 bp products are expected. L - GeneRuler 1 bkp Ladder, 1 - negative control (wild type E. coli Nissle 1917), 2 - colicin wild type, 3 - colicin-GFP mutant, 4 - colicin-GFP mutant, 5 - colicin-GFP mutant, 6 - colicin-GFP mutant, 7 - colicin-GFP mutant, 8 - colicin-GFP mutant, 9 - colicin-GFP mutant, 10 - colicin-GFP mutant.





Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]


References

  1. Doudna, J. A., & Charpentier, E. (2014). The new frontier of genome engineering with CRISPR-Cas9. Science, 346(6213).
  2. Mali, P., Yang, L., Esvelt, K. M., Aach, J., Guell, M., DiCarlo, J. E., Norville, J. E., & Church, G. M. (2013). RNA-guided human genome engineering via Cas9. Science (New York, N.Y.), 339(6121), 823–826.