Difference between revisions of "Part:BBa K1442100"
 
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<partinfo>BBa_K1442100 short</partinfo>
 
<partinfo>BBa_K1442100 short</partinfo>
  
RNA Dependent RNA Polymerase (RdRp)  
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<b>RNA Dependent RNA Polymerase (RdRp)</b>
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== Background ==
  
Background
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<p>RNA dependent RNA polymerase (RdRp) is an enzyme which catalyses the replication of RNA from an RNA template. An essential protein encoded within viruses that lack a DNA phase and replicate using negative sense RNA. The submitted RdRp part derives from the Hepatitis C virus con1 strain, RdRp is also referred to as non-structural protein 5B (NS5B). Part sequence was derived from Lohmann et al., 1997, with the authors achieving full expression and activity of RdRp in a baculovirus expression system. Membrane association of RdRp is essential for replication of HCV subgenomic regions, with the C-terminal tail containing 21 amino acids which confer high hydrophobicity and mediate insertion into the membrane (Moradpour et., 2004).  
 
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The C-terminal tail preceding the C-terminal hydrophobic insertion sequence interacts with structural elements including the β-hairpin loop of NS5b (Leveque et al., 2003). The β-hairpin loop inserts into the active site, believed to position the 3’ terminius of HCV viral RNA to initiate RNA synthesis (Hong et al., 2001). RdRp initiates RNA synthesis with nucleotide transfer activity found within the palm motif (Figure 1a & b), with several amino acid residues implicated in nucleotide triphosphate contact (Bressanelli et al., 2002).  RdRp requires 5’ and 3’ untranslated regions (UTRs) found within the HCV genome to direct RNA synthesis.  The UTRs form ordered RNA structures and are evolutionary conserved. </p>
RNA dependent RNA polymerase (RdRp) is an enzyme which catalyses the replication of RNA from an RNA template. An essential protein encoded within viruses that lack a DNA phase and replicate using negative sense RNA. The submitted RdRp part derives from the Hepatitis C virus con1 strain, RdRp is also referred to as non-structural protein 5B (NS5B). Part sequence was derived from Lohmann et al., 1997, with the authors achieving full expression and activity of RdRp in a baculovirus expression system. Membrane association of RdRp is essential for replication of HCV subgenomic regions, with the C-terminal tail containing 21 amino acids which confer high hydrophobicity and mediate insertion into the membrane (Moradpour et., 2004).  
+
The C-terminal tail preceding the C-terminal hydrophobic insertion sequence interacts with structural elements including the β-hairpin loop of NS5b (Leveque et al., 2003). The β-hairpin loop inserts into the active site, believed to position the 3’ terminius of HCV viral RNA to initiate RNA synthesis (Hong et al., 2001). RdRp initiates RNA synthesis with nucleotide transfer activity found within the palm motif (Figure 1a & b), with several amino acid residues implicated in nucleotide triphosphate contact (Bressanelli et al., 2002).  RdRp requires 5’ and 3’ untranslated regions (UTRs) found within the HCV genome to direct RNA synthesis.  The UTRs form ordered RNA structures and are evolutionary conserved.  
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https://static.igem.org/mediawiki/2014/c/c5/Hcv.png
 
https://static.igem.org/mediawiki/2014/c/c5/Hcv.png
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'''Figure 1. Ribbon diagram of HCV RNA polymerase (NS5B)'''. (left) Molecular surface rendering of NS5B. Images depict the palm, thumb and fingers domain of the RNA dependent RNA polymerase. Taken from (O’Farrell et al., 2003) http://www.ncbi.nlm.nih.gov/pubmed/12589751
 
'''Figure 1. Ribbon diagram of HCV RNA polymerase (NS5B)'''. (left) Molecular surface rendering of NS5B. Images depict the palm, thumb and fingers domain of the RNA dependent RNA polymerase. Taken from (O’Farrell et al., 2003) http://www.ncbi.nlm.nih.gov/pubmed/12589751
  
Design Notes
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== Experimental Design ==
 
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• The 21 amino acid residues have been removed in the part sequence, ensuring cytoplasmic RdRp activity, this ensures no anchoring to the endoplasmic reticulum in human cells (Lai et al., 2004). This modification has no major effect on RdRp activity, which is complimented by previous analysis showing no significant loss of nucleotide polymerization activity (Vo et al., 2004).
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• A single point mutation has been introduced at position 2884, where a guanine has replaced a cytosine. This confers an Arginine to glycine substitution, which increases the number of transformed colonies obtained (Bartenschlager et al., 2001).
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• A PstI restriction site was removed in the part sequence (CTGCAG) and was altered to CTCCAG to allow bio brick compatibility. 
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Experimental Design
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To characterize the RNA dependent RNA polymerase, constructs with 3’ untranslated regions (UTRs) in combination with a Reverse GFP were introduced in E. coli.  The 3’ UTRs comprise previously used DNA sequences that promote RdRp activity. Further information on the 3’ UTRs is below (n.b. only some of the 3’ UTRs listed below have been stably transformed and been used to characterize mRdRp and RdRp activity.  
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<p>To characterize the RNA dependent RNA polymerase, constructs with 3’ untranslated regions (UTRs) in combination with a Reverse GFP were introduced in E. coli.  The 3’ UTRs comprise previously used DNA sequences that promote RdRp activity. Further information on the 3’ UTRs is below (n.b. only some of the 3’ UTRs listed below have been stably transformed and been used to characterize mRdRp and RdRp activity. </p>
  
  
B2(−)26G 5’ GGATTGAACCTCGTTCCGTGGTTTACG 3’
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<p><b>B2(−)26G</b></p> 5’ GGATTGAACCTCGTTCCGTGGTTTACG 3’
  
C2(−)29G 5’ GGTTGAACCGTACGCCTTTGTAAATAAACG 3’
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<p><b>C2(−)29G</b></p> 5’ GGTTGAACCGTACGCCTTTGTAAATAAACG 3’
  
SLC+8 5’ GGACGCATGGGCTTGCATAGCAAGTCTAGATATGCGTCCAGAGACCA 3’
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<p><b>SLC+8</b></p> 5’ GGACGCATGGGCTTGCATAGCAAGTCTAGATATGCGTCCAGAGACCA 3’
  
SLdel+8 5’ GGCTTGCATAGCAAGTCTAGATATGCGTCCAGAGACCA 3’
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<p><b>SLdel+8</b></p> 5’ GGCTTGCATAGCAAGTCTAGATATGCGTCCAGAGACCA 3’
  
SLD3 5’ GGGCTTGCATAGCAAGTCTGAGACC 3’
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<p><b>SLD3</b></p> 5’ GGGCTTGCATAGCAAGTCTGAGACC 3’
  
Mutant RNA dependent RNA polymerase (mRdRp in Figure 4) was also characterized in tandem with the normal RNA dependent RNA polymerase (RdRp in Figure 3). Mutant RNA dependent RNA polymerase is edited, with the removal of a Bgal1 restriction site in the sequence, as this is not biobrick compatible it has not been uploaded to the registry. Normal RNA dependent RNA polymerase is biobrick compatible.  
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<p>Mutant RNA dependent RNA polymerase (mRdRp in Figure 4) <html><body><a href="https://parts.igem.org/Part:BBa_K1442101">Part BBa_K1442102</a></body></html> was also characterized in tandem with the normal RNA dependent RNA polymerase (RdRp in Figure 3). Mutant RNA dependent RNA polymerase is edited, with the removal of a Bgal1 restriction site in the sequence, as this is not biobrick compatible it has not been uploaded to the registry. Normal RNA dependent RNA polymerase is not biobrick compatible but has undergone site directed mutagenesis to remove the PstI site in a silent substitution mutation.</p>
  
 
https://static.igem.org/mediawiki/2014/7/7a/Hcvfig3.png
 
https://static.igem.org/mediawiki/2014/7/7a/Hcvfig3.png
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'''Figure 5. 3’ UTR and Reverse GFP general construct depiction.''' Plasmid containing reverse GFP and 3’ UTR is depicted below. This was used to characterize RdRp and mRdRp activity in E. coli. 3’ UTRs were interchangeable and are referred to as S3, R5 and C2/HP. 3’ UTRs and Reverse GFP are biobrick compatible. For clarity, biobrick prefix and suffix sequences not shown.  
 
'''Figure 5. 3’ UTR and Reverse GFP general construct depiction.''' Plasmid containing reverse GFP and 3’ UTR is depicted below. This was used to characterize RdRp and mRdRp activity in E. coli. 3’ UTRs were interchangeable and are referred to as S3, R5 and C2/HP. 3’ UTRs and Reverse GFP are biobrick compatible. For clarity, biobrick prefix and suffix sequences not shown.  
  
To characterize RdRp and mRdRp activity, co-transformation of the two plasmids with the relevant constructs (Figures 4 & 5) was performed. Table 1 summarizes the experiments and relevant 3’ UTRs tested. Data was obtained using the Tecan micro plate reader
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===Improve===
 
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At the C-terminus of the original NS5B, the 2019 Nanjing_NFLS team added a nuclear localization sequence with a repeat sequence to ensure that the protein can enter the nucleus efficiently so that it can be further designed in transcriptional regulation.<br/>
 
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https://static.igem.org/mediawiki/2014/0/0d/Graph1hcv.png
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Figure 6. Characterization of mRdRp and RdRp activity with S3, R5 and C2/HP 3’ UTRs. Data was collected at different time points using Tecan Microplate reader. Controls also present: (IPTG + RBS + GFP) and NEB only.
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Table 1. RNA dependent RNA polymerase activity following induction at 0.2 and 0.4 OD, relative to control wells (not induced at 0.2 and 0.4 OD). Error bars indicate standard error.
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https://static.igem.org/mediawiki/2014/d/d4/Hcv_table_5.png
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Horizontal axis depicts various different points (1-9:  due to the nature of the analysis time in seconds is not displayed). RdRp induction at 0.2 and 0.4 OD at points 1-3 indicates initial activity and relative increase in fluorescence output. Initial RdRp activity then decays following induction, with decrease in fluorescence activity at both OD 0.2 and 0.4. Conclusively, results suggest initial induction of RdRp activity causes a relative increase in fluorescence with a stabilization/decrease thereafter.
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https://static.igem.org/mediawiki/2014/6/64/Rdrp_linear_graph.png
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Figure 7. RNA dependent RNA polymerase activity following induction at 0.2 and 0.4 OD, relative to control wells (not induced at 0.2 and 0.4 OD).
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https://static.igem.org/mediawiki/2014/3/38/Rdrpgraph3.png
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Figure 8. RNA dependent RNA polymerase activity following induction at 0.2 and 0.4 OD. Rates were extracted by linear regression and is displayed. Error bars indicate standard error of the mean. Rdrp Ni: Non induced, Rdrp I: Induced, mRdRp follows the same conventions.  
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https://2019.igem.org/wiki/images/0/0e/T--Nanjing_NFLS--Parts_BBa_K2989008.jpg
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A: NS5B (no NLS)<br/>
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B: DNLS-NS5B (after adding NLS)<br/>
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We transfected NS5B and DNLS-NS5B with NLS (nuclear localization sequence) into HepG2 cells respectively and detected them by immunofluorescence. The results are shown in figures. NLS-free NS5B was mainly expressed in the cytoplasm, while the NS5B protein with NLS (nuclear localization sequence) was obviously colocalized with the nucleus, which proved that NS5B entered the nucleus successfully.
  
 
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Latest revision as of 14:46, 21 October 2019

RdRP

RNA Dependent RNA Polymerase (RdRp)

Background

RNA dependent RNA polymerase (RdRp) is an enzyme which catalyses the replication of RNA from an RNA template. An essential protein encoded within viruses that lack a DNA phase and replicate using negative sense RNA. The submitted RdRp part derives from the Hepatitis C virus con1 strain, RdRp is also referred to as non-structural protein 5B (NS5B). Part sequence was derived from Lohmann et al., 1997, with the authors achieving full expression and activity of RdRp in a baculovirus expression system. Membrane association of RdRp is essential for replication of HCV subgenomic regions, with the C-terminal tail containing 21 amino acids which confer high hydrophobicity and mediate insertion into the membrane (Moradpour et., 2004). The C-terminal tail preceding the C-terminal hydrophobic insertion sequence interacts with structural elements including the β-hairpin loop of NS5b (Leveque et al., 2003). The β-hairpin loop inserts into the active site, believed to position the 3’ terminius of HCV viral RNA to initiate RNA synthesis (Hong et al., 2001). RdRp initiates RNA synthesis with nucleotide transfer activity found within the palm motif (Figure 1a & b), with several amino acid residues implicated in nucleotide triphosphate contact (Bressanelli et al., 2002). RdRp requires 5’ and 3’ untranslated regions (UTRs) found within the HCV genome to direct RNA synthesis. The UTRs form ordered RNA structures and are evolutionary conserved.

Hcv.png

Figure 1. Ribbon diagram of HCV RNA polymerase (NS5B). (left) Molecular surface rendering of NS5B. Images depict the palm, thumb and fingers domain of the RNA dependent RNA polymerase. Taken from (O’Farrell et al., 2003) http://www.ncbi.nlm.nih.gov/pubmed/12589751

Experimental Design

To characterize the RNA dependent RNA polymerase, constructs with 3’ untranslated regions (UTRs) in combination with a Reverse GFP were introduced in E. coli. The 3’ UTRs comprise previously used DNA sequences that promote RdRp activity. Further information on the 3’ UTRs is below (n.b. only some of the 3’ UTRs listed below have been stably transformed and been used to characterize mRdRp and RdRp activity.


B2(−)26G

5’ GGATTGAACCTCGTTCCGTGGTTTACG 3’

C2(−)29G

5’ GGTTGAACCGTACGCCTTTGTAAATAAACG 3’

SLC+8

5’ GGACGCATGGGCTTGCATAGCAAGTCTAGATATGCGTCCAGAGACCA 3’

SLdel+8

5’ GGCTTGCATAGCAAGTCTAGATATGCGTCCAGAGACCA 3’

SLD3

5’ GGGCTTGCATAGCAAGTCTGAGACC 3’

Mutant RNA dependent RNA polymerase (mRdRp in Figure 4) Part BBa_K1442102 was also characterized in tandem with the normal RNA dependent RNA polymerase (RdRp in Figure 3). Mutant RNA dependent RNA polymerase is edited, with the removal of a Bgal1 restriction site in the sequence, as this is not biobrick compatible it has not been uploaded to the registry. Normal RNA dependent RNA polymerase is not biobrick compatible but has undergone site directed mutagenesis to remove the PstI site in a silent substitution mutation.

Hcvfig3.png

Figure 3. Construct depiction. Plasmid containing RNA dependent RNA polymerase (RdRp), driven by a T3 promoter in combination with an ampicillin resistance gene for selection of transformant colonies. For clarity, biobrick prefix and suffix sequences not shown.

Hcvfig4.png

Figure 4. Construct depiction. Plasmid containing mutant RNA dependent RNA polymerase (RdRp), driven by a T3 promoter in combination with an ampicillin resistance gene for selection of transformant colonies. Mutant RdRp is not biobrick compatible, but has been included as an additional control.

Hcvfig5.png

Figure 5. 3’ UTR and Reverse GFP general construct depiction. Plasmid containing reverse GFP and 3’ UTR is depicted below. This was used to characterize RdRp and mRdRp activity in E. coli. 3’ UTRs were interchangeable and are referred to as S3, R5 and C2/HP. 3’ UTRs and Reverse GFP are biobrick compatible. For clarity, biobrick prefix and suffix sequences not shown.

Improve

At the C-terminus of the original NS5B, the 2019 Nanjing_NFLS team added a nuclear localization sequence with a repeat sequence to ensure that the protein can enter the nucleus efficiently so that it can be further designed in transcriptional regulation.

T--Nanjing_NFLS--Parts_BBa_K2989008.jpg A: NS5B (no NLS)
B: DNLS-NS5B (after adding NLS)
We transfected NS5B and DNLS-NS5B with NLS (nuclear localization sequence) into HepG2 cells respectively and detected them by immunofluorescence. The results are shown in figures. NLS-free NS5B was mainly expressed in the cytoplasm, while the NS5B protein with NLS (nuclear localization sequence) was obviously colocalized with the nucleus, which proved that NS5B entered the nucleus successfully.

Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    INCOMPATIBLE WITH RFC[21]
    Illegal BglII site found at 492
    Illegal BglII site found at 1340
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    INCOMPATIBLE WITH RFC[1000]
    Illegal BsaI site found at 537