Difference between revisions of "Part:BBa K404157"
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__NOTOC__ | __NOTOC__ | ||
− | <partinfo>BBa_K404157 short</partinfo> | + | <partinfo>BBa_K404157 short</partinfo><br> |
+ | {| style="color:black" cellpadding="6" cellspacing="1" border="2" align="left" | ||
+ | ! colspan="2" style="background:#66bbff;"|[https://parts.igem.org/Part:BBa_K404157 pCMV_Z-EGFR-1907_Long-Linker_[AAV2]-VP23_(ViralBrick-587KO-Empty)] | ||
+ | |- | ||
+ | |'''BioBrick Nr.''' | ||
+ | |[https://parts.igem.org/Part:BBa_K404157 BBa_K404157] | ||
+ | |- | ||
+ | |'''RFC standard''' | ||
+ | |[https://parts.igem.org/Help:Assembly_standard_10 RFC 10] | ||
+ | |- | ||
+ | |'''Requirement''' | ||
+ | |pSB1C3<br> | ||
+ | |- | ||
+ | |'''Source''' | ||
+ | | | ||
+ | |- | ||
+ | |'''Submitted by''' | ||
+ | |[http://2010.igem.org/Team:Freiburg_Bioware FreiGEM 2010] | ||
+ | |} | ||
+ | <br> | ||
+ | <br> | ||
+ | <br> | ||
+ | <br> | ||
+ | <br> | ||
+ | <br> | ||
+ | <br> | ||
+ | <br><br><br><br><br><br><br> | ||
+ | |||
+ | |||
+ | |||
+ | This part is used for cotranfection with parts containing VP1up (BBa_K404164-BBa_K404166)<br> | ||
<h2>Affibody Z-EGFR-1907</h2> (BBa_K404302)<br> | <h2>Affibody Z-EGFR-1907</h2> (BBa_K404302)<br> | ||
Line 8: | Line 38: | ||
<h2>CMV</h2> | <h2>CMV</h2> | ||
CMV promoter is derived from human Cytomegalovirus, which belongs to Herpesvirus group. All family members share the ability to remain in latent stage in the human body. CMV is located upstream of immediate-early gene. However, CMV promoter is an example of widely used promoters and is present in mammalian expression vectors. The advantage of CMV is the high-level constitutive expression in mostly all human tissues [Fitzsimons et al., 2002]. <br> | CMV promoter is derived from human Cytomegalovirus, which belongs to Herpesvirus group. All family members share the ability to remain in latent stage in the human body. CMV is located upstream of immediate-early gene. However, CMV promoter is an example of widely used promoters and is present in mammalian expression vectors. The advantage of CMV is the high-level constitutive expression in mostly all human tissues [Fitzsimons et al., 2002]. <br> | ||
− | <h2>Long Linker ( Gly-Gly-Ser-Gly) | + | <h2>Long Linker ( Gly-Gly-Ser-Gly)x3</h2> (BBa_K243006)<br> |
This part is a linker, it can be used to connect two parts and add additional space between them. That can be necessary to avoid interactions between these parts.<br> | This part is a linker, it can be used to connect two parts and add additional space between them. That can be necessary to avoid interactions between these parts.<br> | ||
<h2>Capsid</h2> (BBa_K404006)<br> | <h2>Capsid</h2> (BBa_K404006)<br> | ||
− | The AAV capsid consists of 60 capsid protein subunits. The three cap proteins VP1, VP2, and VP3 are encoded in an overlapping reading frame. Arranged in a stoichiometric ratio of 1:1:10, they form an icosahedral symmetry. The mRNA encoding for the cap proteins is transcribed from p40 and alternative spliced to minor and major products. Alternative splicing and translation initiation of VP2 at a nonconventional ACG initiation codon promote the expression of VP1, VP2 and VP3. The VP proteins share a common C terminus and stop codon, but begin with a different start codon. The N | + | The AAV capsid consists of 60 capsid protein subunits. The three cap proteins VP1, VP2, and VP3 are encoded in an overlapping reading frame. Arranged in a stoichiometric ratio of 1:1:10, they form an icosahedral symmetry. The mRNA encoding for the cap proteins is transcribed from p40 and alternative spliced to minor and major products. Alternative splicing and translation initiation of VP2 at a nonconventional ACG initiation codon promote the expression of VP1, VP2 and VP3. The VP proteins share a common C terminus and stop codon, but begin with a different start codon. The N-terminus of VP1 plays important role in infection and contains a motif highly homologous to a phospholipase A2 (PLA2) domain and nuclear localization signals (BR)(+). VP2 contains basic regions, too. |
<html><center><img src="https://static.igem.org/mediawiki/parts/a/a7/Freiburg10_Cap_proteins_VP1_2%263.png" width="600" height="auto"/></center></html><br> | <html><center><img src="https://static.igem.org/mediawiki/parts/a/a7/Freiburg10_Cap_proteins_VP1_2%263.png" width="600" height="auto"/></center></html><br> | ||
<h2>ViralBrick 587-KO empty</h2> | <h2>ViralBrick 587-KO empty</h2> | ||
The primary receptor of AAV-2 is the heparan sulfate proteoglycan (HSPG) receptor (Perabo et al. 2006). Its binding motif consists of five amino-acids located on the capsid surface: R484/R487, K532, R585/587. (Trepel et al. 2009). The positively charged arginine residues interact with the HSPGs' negatively charged acid residues. Opie et al. have shown that two point mutations (R585A and R588A) are sufficient to eliminate the heparin binding affinity in AAV2. (Opie et al. 2003). This ViralBrick has been created to introduce this knockout into other constructs. The biobricks with containing this knockout are annotated with „HSPG-ko“.<br> | The primary receptor of AAV-2 is the heparan sulfate proteoglycan (HSPG) receptor (Perabo et al. 2006). Its binding motif consists of five amino-acids located on the capsid surface: R484/R487, K532, R585/587. (Trepel et al. 2009). The positively charged arginine residues interact with the HSPGs' negatively charged acid residues. Opie et al. have shown that two point mutations (R585A and R588A) are sufficient to eliminate the heparin binding affinity in AAV2. (Opie et al. 2003). This ViralBrick has been created to introduce this knockout into other constructs. The biobricks with containing this knockout are annotated with „HSPG-ko“.<br> | ||
+ | <br/> | ||
+ | <h2>Characterization</h2> | ||
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+ | <h4><span lang="EN-US">Transduction Efficacy by Flow Cytometry</span></h4> | ||
+ | <p class="MsoNormal" style="text-align: justify;"><span lang="EN-US">For | ||
+ | determination of transduction efficacy flow cytometry analysis was | ||
+ | conducted. 250.000 | ||
+ | AAV-293 cells were transfected with 1 µg total DNA. 72 hours post | ||
+ | transfection | ||
+ | viruses were harvested and two different cell lines, HT1080 and A431, | ||
+ | were | ||
+ | transduced with 1 mL virus stock. By encapsulating mVenus coding | ||
+ | sequence, the | ||
+ | amount of transduced cells could be determined via flow cytometry.</span></p> | ||
+ | <p class="MsoNormal" style="text-align: center;"><img | ||
+ | src="https://static.igem.org/mediawiki/parts/7/77/Freiburg10_FACS3.PNG" | ||
+ | style=""></p> | ||
+ | <p class="MsoNormal" style="text-align: justify; line-height: normal;"><b><span | ||
+ | style="font-size: 10pt;" lang="EN-US">Figure 1: Flow cytometry.</span></b><span | ||
+ | style="font-size: 10pt;" lang="EN-US"> Investigating transduction | ||
+ | efficiency with | ||
+ | HT1080 and A431 cells by detecting mVenus expression from <b>Z<sub>EGFR:1907</sub>_LongLinker_VP2/3</b> | ||
+ | virus particles (Transfection ratio: 50:50 in respect to Rep/Cap | ||
+ | plasmid). A) Gating | ||
+ | non transduced cells (control); subcellular debris and cellular | ||
+ | aggregates can | ||
+ | be distinguished from single cells by size, estimated via forward | ||
+ | scatter (FS | ||
+ | Lin) and granularity, estimated via side scatter (SS Lin). B) <b>:</b> | ||
+ | Non | ||
+ | transduced cells plotted against mVenus fluorescence (Analytical gate | ||
+ | was set | ||
+ | such that 1% or fewer of negative control cells fell within the | ||
+ | positive region | ||
+ | (R6). C) Gating transduced cells. D) Transduced cells plotted against | ||
+ | mVenus | ||
+ | fluorescence, R10 comprised transduced, mVenus expressing cells. E) | ||
+ | Overlay of | ||
+ | non transduced (red) and transduced (green) cells plotted against | ||
+ | mVenus | ||
+ | fluorescence.</span></p> | ||
+ | <p class="MsoNormal" style="text-align: justify;"><span lang="EN-US">Figure | ||
+ | 2 | ||
+ | overviews transduction efficacy of all ratio combinations.</span></p> | ||
+ | <br> | ||
+ | <p class="MsoNormal" style="text-align: center;"><img alt="HT1080" | ||
+ | src="https://static.igem.org/mediawiki/parts/c/cd/Freiburg10_FACSHT1080.png" | ||
+ | style="width: 700px; height: 525px;"><img alt="A431" | ||
+ | src="https://static.igem.org/mediawiki/parts/c/c7/Freiburg10_FACSA431.png" | ||
+ | style="width: 700px; height: 525px;"></p> | ||
+ | <p class="MsoNormal" style="text-align: center;"></p> | ||
+ | <p class="MsoNormal" style="line-height: normal;"><b><span | ||
+ | style="font-size: 10pt;" lang="EN-US">Figure 2: Flow cytometry analysis</span></b><span | ||
+ | style="font-size: 10pt;" lang="EN-US">. Transduced and therefore | ||
+ | mVenus positive | ||
+ | HT1080 and A431 cells, infected with virus particles consisting of | ||
+ | different ratios | ||
+ | of VP2 fusion construct in respect to Rep/Cap plasmid. </span></p> | ||
+ | <p class="MsoNormal" style="line-height: normal;"><span lang="EN-US"> </span></p> | ||
+ | <p class="MsoNormal"><span lang="EN-US">Transduction of HT1080 cells | ||
+ | revealed that | ||
+ | all viral particles remained infectious with efficacies up to 55 %. | ||
+ | This | ||
+ | indicates that larger peptides could be inserted into the AAV2 capsids | ||
+ | without | ||
+ | affecting virus assembly and packaging. A431 cells, which overexpress | ||
+ | EGF | ||
+ | receptor, were generally transduced with reduced efficacy. </span></p> | ||
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<!-- Add more about the biology of this part here | <!-- Add more about the biology of this part here |
Latest revision as of 16:13, 31 October 2010
pCMV_Z-EGFR-1907_Long-Linker_[AAV2]-VP23 (ViralBrick-587KO-Empty)
pCMV_Z-EGFR-1907_Long-Linker_[AAV2-VP23_(ViralBrick-587KO-Empty)] | |
---|---|
BioBrick Nr. | BBa_K404157 |
RFC standard | RFC 10 |
Requirement | pSB1C3 |
Source | |
Submitted by | [http://2010.igem.org/Team:Freiburg_Bioware FreiGEM 2010] |
This part is used for cotranfection with parts containing VP1up (BBa_K404164-BBa_K404166)
Affibody Z-EGFR-1907
(BBa_K404302)Affibodies are small (6 kDa), soluble high-affinity proteins. They are derived from the IgG-binding B domain of the Staphylococcal protein A, which was engineered to specifically bind to certain peptides or proteins. This so-called Z domain consists of an antiparallel three-helix bundle and is advantageous due to its proteolytic and thermodynamic stability, its good folding properties and the ease of production via recombinant bacteria (Nord et al., 1997). Affibodies can be used for example for tumor targeting (Wikman et al., 2004) and diagnostic imaging applications (Orlova et al., 2006; Orlova et al., 2007). The ZEGFR:1907 Affibody was engineered to specifically bind the EGF receptor with an affinity determined to be KD = 2.8 nM (Friedman et al., 2008).
The EGF receptor is overexpressed in certain types of tumors, e.g. in breast (Walker & Dearing, 1999), lung (Hirsch et al., 2003) and bladder (Colquhoun & Mellon, 2002) carcinomas, and is therefore a suitable target for cancer imaging or therapeutic applications. Because of their good tumor uptake, and their property to become internalized into the target cells with an efficiency of 19 – 24% within one hour – compared to 45% of the natural ligand EGF - the ZEGFR:1907 Affibody was chosen for therapeutic applications by the Freiburg iGEM Team 2010 (Friedman et al., 2008; Göstring et al., 2010).
CMV
CMV promoter is derived from human Cytomegalovirus, which belongs to Herpesvirus group. All family members share the ability to remain in latent stage in the human body. CMV is located upstream of immediate-early gene. However, CMV promoter is an example of widely used promoters and is present in mammalian expression vectors. The advantage of CMV is the high-level constitutive expression in mostly all human tissues [Fitzsimons et al., 2002].
Long Linker ( Gly-Gly-Ser-Gly)x3
(BBa_K243006)This part is a linker, it can be used to connect two parts and add additional space between them. That can be necessary to avoid interactions between these parts.
Capsid
(BBa_K404006)The AAV capsid consists of 60 capsid protein subunits. The three cap proteins VP1, VP2, and VP3 are encoded in an overlapping reading frame. Arranged in a stoichiometric ratio of 1:1:10, they form an icosahedral symmetry. The mRNA encoding for the cap proteins is transcribed from p40 and alternative spliced to minor and major products. Alternative splicing and translation initiation of VP2 at a nonconventional ACG initiation codon promote the expression of VP1, VP2 and VP3. The VP proteins share a common C terminus and stop codon, but begin with a different start codon. The N-terminus of VP1 plays important role in infection and contains a motif highly homologous to a phospholipase A2 (PLA2) domain and nuclear localization signals (BR)(+). VP2 contains basic regions, too.
ViralBrick 587-KO empty
The primary receptor of AAV-2 is the heparan sulfate proteoglycan (HSPG) receptor (Perabo et al. 2006). Its binding motif consists of five amino-acids located on the capsid surface: R484/R487, K532, R585/587. (Trepel et al. 2009). The positively charged arginine residues interact with the HSPGs' negatively charged acid residues. Opie et al. have shown that two point mutations (R585A and R588A) are sufficient to eliminate the heparin binding affinity in AAV2. (Opie et al. 2003). This ViralBrick has been created to introduce this knockout into other constructs. The biobricks with containing this knockout are annotated with „HSPG-ko“.
Characterization
Transduction Efficacy by Flow Cytometry
For determination of transduction efficacy flow cytometry analysis was conducted. 250.000 AAV-293 cells were transfected with 1 µg total DNA. 72 hours post transfection viruses were harvested and two different cell lines, HT1080 and A431, were transduced with 1 mL virus stock. By encapsulating mVenus coding sequence, the amount of transduced cells could be determined via flow cytometry.
Figure 1: Flow cytometry. Investigating transduction efficiency with HT1080 and A431 cells by detecting mVenus expression from ZEGFR:1907_LongLinker_VP2/3 virus particles (Transfection ratio: 50:50 in respect to Rep/Cap plasmid). A) Gating non transduced cells (control); subcellular debris and cellular aggregates can be distinguished from single cells by size, estimated via forward scatter (FS Lin) and granularity, estimated via side scatter (SS Lin). B) : Non transduced cells plotted against mVenus fluorescence (Analytical gate was set such that 1% or fewer of negative control cells fell within the positive region (R6). C) Gating transduced cells. D) Transduced cells plotted against mVenus fluorescence, R10 comprised transduced, mVenus expressing cells. E) Overlay of non transduced (red) and transduced (green) cells plotted against mVenus fluorescence.
Figure 2 overviews transduction efficacy of all ratio combinations.
Figure 2: Flow cytometry analysis. Transduced and therefore mVenus positive HT1080 and A431 cells, infected with virus particles consisting of different ratios of VP2 fusion construct in respect to Rep/Cap plasmid.
Transduction of HT1080 cells revealed that all viral particles remained infectious with efficacies up to 55 %. This indicates that larger peptides could be inserted into the AAV2 capsids without affecting virus assembly and packaging. A431 cells, which overexpress EGF receptor, were generally transduced with reduced efficacy.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21INCOMPATIBLE WITH RFC[21]Illegal BamHI site found at 2207
- 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal NgoMIV site found at 665
- 1000INCOMPATIBLE WITH RFC[1000]Illegal BsaI site found at 2733
Illegal SapI site found at 1644
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