Difference between revisions of "Part:BBa K3120018"
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| − | + | This part is the homologous recombination plasmid of E-Cadherin. Using CRISPR/cas9 technology, homologous recombination can occur between the left arm and right arm of E-Cadherin and the corresponding fragments on the genome, so as to realize the insertion of tdTomato before the termination codon of E-Cadherin gene of homo sapiens WA09(human embryonic stem cell line).<b>(Fig.1A ,Fig.1B)</b> | |
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| − | [[Image:T--BM-AMU--part7.jpg|center|thumb|500px|'''Fig1 . | + | After co-transfection with plasmid pBluescriptll SK-Ecadherin-tdTomato into WA09 cells, monoclonal cloning, we identified the correct insertion of tdTomato at the genome level and mRNA level(cDNA).<b>(Fig1C)</b>The correct subcellular localiza-tion of ECAD and tdTomato (Fusion expression)was observed by confocal micro-scope.<b>(Fig.1D)</b> |
| − | <b>( A)</b>Schematic of plasmid pBluescriptll SK-Ecadherin-tdTomato. <b>(B)</b>Schematic of plasmid PX330. <b>(C)</b>The correct insertion of tdTomato at the genome level and mRNA level(cDNA) by PCR.<b>(D)</b>The correct subcellular localization of ECAD and tdTomato (Fusion expression)was observed by confocal microscope. | + | [[Image:T--BM-AMU--part7.jpg|center|thumb|500px|'''Fig1 . <b>( A)</b>Schematic of plasmid pBluescriptll SK-Ecadherin-tdTomato. <b>(B)</b>Schematic of plasmid PX330. <b>(C)</b>The correct insertion of tdTomato at the genome level and mRNA level(cDNA) by PCR.<b>(D)</b>The correct subcellular localization of ECAD and tdTomato (Fusion expression)was observed by confocal microscope. |
''']] | ''']] | ||
Revision as of 01:22, 20 October 2019
E-cad LA+Glycine linker+tdTomato+E-cad RA
This part is the homologous recombination plasmid of E-Cadherin. Using crisper CAS9 technology, homologous recombination can occur between the left arm and right arm of E-Cadherin and the corresponding fragments on the genome, so as to realize the insertion of tdTomato before the termination codon of E-Cadherin gene of homo sapiens H9(human embryonic stem cell line).
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21INCOMPATIBLE WITH RFC[21]Illegal XhoI site found at 3994
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000INCOMPATIBLE WITH RFC[1000]Illegal BsaI site found at 333
Illegal BsaI site found at 782
Illegal BsaI site found at 4472
Illegal BsaI site found at 4635
Illegal BsaI site found at 4658
Illegal BsaI.rc site found at 1647
This part is the homologous recombination plasmid of E-Cadherin. Using CRISPR/cas9 technology, homologous recombination can occur between the left arm and right arm of E-Cadherin and the corresponding fragments on the genome, so as to realize the insertion of tdTomato before the termination codon of E-Cadherin gene of homo sapiens WA09(human embryonic stem cell line).(Fig.1A ,Fig.1B)
After co-transfection with plasmid pBluescriptll SK-Ecadherin-tdTomato into WA09 cells, monoclonal cloning, we identified the correct insertion of tdTomato at the genome level and mRNA level(cDNA).(Fig1C)The correct subcellular localiza-tion of ECAD and tdTomato (Fusion expression)was observed by confocal micro-scope.(Fig.1D)
