Difference between revisions of "Part:BBa K243036"
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[[Image:Freiburg09_Fok_80mer.jpg|250x400px]]<br> | [[Image:Freiburg09_Fok_80mer.jpg|250x400px]]<br> | ||
Gellanes:1.Marker(1kb ladder mix)2.Cell extract+sample1 3.Cell extract+sample2 4.control w/o cell extract.<br> | Gellanes:1.Marker(1kb ladder mix)2.Cell extract+sample1 3.Cell extract+sample2 4.control w/o cell extract.<br> | ||
− | [https://static.igem.org/mediawiki/parts/a/ac/Fok_in_vitro_80mer_cutting_assay.pdf Method] | + | [https://static.igem.org/mediawiki/parts/a/ac/Fok_in_vitro_80mer_cutting_assay.pdf Method]<br> |
− | '''Detection of the Cy3<br>''' | + | The pictures shows our gel one left excited by wavelength of 353 nm and on right side filtered with the cutoff filter of 580nm. The first lane shows the marker only visible on right gel picture, the second and third lane show the products of the cutting event made by our universal endonuclease. The comparison with fourth lane shows that the origin oligonucleotides are cut.In the fourth lane there were only the oligonucleotides loaded. |
+ | '''Detection of the Cy3<br>'''<br> | ||
To excite the Cy3-tagged nucleotides a laser with a wavelength of 353 nm was used. To cut of the excitation wavelength in the pictures a cutoff filter of 580nm was used. In another approach the SteREO Lumar.V12 from Zeiss was used to excite the Cy3-tagged oligonucleotides. | To excite the Cy3-tagged nucleotides a laser with a wavelength of 353 nm was used. To cut of the excitation wavelength in the pictures a cutoff filter of 580nm was used. In another approach the SteREO Lumar.V12 from Zeiss was used to excite the Cy3-tagged oligonucleotides. | ||
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Revision as of 02:25, 22 October 2009
His-Dig-Split Linker-Fok_a
This combination uses the benefits of a His tag (Polyhistidin tag) for purification. It is also linked with a DigoxigeninA tag (DigA). The Split Linker connects the parts and adds additional space between them to guarantee the independent function of DigA tag and the protein domain Fok_a.
Usage and Biology
This composite part is one part of our universal endonuclease and it needs another composite part like BBa_K243010 to build a functional heterodimer. The DigA tag guides the part to the DNA which is hybridized with a Digoxigenin labeled oligonucleotide. The Split Linker creates a distance of 51bp between the DigA and the linked Fok_a protein domain. The His Tag serves as a purification tag for Ni-NTA column purification.
Application
At least we succeeded to produce a working universal endonuclease with this part in combination with the part BBa_K243010, by cotransformation into E.coli(XL1blue). The part BBa_K243010 was cloned into our expression vector BBa_K243033 and this part was cloned into the vector pJS419 BBa_K243035.
The made a cutting assay was conducted with cleared cell lysate and DNA hybridized with oligonucleotides labeled with fluorescence molecule(Cy3). The two proteins linked to the hybridized oligonucleotides and cut them at chosen site.We proved the cutting event by gel electrophoresis and excitation of the fluorescence.
Gellanes:1.Marker(1kb ladder mix)2.Cell extract+sample1 3.Cell extract+sample2 4.control w/o cell extract.
Method
The pictures shows our gel one left excited by wavelength of 353 nm and on right side filtered with the cutoff filter of 580nm. The first lane shows the marker only visible on right gel picture, the second and third lane show the products of the cutting event made by our universal endonuclease. The comparison with fourth lane shows that the origin oligonucleotides are cut.In the fourth lane there were only the oligonucleotides loaded.
Detection of the Cy3
To excite the Cy3-tagged nucleotides a laser with a wavelength of 353 nm was used. To cut of the excitation wavelength in the pictures a cutoff filter of 580nm was used. In another approach the SteREO Lumar.V12 from Zeiss was used to excite the Cy3-tagged oligonucleotides.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21INCOMPATIBLE WITH RFC[21]Illegal BglII site found at 272
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000INCOMPATIBLE WITH RFC[1000]Illegal SapI.rc site found at 1126