Difference between revisions of "Part:BBa K1111012:Design"

Latest revision as of 21:41, 2 October 2013

Ice Nucleation Protein fused to Streptavidin Alive

Assembly Compatibility:

10
INCOMPATIBLE WITH RFC[10]
Illegal XbaI site found at 1727
12
COMPATIBLE WITH RFC[12]
21
INCOMPATIBLE WITH RFC[21]
Illegal BamHI site found at 1649
23
INCOMPATIBLE WITH RFC[23]
Illegal XbaI site found at 1727
25
INCOMPATIBLE WITH RFC[25]
Illegal XbaI site found at 1727
Illegal NgoMIV site found at 1036
Illegal AgeI site found at 1691
Illegal AgeI site found at 1742
1000
COMPATIBLE WITH RFC[1000]

Gibson Assembly Design

Insert: we amplified the streptavidin coding sequence received in a plasmid from Mark Howarth laboratory at Oxford university Dept. of Biochemistry.
Backbone: Starting from the biobrick BBa_K523013 (INP fused with YFP), we amplified the whole sequence except the EYFP and added gibson overhang complementary to streptavidin ends.

Primers

Streptavidin Alive PCR :
5' ATGGCTGAAGCTGGTATCACC 3'
5' TTAGGAAGCAGCGGACGGTTTAAC 3'

BBa_K523013 PCR :
Fw: 5' ACCAAAGTTAAACCGTCCGCTGCTTCTAACATATCATAACGGAGTGATCGCAATG 3'
Rev: 5' CCAGGTGCCGGTGATACCAGCTTCAGCCATAGATCCCGCCACGCTGCT 3'

Source

Can be expressed in Escherichia Coli.

References and acknowledgements

Thanks to the Mark Howarth laboratory at Oxford university Dept. of Biochemistry [http://users.ox.ac.uk/~bioc0756/MyWebs/activesite/ReagentDistribution.htm] for providing us with the streptavidin cloning plasmid.
Thanks to the iGEM team of Edinburgh 2011 that designed the Biobrick BBa_K523013 [1].

@@ Line 4: / Line 4: @@
 <partinfo>BBa_K1111012 SequenceAndFeatures</partinfo>
-==Design Notes==
+==Gibson Assembly Design ==
-To assemble this part, we orderd a plasmid containing the streptavidin alive.
+''Insert:'' we amplified the streptavidin coding sequence received in a plasmid from Mark Howarth laboratory at Oxford university Dept. of Biochemistry.
-We amplified only the coding sequence of streptavidin of the plasmid by PCR. Also, we did a PCR with overlapping ends corresponding to streptavidin on the '''Biobrick BBa_K523013''' (INP fused with YFP). This PCR was keeping all the plasmid including RBS and Lac promoter but excluding YFP. The linearized plasmid and the insert were then assembled by Gibson assembly.
+<br>''Backbone:'' Starting from the biobrick BBa_K523013 (INP fused with YFP), we amplified the whole sequence except the EYFP and added gibson overhang complementary to streptavidin ends.
 ==Primers==
-PCR of streptavidin alive :
+Streptavidin Alive PCR :
-' ATGGCTGAAGCTGGTATCACC 3'
+<br>5' <font color = #0000FF>ATGGCTGAAGCTGGTATCACC</font> 3'
-' TTAGGAAGCAGCGGACGGTTTAAC 3'
+<br>5' <font color = #0000FF>TTAGGAAGCAGCGGACGGTTTAAC</font> 3'
-Overlapping PCR of BBa_K523013 :
+BBa_K523013 PCR :
-' accaaagttaaaccgtccgctgcttcctaacatatcataacggagtgatcgcaatg 3'
+<br>Fw: 5' <font color = #0000FF>ACCAAAGTTAAACCGTCCGCTGCTTCT</font><font color= red>AACATATCATAACGGAGTGATCGCAATG</font> 3'
-' ccaggtgccggtgataccagcttcagcCATagatcccgccacgctgct 3'
+<br>Rev: 5' <font color = #0000FF>CCAGGTGCCGGTGATACCAGCTTCAGCCAT</font><font color= red>AGATCCCGCCACGCTGCT</font> 3'
-==References and Acknowledgements==
+==Source==
-Thanks to the Mark Howarth lab, Biochemistry Dpt in Oxford, for providing us the needed plasmid.
+Can be expressed in Escherichia Coli.
+==References and acknowledgements==
+Thanks to the '''Mark Howarth laboratory at Oxford university Dept. of Biochemistry''' [http://users.ox.ac.uk/~bioc0756/MyWebs/activesite/ReagentDistribution.htm] for providing us with the streptavidin cloning plasmid.
+<br>Thanks to the '''iGEM team of Edinburgh 2011''' that designed the Biobrick BBa_K523013 [https://parts.igem.org/Part:BBa_K523013].