Difference between revisions of "Part:BBa K1114701"
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The fusion site letters refer to 4bp fusion sites: A = GGAG; B = TACT; C = AATG; D = AGGT; E = GCTT; F = CGCT; G = TGCC; H = ACTA. See Level 0 pages for further information. | The fusion site letters refer to 4bp fusion sites: A = GGAG; B = TACT; C = AATG; D = AGGT; E = GCTT; F = CGCT; G = TGCC; H = ACTA. See Level 0 pages for further information. | ||
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<p>We characterized this part using flow cytometry. The cells were grown overnight into stationary phase prior to a 1:200 dilution into 1XPBS, which was then run on a SORP LSRFortessa machine. We then used the <a href="https://synbiotools.bbn.com/">TASBE tools</a> to analyze our data and convert our readings into molecules of equivalent fluorescin (MEFL). </p> | <p>We characterized this part using flow cytometry. The cells were grown overnight into stationary phase prior to a 1:200 dilution into 1XPBS, which was then run on a SORP LSRFortessa machine. We then used the <a href="https://synbiotools.bbn.com/">TASBE tools</a> to analyze our data and convert our readings into molecules of equivalent fluorescin (MEFL). </p> |
Revision as of 22:06, 27 September 2013
BioBrick of Level 1 MoClo RFP Reporter
This is a BioBrick adaptation of the Level 1 MoClo device that constitutively expresses RFP. It contains the Level 0 parts J23104_AB, BCD8_BC, E1010m_CD, and B0015_DE within the pSB1C3 backbone. In the given sequence the internal fusion sites are incorrectly duplicated.
The fusion site letters refer to 4bp fusion sites: A = GGAG; B = TACT; C = AATG; D = AGGT; E = GCTT; F = CGCT; G = TGCC; H = ACTA. See Level 0 pages for further information.
Characterization
We characterized this part using flow cytometry. The cells were grown overnight into stationary phase prior to a 1:200 dilution into 1XPBS, which was then run on a SORP LSRFortessa machine. We then used the TASBE tools to analyze our data and convert our readings into molecules of equivalent fluorescin (MEFL).
By converting the flow cytometry data into MEFLs, we now have an absolute unit of measurement for comparison.
The data is binned by fluorescence intensity and the tool also provides the cell count for each bin. We can see the population has a wide distribution of expression (top graph, blue bars).
The bottom graph shows the same data as the one above, but this is now ordered by cell count, from highest (dark purple) to lowest (pale purple).
We can now see that within the population of cells, the smallest binned group shows the highest level of expression. This may be due to higher copy counts of plasmids within that subpopulation of cells.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12INCOMPATIBLE WITH RFC[12]Illegal NheI site found at 11
Illegal NheI site found at 34 - 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal AgeI site found at 694
Illegal AgeI site found at 806 - 1000COMPATIBLE WITH RFC[1000]