Difference between revisions of "Part:BBa J63006:Experience"
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DISCLAIMER: It may be that there was some error in cloning. We have to sequence to find out if we placed the <partinfo>BBa_J63006</partinfo> GAL Promoter accurately into our GFP reporter construct. Nonetheless, PCR has been performed to confirm the presence of the <partinfo>BBa_J63006</partinfo> GAL Promoter upstream of the GFP reporter. We are currently sequencing this construct and will have details at the Regional Jamboree 2011. | DISCLAIMER: It may be that there was some error in cloning. We have to sequence to find out if we placed the <partinfo>BBa_J63006</partinfo> GAL Promoter accurately into our GFP reporter construct. Nonetheless, PCR has been performed to confirm the presence of the <partinfo>BBa_J63006</partinfo> GAL Promoter upstream of the GFP reporter. We are currently sequencing this construct and will have details at the Regional Jamboree 2011. | ||
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+ | Another potential explanation for why this part may not have worked compared to our own <partinfo>BBa_K517000</partinfo> GAL Promoter is that the kozak sequence may be interfering with expression of protein downstream; since the kozak sequence itself carries an ATG, it may be possible that this is competing with the ATG of the GFP to result in less expression even under galactose induction. | ||
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+ | [[Image:ubcigem2011alignmentgal.jpg | frame | center | We aligned this (1) <partinfo>BBa_J63006</partinfo> GAL Promoter+Kozak Sequence against our (2) <partinfo>BBa_K517000</partinfo> GAL Promoter. There is 180bp upstream sequence present in (1) that is absent in (2), as well as the 27bp Kozak Sequence downstream of the identical sequence regions.]] | ||
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Revision as of 21:42, 27 September 2011
This experience page is provided so that any user may enter their experience using this part.
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how you used this part and how it worked out.
Applications of BBa_J63006
User Reviews
UNIQ699c76acf8c50d47-partinfo-00000000-QINU
•••
British Columbia iGEM 2011 |
Inconclusive results on our part since we have not yet sequenced but only used PCR to determine accurate placement of promoter and kozak sequence in front of GFP reporter. Please refer to characterization data below for more details. |
UNIQ699c76acf8c50d47-partinfo-00000002-QINU
Characterization by British Columbia iGEM 2011
Fluorescence Analysis of GFP expression as regulated by GPD and GAL Promoters
The GPD promoter (BBa_K517001), GAL promoter (BBa_K517000) and GAL1 promoter with Kozak sequence (BBa_J63006) as characterized by their regulation of the expression of a GFP reporter.
Microscopy images show that the BBa_K517001 GPD promoter is constitutively activated and there is induction of the BBa_K517000 GAL promoter when it is shifted to galactose media. However, it is difficult to differentiate the expression of GFP under the regulation of the BBa_J63006 GAL Promoter with kozak sequence whether in glucose or galactose media. We have also analysed these by fluorescence activated cell sorting (FACS) (data available on BBa_K517000 and BBa_K517001 experience pages) but it remains ambiguous for the BBa_J63006 GAL Promoter. It would appear that were is a very weak constitutive expression of the GFP reporter under the BBa_J63006 GAL Promoter.
As a follow up to this experiment, we did a quick check of the BBa_J63006 GAL Promoter, but results were again not conclusive; there does not seem to be a clear induction of GFP expression when grown in galactose media.
DISCLAIMER: It may be that there was some error in cloning. We have to sequence to find out if we placed the BBa_J63006 GAL Promoter accurately into our GFP reporter construct. Nonetheless, PCR has been performed to confirm the presence of the BBa_J63006 GAL Promoter upstream of the GFP reporter. We are currently sequencing this construct and will have details at the Regional Jamboree 2011.
Another potential explanation for why this part may not have worked compared to our own BBa_K517000 GAL Promoter is that the kozak sequence may be interfering with expression of protein downstream; since the kozak sequence itself carries an ATG, it may be possible that this is competing with the ATG of the GFP to result in less expression even under galactose induction.