Difference between revisions of "Part:BBa K2403005"
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The results of the detection by qRT-PCR were as follows | The results of the detection by qRT-PCR were as follows | ||
− | [[File:プロモーター比較表.jpg|500px|thumb|center|'''Figure 1 : Results of detection by qRT-PCR (qRT-PCR targeted to the loop portion of hairpin. Data was normalized with 25S rRNA. n=3 )''']] | + | [[File:プロモーター比較表.jpg|500px|thumb|center|'''Figure 1 : Results of detection by qRT-PCR |
+ | (qRT-PCR targeted to the loop portion of hairpin. Data was normalized with 25S rRNA. n=3 )''']] | ||
As a result, it was revealed that RNA expression from the conditional Gal1promoter was high in the presence of galactose, and repressed in the presence of glucose, as we expected. The constitutive GPD promoter had an RNA expression level even lower than from the conditional Gal1 promoter (''' [https://parts.igem.org/Part:BBa_J63006 BBa_J63006] ''') in Glucose (Glu) medium, a condition which suppresses expression from Gal1promoter. | As a result, it was revealed that RNA expression from the conditional Gal1promoter was high in the presence of galactose, and repressed in the presence of glucose, as we expected. The constitutive GPD promoter had an RNA expression level even lower than from the conditional Gal1 promoter (''' [https://parts.igem.org/Part:BBa_J63006 BBa_J63006] ''') in Glucose (Glu) medium, a condition which suppresses expression from Gal1promoter. | ||
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==Reference== | ==Reference== |
Revision as of 02:35, 2 November 2017
Gal1 promoter>loop for dsRNA
This parts can be used for expressing dsRNA in Saccharomyces Cerevisiae.
Usage and Biology
In order to kill pine wood nematodes by feeding RNAi, we made hairpin loop-dsRNA targeted to the nematodes expressed in budding yeast serving as feed. We used BBa_J63006 as a promoter in that case. This part was used to express hairpin-dsRNA in budding yeast by adding loop [1], [2] to BBa_J63006 . You can create plasmid transcribing dsRNA with hairpin loop which can be expressed in budding yeast by cleaving with restriction enzyme Not1, connecting sense part between the loop part and the promoter, further cleaving with a restriction enzyme, Hind 3 sand connecting antisense strand.
Characterization
The expression level of dsRNA was assayed using Gal1 promoter ( BBa_J63006 ) and GPD promoter ( BBa_K517001 ) to characterize the RNA expression ability of these promoter parts.
The results of the detection by qRT-PCR were as follows
As a result, it was revealed that RNA expression from the conditional Gal1promoter was high in the presence of galactose, and repressed in the presence of glucose, as we expected. The constitutive GPD promoter had an RNA expression level even lower than from the conditional Gal1 promoter ( BBa_J63006 ) in Glucose (Glu) medium, a condition which suppresses expression from Gal1promoter.
Reference
For the sequence of the loop part used for Hairpin loop-dsRNA expression, the following paper was referred to.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12INCOMPATIBLE WITH RFC[12]Illegal NotI site found at 550
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal AgeI site found at 150
- 1000COMPATIBLE WITH RFC[1000]