Difference between revisions of "Part:BBa K518010"
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<Figure: UV-induced expression levels of [[Part:BBa_K518010 |sulAp]]. The expression levels from sulAp were evaluated before and after UV induction. We evaluated it using both ''recA''(-) (JM109) and ''recA''(+) (BL21) strain. RecA is known to be necessary for releasing sulAp from repression. We successfully demonstrated a significant alteration of expression in ''recA''(+) strain only after UV irradiation. The expression level of [[Part:BBa_J23119 |BBa_J23119]], a constitutive <i>E. coli</i> promoter which is often used as a comparison, was simultaneously presented. Data is expressed as mean ± S.D.. Data is obtained from the average of three independent experiments.>
 
<Figure: UV-induced expression levels of [[Part:BBa_K518010 |sulAp]]. The expression levels from sulAp were evaluated before and after UV induction. We evaluated it using both ''recA''(-) (JM109) and ''recA''(+) (BL21) strain. RecA is known to be necessary for releasing sulAp from repression. We successfully demonstrated a significant alteration of expression in ''recA''(+) strain only after UV irradiation. The expression level of [[Part:BBa_J23119 |BBa_J23119]], a constitutive <i>E. coli</i> promoter which is often used as a comparison, was simultaneously presented. Data is expressed as mean ± S.D.. Data is obtained from the average of three independent experiments.>
 
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===Team: 2020 SZ-SHD: Investigated the UV-induction time to the expression level of SulAp:===
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In our project, experiments have been carried out to measure the expression level of eGFP gene behind SulAp promoter in BL21, with different exposure time under UV induction.
  
 
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Revision as of 08:35, 25 October 2020

sulA promoter

Microbes including Escherichia coli are known to respond to various DNA-injuring stress (ionizing radiation, ultraviolet radiation, peroxides etc...), altering their gene expression patterns. This response, known as the "SOS response", is induced by a regulatory protein called RecA when it binds to single-strand DNA. The DNA-RecA complex promotes the degradation of LexA, a common repressor of SOS genes.

SulA is responsible for stress-induced halt of cell division. The promoter of sulA, sulAp, is induced by various stress factors, including ultraviolet irradiation.

Application

We utilized this property (induced-expression by UV irradiation) to design a "UV switch". This makes it possible to "switch on" a genetic circuit using UV. As a first step for this, we characterized the UV-induction of sulAp.

The UV-induced expression level of BBa_K518010 was evaluated using BBa_K518013. As a measurement tool, our dual luciferase assay kit was employed. For detailed infomation, see BBa_K518002.

SulApexpression.png

<Figure: UV-induced expression levels of sulAp. The expression levels from sulAp were evaluated before and after UV induction. We evaluated it using both recA(-) (JM109) and recA(+) (BL21) strain. RecA is known to be necessary for releasing sulAp from repression. We successfully demonstrated a significant alteration of expression in recA(+) strain only after UV irradiation. The expression level of BBa_J23119, a constitutive E. coli promoter which is often used as a comparison, was simultaneously presented. Data is expressed as mean ± S.D.. Data is obtained from the average of three independent experiments.>

Team: 2020 SZ-SHD: Investigated the UV-induction time to the expression level of SulAp:

In our project, experiments have been carried out to measure the expression level of eGFP gene behind SulAp promoter in BL21, with different exposure time under UV induction.

Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]