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Latest revision as of 02:07, 28 October 2013

National Yang Ming University

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 <div lang="latex" class="equation">
-\frac{d[CI]}{dt}={RBS}\times{[mRNACI]} -KdegCI\times[CI]
+\frac{d[LacI]}{dt}={RBS}\times{[mRNA LacI]} –{Kdeg LacI} \times{[LacI]}
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 </html>
 In this equation, RBS represents ribosome binding site strength, which is the affinity of ribosome to the starting site of mRNA.
+For the section of the equation, <html><span lang="latex"> RBS\times [mRNALacI] </span></html> represents the synthesizing rate of LacI; <html><span lang="latex"> -KdegCI\times [LacI] </span></html> represents the degrading rate of LacI .
-	For the section of the equation, <html><span lang="latex"> RBS\times [mRNAcI] </span></html> represents the synthesizing rate of CI; <html><span lang="latex">  -{kdegCI}\times {[CI]} </span></html> represents the degrading rate of CI.
+LacI will repress pLac promoter, which leads to no production of CI. Without CI, LuxCI hybrid promoter will no longer be repressed, and kill protein can thus be generated. This situation happens when Nosema exists and the sensor promoter is turned on.s.
-	Since LuxCI hybrid promoter is CI dominant, the presence of CI block the promoter and kill protein is not produced. This situation happens when there is no Nosema in bees.
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