Team:SDU-Denmark/project-t
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=== Background === | === Background === | ||
+ | <br> | ||
+ | The flagella regulon in Escherichia coli is composed of at least 50 genes organized in no less than 14 ope-rons that all contribute to the synthesis and operation of flagella. The operons are synthesized in a three-level transcriptional cascade where the FlhDC operon is the master regulator at the top of the cascade. The flagella regulon is tightly controlled by nutritional and environmental conditions, E. coli starved of ami-no acids showed temporarily decrease of the flagella regulon transcripts which are needed for the synthesis and operation of the flagellum.[http://onlinelibrary.wiley.com/doi/10.1111/j.1365-2958.2009.06939.x/full (1)] | ||
+ | The synthesis and assembly of flagella are regulated by the transcriptional cascade composed of three levels of gene products (class I, -II and –III). Class I genes consist of a single operon encoding the proteins FlhD and FlhC that form a multimeric (FlhD4C2) transcriptional activation complex. This ‘master regulator’ stimulates transcription by binding upstream of Class II promoters. Class II genes encode proteins that assemble to form the basal body and hook of the flagellum, as well as the fliA gene that encodes the alternative σ factor σ28, also called σF. σ28 binds to RNA polymerase (RNAP) core enzyme and directs it to Class III promoters. Class III genes encode the rest of the structural genes of the flagellum, including fliC encoding flagellin, as well as the chemotaxis apparatus. [http://onlinelibrary.wiley.com/doi/10.1111/j.1365-2958.2009.06939.x/full (1)] | ||
+ | <br> | ||
+ | It has been shown that overexpression of the FlhDC operon restores motility in mutants that have been made immotile [http://jb.asm.org/cgi/content/short/181/24/7500 (2)]. Also, overexpression of FlhDC in the E. coli K12 strain MG1655 made the cells hypermotile.[http://iai.asm.org/cgi/content/abstract/75/7/3315 (3)] | ||
+ | <br><br> | ||
+ | '''Our system''' | ||
<br> | <br> | ||
To maximize the microflow system's effectivity, we want to increase the force each single bacterium can generate. Since the main motor for the flow is the flagellum we will have to modify this factor for increasing the force. Flagella in E.Coli rotate at a maximum speed around 6000 rpm, which can not easily be exceeded. So if we wanted to increse the generated force we would have to opt for more flagella on the surface of our bacteria, instead of faster flagella. This is called hyperflagellation, which is a process that is not all too well studied in normally-flagellated coli, so we will have to test it out.<br> | To maximize the microflow system's effectivity, we want to increase the force each single bacterium can generate. Since the main motor for the flow is the flagellum we will have to modify this factor for increasing the force. Flagella in E.Coli rotate at a maximum speed around 6000 rpm, which can not easily be exceeded. So if we wanted to increse the generated force we would have to opt for more flagella on the surface of our bacteria, instead of faster flagella. This is called hyperflagellation, which is a process that is not all too well studied in normally-flagellated coli, so we will have to test it out.<br> | ||
- | The way we are hoping to achieve the hyper flagellation is by upregulating the FlhD,C operon | + | The way we are hoping to achieve the hyper flagellation is by upregulating the FlhD,C operon.Since FlhD,C is sitting on top of the regulating cascade we want to overexpress it, so that we will get an increase in flagellar count.<br> |
The way we are going to achieve that is by isolating the operon from an E.Coli and inserting the coding sequence into a biobrick where we can control both the ribosome binding site and the type of promoter. We are going to use a constitutive promoter, so that flagella will be constantly expressed. The effects of this on other areas of the organism like the cell cycle are not entirely clear, but we will first try to overxpress the operon and then analyse the effect on the cells behavior.<br><br> | The way we are going to achieve that is by isolating the operon from an E.Coli and inserting the coding sequence into a biobrick where we can control both the ribosome binding site and the type of promoter. We are going to use a constitutive promoter, so that flagella will be constantly expressed. The effects of this on other areas of the organism like the cell cycle are not entirely clear, but we will first try to overxpress the operon and then analyse the effect on the cells behavior.<br><br> | ||
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<br> | <br> | ||
FlhD,C coding sequence: BBa_K343000 (Sandboxed) | FlhD,C coding sequence: BBa_K343000 (Sandboxed) | ||
+ | FlhDC composite part: BBa_K343004 | ||
</div> | </div> |
Revision as of 10:02, 14 October 2010