Team:IIT Madras/Project

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Revision as of 06:33, 23 July 2008

Home	About Us	Project Details	Notebook

Overall project

Background

Our project looks at a specific category of bacterial transcription factors. Sigma factors are prokaryotic transcription initiation factors that enable the specific binding of RNA polymerase to a variety of promoters. Escherichia coli sigma factors function to differentially express various sets of genes under different environmental conditions. Based on the feasibility of different promoters and their architectures, we've selected the following as ideal candidates for our project:

sigma70 (rpoD):housekeeping genes during exponential growth
sigma38/S (rpoS):master regulator for a generalized stress response
sigma32/H (rpoH):unfolded protein response
sigma28/F (rpoF):flagellar biosynthesis
sigma24/E (rpoE):response to unfolded proteins in the cell envelope

Objectives

Our goal is to assemble a library of sigma-dependent and lac contorlled promoters, and submit these to the Registry of Standard Biological Parts. This "StressKit" can be used to control gene expression specifically during each phase of the bacterial growth curve and will also give users the ability to regulate gene expression using temperature, pH and other stress inducers as external cues. This modular approach, identifying and standardizing a set of functional parts so they may be used in diverse future applications, is one of the central themes of synthetic biology.

Methodology

Candidate promoters have been identified from literature searches and bioinformatics. We've chosen 4 special sigma factors listed above in addition to the houskeeping sigma 70 to include in our library. Our design is an attempt to engineer the regulation achievable with a lac promoter fused with the differential expression of the sigma factor dependent promoters. The custom promoters have recognition elements of the 2 classes of promoters pasted between each other in the least intrusive fashion. These promoters are also designed to conform to the Registry's 'BioBrick' format (involving the removal of various restriction sites, and insertion into a standard plasmid backbone). We will then introduce these promoters into fluorescent expression systems and test their activity under various environmental stresses using fluorescence microscopy and spectroscopic techniques.

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-{|align="justify"
-|You can write a background of your team here.  Give us a background of your team, the members, etc.  Or tell us more about something of your choosing.
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-|-
-|
-''Tell us more about your project.  Give us background.  Use this is the abstract of your project.  Be descriptive but concise (1-2 paragraphs)''
-|[[Image:Team.png|right|frame|Your team picture]]
-|-
-|
-|align="center"|[[Team:IIT_Madras | Team Example 2]]
-|}
-<!--- The Mission, Experiments --->
-{| style="color:#1b2c8a;background-color:#0c6;" cellpadding="3" cellspacing="1" border="1" bordercolor="#fff" width="62%" align="center"
 !align="center"|[[Team:IIT_Madras|Home]]
-!align="center"|[[Team:IIT_Madras/Team|The Team]]
+!align="center"|[[Team:IIT_Madras/Team|About Us]]
-!align="center"|[[Team:IIT_Madras/Project|The Project]]
+!align="center"|[[Team:IIT_Madras/Project|Project Details]]
-!align="center"|[[Team:IIT_Madras/Parts|Parts Submitted to the Registry]]
-!align="center"|[[Team:IIT_Madras/Modeling|Modeling]]
 !align="center"|[[Team:IIT_Madras/Notebook|Notebook]]
 |}
-(''Or you can choose different headings.  But you must have a team page, a project page, and a notebook page.'')
 == '''Overall project''' ==
-Your abstract
+=== Background ===
+Our project looks at a specific category of bacterial transcription factors. Sigma factors are prokaryotic transcription initiation factors that enable the specific binding of RNA polymerase to a variety of promoters. Escherichia coli sigma factors function to differentially express various sets of genes under different environmental conditions. Based on the feasibility of different promoters and their architectures, we've selected the following as ideal candidates for our project:
+* sigma70 (rpoD):housekeeping genes during exponential growth
+* sigma38/S (rpoS):master regulator for a generalized stress response
+* sigma32/H (rpoH):unfolded protein response
+* sigma28/F (rpoF):flagellar biosynthesis
+* sigma24/E (rpoE):response to unfolded proteins in the cell envelope
+=== Objectives ===
+Our goal is to assemble a library of sigma-dependent and lac contorlled promoters, and submit these to the Registry of Standard Biological Parts. This "StressKit" can be used to control gene expression specifically during each phase of the bacterial growth curve and will also give users the ability to regulate gene expression using temperature, pH and other stress inducers as external cues. This modular approach, identifying and standardizing a set of functional parts so they may be used in diverse future applications, is one of the central themes of synthetic biology.
+===  Methodology ===
+Candidate promoters have been identified from literature searches and bioinformatics. We've chosen 4 special sigma factors listed above in addition to the houskeeping sigma 70 to include in our library. Our design is an attempt to engineer the regulation achievable with a ''lac'' promoter fused with the differential expression of the sigma factor dependent promoters. The custom promoters have recognition elements of the 2 classes of promoters pasted between each other in the least intrusive fashion. These promoters are also designed to conform to the Registry's 'BioBrick' format (involving the removal of various restriction sites, and insertion into a standard plasmid backbone). We will then introduce these promoters into fluorescent expression systems and test their activity under various environmental stresses using fluorescence microscopy and spectroscopic techniques.
 == Project Details==
+=== Project Design ===
-=== Part 2 ===
 === The Experiments ===
+=== Modelling ===
-=== Part 3 ===
 == Results ==

Team:IIT Madras/Project

From 2008.igem.org

Revision as of 06:33, 23 July 2008

Contents

Overall project

Background

Objectives

Methodology

Project Details

Project Design

The Experiments

Modelling

Results