Team:MIT/Projects/Project2

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(Mechanism)
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Construction of the PhyB-CFP and Pif3-YFP Plasmids began with the amplification of each of the individual sequences, PhyB, CFP, PIF3 and YFP, from the Berkley Lab Plasmids. These sequences were subsequently digested and ligated into the prS313 backbone, a plasmid that contains a constitutive Myo2 promoter and the His gene.  PIF3 and CFP were inserted using NotI and SacII, while PhyB, YFP used NotI and XmaI.  Once the plasmid was complete it was transformed into ''E. coli''.  The PhyB and Pif3 plasmids transformed successfully, which was confirmed through a check digest and sequencing.  The corresponding fluorescent protein DNA was then incorporated into the plasmid through another round of digestion, ligation and transformation.  The sequencing results for these plasmids were positive for incorporation of both DNA pieces for both of the constructs.  Therefore, each of these plasmids were transformed into yeast and observed for fluorescence through microscopy.   
Construction of the PhyB-CFP and Pif3-YFP Plasmids began with the amplification of each of the individual sequences, PhyB, CFP, PIF3 and YFP, from the Berkley Lab Plasmids. These sequences were subsequently digested and ligated into the prS313 backbone, a plasmid that contains a constitutive Myo2 promoter and the His gene.  PIF3 and CFP were inserted using NotI and SacII, while PhyB, YFP used NotI and XmaI.  Once the plasmid was complete it was transformed into ''E. coli''.  The PhyB and Pif3 plasmids transformed successfully, which was confirmed through a check digest and sequencing.  The corresponding fluorescent protein DNA was then incorporated into the plasmid through another round of digestion, ligation and transformation.  The sequencing results for these plasmids were positive for incorporation of both DNA pieces for both of the constructs.  Therefore, each of these plasmids were transformed into yeast and observed for fluorescence through microscopy.   
<center>[[Image:Trans.jpg]] </center>
<center>[[Image:Trans.jpg]] </center>
 +
Caption: The construct design with Restriction Enzymes for Sequential Transformation.
Alongside work in the base constructs, a variety of C and N terminus localization sequences were chosen to test the PhyB, Pif System. Each localization sequence, once amplified, would be cloned into the appropriate backbone using the restriction enzymes. N terminus tags were destined for the Pif3-YPF backbone and C terminus for the PhyB-CFP Backbone
Alongside work in the base constructs, a variety of C and N terminus localization sequences were chosen to test the PhyB, Pif System. Each localization sequence, once amplified, would be cloned into the appropriate backbone using the restriction enzymes. N terminus tags were destined for the Pif3-YPF backbone and C terminus for the PhyB-CFP Backbone
<center>[[Image:Target sequences.jpg]] </center>
<center>[[Image:Target sequences.jpg]] </center>
-
Caption: These demonstrate the anchor traveler constructs we designed for the PhyB-PIF3 system
+
Caption: A table of the signaling sequences chosen.  These would serve to anchor one protein to a particular organelle.
=== Homologous Recombination===
=== Homologous Recombination===

Revision as of 01:06, 22 October 2009

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Light-inducible protein localization in Yeast

Localization system2.jpg
Caption:Shown here the blue dots represent PhyB bound to a CFP, which diffuses throughout the cell. Meanwhile PIF3 tagged with YFP is constitutively localized to an organelle, (a mitochondria shown here). In the presence of red light, PhyB changes conformation so that it can bind to PIF3. As the PhyB travels throughout the cell it binds to PIF3, causing CFP to localize to the mitochondria. The introduction of far red light will reverse this process allowing PhyB-CFP fusion to diffuse throughout the cell again.

Objective

We set out to create a quick, reversible switch to control the localization to various targets within a yeast cell, such as the nuclear membrane, plasma membrane, mitochondrial membrane, and vacuole.

Motivation

To fully control cellular functioning, it would be useful to have a modular system that can provide both temporal and spatial control over any protein of interest within a cell. In other words, we should be able to control both when a gene is expressed and where the protein is functioning. The existing PhyB-PIF3 system provides temporal control over gene expression by acting as a transcriptional regulator. However, by adapting the PhyB-PIF3 system to control protein targeting, we can have both temporal and spatial control over a protein's functioning. Such a system can potentially be used as an on-off switch for essential genes by controlling movement the protein to and from where the protein functions in the cell. In addition, because protein targeting is key in controlling the cell cycle, the system can also potentially be used to control cell cycling and differentiation. Furthermore, reversible control of protein localization and delocalization can be useful as a tool to study diffusion rates within a cell.

Background on PhyB-PIF3 System

PhyPIFbkgrd.jpg

Mechanism

To localize our protein of interest, either PhyB or PIF3 is anchored to the target while the other diffuses throughout the cell.

Mechanism.jpg

Caption: This figure is an overview of the PhyB-PIF3 anchor traveler mechanism for the localization of proteins in the cell

Localization design.jpg

Caption: These demonstrate the anchor traveler constructs we designed for the PhyB-PIF3 system

Materials and Methods

Construct Construction

Sequential Transformation Plasmid Construction

Construction of the PhyB-CFP and Pif3-YFP Plasmids began with the amplification of each of the individual sequences, PhyB, CFP, PIF3 and YFP, from the Berkley Lab Plasmids. These sequences were subsequently digested and ligated into the prS313 backbone, a plasmid that contains a constitutive Myo2 promoter and the His gene. PIF3 and CFP were inserted using NotI and SacII, while PhyB, YFP used NotI and XmaI. Once the plasmid was complete it was transformed into E. coli. The PhyB and Pif3 plasmids transformed successfully, which was confirmed through a check digest and sequencing. The corresponding fluorescent protein DNA was then incorporated into the plasmid through another round of digestion, ligation and transformation. The sequencing results for these plasmids were positive for incorporation of both DNA pieces for both of the constructs. Therefore, each of these plasmids were transformed into yeast and observed for fluorescence through microscopy.

Trans.jpg

Caption: The construct design with Restriction Enzymes for Sequential Transformation.

Alongside work in the base constructs, a variety of C and N terminus localization sequences were chosen to test the PhyB, Pif System. Each localization sequence, once amplified, would be cloned into the appropriate backbone using the restriction enzymes. N terminus tags were destined for the Pif3-YPF backbone and C terminus for the PhyB-CFP Backbone

Target sequences.jpg

Caption: A table of the signaling sequences chosen. These would serve to anchor one protein to a particular organelle.

Homologous Recombination

Homologous recombination.jpg
Hom.jpg

LED Arrays for Red and Far Red Light

LEDbox.jpg

Plans