Team:Bielefeld-Germany/Results/Unfinished

From 2010.igem.org

(Difference between revisions)
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===Mutated ''virG''===
===Mutated ''virG''===
-
This version of ''virG'' activates ''vir'' promotors in ''Escherichia coli'' without the ''rpoA''-gene from ''Agrobacterium tumefaciens''. For this reason the point mutations G56V and I77V are brought into the molecule (compare YC Jung ''et al.'', 2004). Because this BioBrick is synthesized (Mr.Gene GmbH), codon usage is optimized for ''E. coli'' and illegal restriction sites were removed.
+
Phosphorylated VirG binds to ''vir'' promotors and activates them. VirG is activated by the acetosyringone receptor VirA.
 +
This version of VirG activates ''vir'' promotors in ''Escherichia coli'' without the ''rpoA''-gene from ''Agrobacterium tumefaciens''. For this reason the point mutations G56V and I77V are brought into the molecule (compare YC Jung ''et al.'', 2004). Because this BioBrick is synthesized (Mr.Gene GmbH), codon usage is optimized for ''E. coli'' and illegal restriction sites were removed. When you use this ''virG'' gene in a ''virA/G'' signaling system you do not need <partinfo>K238010</partinfo> anymore to get the system working in ''E. coli''.  
You can find this BioBrick here: <partinfo>K389002</partinfo>
You can find this BioBrick here: <partinfo>K389002</partinfo>
Line 11: Line 12:
===''virA'' receptor===
===''virA'' receptor===
-
Actually we wanted to use the ''virA'' receptor already existing in the partsregistry (<partinfo>K238008</partinfo>). But due to some problems (compare results in BioBricks/tested) we decided to isolate the ''virA'' gene from ''A. tumefaciens'' C58 ourselves and bring it into a BioBrick compatible form. We removed an illegal ''PstI'' restriction site in the ''virA'' gene by site-directed mutagenesis.  
+
The VirA receptor is used by ''A. tumefaciens'' to detect acetosyringone and other phenolic substances which are secreted by plants after injury. In presence of these substances VirA phosphorylates VirG, a response regulator which activates ''vir'' promotors. These promotors control genes which are used for infecting the injured plant.
 +
Actually we wanted to use the ''virA'' receptor already existing in the partsregistry (<partinfo>K238008</partinfo>). But due to some problems (compare results in BioBricks/tested) we decided to isolate the ''virA'' gene from the TI-plasmid of ''A. tumefaciens'' C58 ourselves and bring it into a BioBrick compatible form. We removed an illegal ''PstI'' restriction site in the ''virA'' gene by site-directed mutagenesis.  
You can find this BioBrick here: <partinfo>K389001</partinfo>
You can find this BioBrick here: <partinfo>K389001</partinfo>
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===''vir''-promotor===
===''vir''-promotor===
-
We wanted to use the ''vir''-promotor from the partsregistry (<partinfo>K238011</partinfo>) but the same problems occurred like with the use of the ''virA'' receptor from the partsregistry. So we also have to create a new ''vir''-promotor BioBrick (again from ''A. tumefaciens'' C58).
+
We wanted to use the ''vir''-promotor from the partsregistry (<partinfo>K238011</partinfo>) but the same problems occurred like with the use of the ''virA'' receptor from the partsregistry. So we also have to create a new ''vir''-promotor BioBrick (again from TI-plasmid of ''A. tumefaciens'' C58).
You can find this BioBrick here: <partinfo>K389003</partinfo>
You can find this BioBrick here: <partinfo>K389003</partinfo>
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===''virA'' screening system===
===''virA'' screening system===
-
We will use the BioBrick for ''virA''-screenings in a plasmid with R6K ori and the mutated ''virA'' in the pSB1C3 plasmid with ColE1 ori. Both plasmids will be installed and screened in ''E. coli'' EC100D. Once we will find a construct with high sensitivity for a screened substance, we will isolate the plasmids and transform them to ''e.g.'' ''E. coli'' TOP10. Because the R6K ori does not work in this strain, we can easily separate the mutated ''virA'' BioBrick from the screening plasmid. Because the ''virA'' is in the pSB1C3 vector, we won't have to do further cloning.  
+
We will use the BioBrick for ''virA''-screenings (<partinfo>K389011</partinfo>) in a plasmid with R6K ori and the mutated ''virA'' in the pSB1C3 plasmid with ColE1 ori. Both plasmids will be transformed to and screened in ''E. coli'' EC100D. Once we will find a construct with high sensitivity for a screened substance, we will isolate the plasmids and transform them to ''e.g.'' ''E. coli'' TOP10. Because the R6K ori does not work in this strain, we can easily separate the mutated ''virA'' BioBrick from the screening plasmid. Because the ''virA'' is in the pSB1C3 vector, we won't have to do further cloning.  
===Firefly luciferase===
===Firefly luciferase===
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===Reporter construct===
===Reporter construct===
-
The reporter construct is similar to the ''virA'' screening construct but instead of the antibiotic resistance it carries a reporter gene (''e.g.'' GFP or luciferase). The amount of produced reporter shows the activity of the ''virA'' receptor.
+
The reporter construct is similar to the ''virA'' screening construct but instead of the antibiotic resistance it carries a reporter gene (''e.g.'' GFP or luciferase). The amount of produced reporter shows the activity of the ''virA'' receptor. If the original ''vir'' promotor is too weak, we will use Cambridge's sensitivity tuners to increase the output signal of our biosensor.  
==Literature==
==Literature==
YC Jung ''et al.'' (2004) Mutants of ''Agrobacterium tumefaciens'' ''virG'' Gene That Activate Transcription of ''vir'' Promoter in ''Escherichia coli'', ''Current Microbiol'' 49:334-340.
YC Jung ''et al.'' (2004) Mutants of ''Agrobacterium tumefaciens'' ''virG'' Gene That Activate Transcription of ''vir'' Promoter in ''Escherichia coli'', ''Current Microbiol'' 49:334-340.

Revision as of 11:38, 4 September 2010

{{{1}}}

Contents

Unfinished BioBricks

Mutated virG

Phosphorylated VirG binds to vir promotors and activates them. VirG is activated by the acetosyringone receptor VirA. This version of VirG activates vir promotors in Escherichia coli without the rpoA-gene from Agrobacterium tumefaciens. For this reason the point mutations G56V and I77V are brought into the molecule (compare YC Jung et al., 2004). Because this BioBrick is synthesized (Mr.Gene GmbH), codon usage is optimized for E. coli and illegal restriction sites were removed. When you use this virG gene in a virA/G signaling system you do not need <partinfo>K238010</partinfo> anymore to get the system working in E. coli.

You can find this BioBrick here: <partinfo>K389002</partinfo>

This BioBrick is finished but we haven't submitted it to the registry yet.

virA receptor

The VirA receptor is used by A. tumefaciens to detect acetosyringone and other phenolic substances which are secreted by plants after injury. In presence of these substances VirA phosphorylates VirG, a response regulator which activates vir promotors. These promotors control genes which are used for infecting the injured plant. Actually we wanted to use the virA receptor already existing in the partsregistry (<partinfo>K238008</partinfo>). But due to some problems (compare results in BioBricks/tested) we decided to isolate the virA gene from the TI-plasmid of A. tumefaciens C58 ourselves and bring it into a BioBrick compatible form. We removed an illegal PstI restriction site in the virA gene by site-directed mutagenesis.

You can find this BioBrick here: <partinfo>K389001</partinfo>

This BioBrick is finished but we haven't submitted it to the registry yet.

vir-promotor

We wanted to use the vir-promotor from the partsregistry (<partinfo>K238011</partinfo>) but the same problems occurred like with the use of the virA receptor from the partsregistry. So we also have to create a new vir-promotor BioBrick (again from TI-plasmid of A. tumefaciens C58).

You can find this BioBrick here: <partinfo>K389003</partinfo>

This BioBrick is finished but we haven't submitted it to the registry yet.

Neomycin / kanamycin resistance

A neomycin / kanamycin resistance gene without promotor is isolated and brought into a BioBrick compatible form. We will use the BioBrick <partinfo>P1003</partinfo> as source for the kanamycin resistance gene.

You can find this BioBrick here: <partinfo>K389005</partinfo>

This BioBrick is finished, but we have not submitted it to the registry yet

BioBrick for virA-screenings

This part contains our mutated virG BioBrick under the control of a constitutive promotor (<partinfo>J23110</partinfo>) and an antibiotic resistance (<partinfo>K389005</partinfo>) under the control of the virB promotor (<partinfo>K389003</partinfo>). The better the virA receptor recognizes a substance the stronger will the antibiotic resistance be expressed.

You can find this BioBrick here: <partinfo>K389011</partinfo>

Mutated virA

The virA gene is mutated by error prone PCR and screened for several phenolic substances (e.g. capsaicin and homovanillic acid). The goal is to receive highly specific and sensitive mutated virA receptors by directed evolution. The virA will be under the control of a constitutive promotor (<partinfo>J23110</partinfo>).

Plasmid with R6K origin of replication

In order to install our virA screening system, we need two plasmids in one cell. So we have to create a BioBrick compliant plasmid which has a different compatibility group as the standard pSBXXX plasmids. Our plan is to replace the ColE1 ori from a pSBXXX plasmid with a R6K ori (<partinfo>J61001</partinfo>). The R6K ori works e.g. in E. coli EC100D strains and is compatible with ColE1 oris.

virA screening system

We will use the BioBrick for virA-screenings (<partinfo>K389011</partinfo>) in a plasmid with R6K ori and the mutated virA in the pSB1C3 plasmid with ColE1 ori. Both plasmids will be transformed to and screened in E. coli EC100D. Once we will find a construct with high sensitivity for a screened substance, we will isolate the plasmids and transform them to e.g. E. coli TOP10. Because the R6K ori does not work in this strain, we can easily separate the mutated virA BioBrick from the screening plasmid. Because the virA is in the pSB1C3 vector, we won't have to do further cloning.

Firefly luciferase

Bringing the firefly luciferase gene from Promega's pGL4 vector into a BioBrick compatible form as a sensitive reporter gene.

You can find this BioBrick here: <partinfo>K389004</partinfo>

This BioBrick is finished, but we have not submitted it to the registry yet

Reporter construct

The reporter construct is similar to the virA screening construct but instead of the antibiotic resistance it carries a reporter gene (e.g. GFP or luciferase). The amount of produced reporter shows the activity of the virA receptor. If the original vir promotor is too weak, we will use Cambridge's sensitivity tuners to increase the output signal of our biosensor.

Literature

YC Jung et al. (2004) Mutants of Agrobacterium tumefaciens virG Gene That Activate Transcription of vir Promoter in Escherichia coli, Current Microbiol 49:334-340.