Team:ETH Zurich/Mutant

From 2013.igem.org

(Difference between revisions)
Line 5: Line 5:
<p align="justify">In order to use the orthogonal hydrolases as our reporter system in the sender-receiver set-up, we needed to use a strain of ''E. coli'' where the expression of native hydrolase genes were knocked out. This is to prevent background hydrolysis of hydrolases. <br>
<p align="justify">In order to use the orthogonal hydrolases as our reporter system in the sender-receiver set-up, we needed to use a strain of ''E. coli'' where the expression of native hydrolase genes were knocked out. This is to prevent background hydrolysis of hydrolases. <br>
-
In our sender-receiver circuit, we use three hydrolases'' gusA'' , ''aes'' and ''nagZ''. Hence, three hydrolase genes were knocked out of ''E. coli'' strain MG1655. The ''gusA'' hydrolase was knocked out by a scarless deletion scheme that left no scar sequences after the deletion method [1]. The subsequent deletions of ''aes'' and ''nagZ'' was carried out by the P1 phage transduction by using deletion strain from the Keio collection [2]. Thus we were able to use this strain MG1655&#9651;''gusA''&#9651;''aes''&#9651;''nagZ'' knocked out of expression of the three hydrolase genes in our project.<br> </p>
+
In our sender-receiver circuit, we use three hydrolases'' gusA'' , ''aes'' and ''nagZ''. Hence, three hydrolase genes were knocked out of ''E. coli'' strain MG1655. The ''gusA'' hydrolase was knocked out by a scarless deletion scheme that left no scar sequences after the deletion method (1). The subsequent deletions of ''aes'' and ''nagZ'' was carried out by the P1 phage transduction by using deletion strain from the Keio collection (2). Thus we were able to use this strain MG1655&#9651;''gusA''&#9651;''aes''&#9651;''nagZ'' knocked out of expression of the three hydrolase genes in our project.<br> </p>
The triple mutant is used for the sender cells which are made to constitutively express ''nagZ''. In the receiver cells, the hydrolases aes and ''gusA'' are expressed under the control of OHHL induced pluxR promoters.
The triple mutant is used for the sender cells which are made to constitutively express ''nagZ''. In the receiver cells, the hydrolases aes and ''gusA'' are expressed under the control of OHHL induced pluxR promoters.
Line 11: Line 11:
<h1>References</h1>
<h1>References</h1>
-
1. Martinez-Garcia .E, de Lorenzo .V. 2012. Transposon based and plasmid based genetic tools for editing genomes of gram-negative bacteria. Methods in Molecular Biology. 813:267-283.doi: 10.1007/978-1-61779-412-4_16. <br>
+
(1) Martinez-Garcia .E, de Lorenzo .V. 2012. Transposon based and plasmid based genetic tools for editing genomes of gram-negative bacteria. Methods in Molecular Biology. 813:267-283.doi: 10.1007/978-1-61779-412-4_16. <br>
-
2. Thomason L.C., Costantino .N, Court .D .L, 2007. ''E. coli'' Genome Manipulation by P1 Transduction. Current Protocols in Molecular Biology.1.17.1-1.17.8.
+
(2) Thomason L.C., Costantino .N, Court .D .L, 2007. ''E. coli'' Genome Manipulation by P1 Transduction. Current Protocols in Molecular Biology.1.17.1-1.17.8.
<br clear="all"/>
<br clear="all"/>
{{:Team:ETH_Zurich/templates/footer}}
{{:Team:ETH_Zurich/templates/footer}}

Revision as of 17:35, 4 October 2013

Header2.png
80px-Eth igem logo.png

Triple knockout strain

In order to use the orthogonal hydrolases as our reporter system in the sender-receiver set-up, we needed to use a strain of E. coli where the expression of native hydrolase genes were knocked out. This is to prevent background hydrolysis of hydrolases.
In our sender-receiver circuit, we use three hydrolases gusA , aes and nagZ. Hence, three hydrolase genes were knocked out of E. coli strain MG1655. The gusA hydrolase was knocked out by a scarless deletion scheme that left no scar sequences after the deletion method (1). The subsequent deletions of aes and nagZ was carried out by the P1 phage transduction by using deletion strain from the Keio collection (2). Thus we were able to use this strain MG1655△gusAaesnagZ knocked out of expression of the three hydrolase genes in our project.

The triple mutant is used for the sender cells which are made to constitutively express nagZ. In the receiver cells, the hydrolases aes and gusA are expressed under the control of OHHL induced pluxR promoters.

References

(1) Martinez-Garcia .E, de Lorenzo .V. 2012. Transposon based and plasmid based genetic tools for editing genomes of gram-negative bacteria. Methods in Molecular Biology. 813:267-283.doi: 10.1007/978-1-61779-412-4_16.
(2) Thomason L.C., Costantino .N, Court .D .L, 2007. E. coli Genome Manipulation by P1 Transduction. Current Protocols in Molecular Biology.1.17.1-1.17.8.