Team:Freiburg bioware

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  class="art-PostHeader">Welcome</span> </h2>
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<big><font size="5">Team Freiburg Bioware</font></big>
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<h1>Team Freiburg Bioware</h1>
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<br>
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<br />
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The first German team ever to participate in iGEM is back again and
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<p>The first German team ever to participate in iGEM is back
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again and
after last year's second place we're highly motivated &nbsp;to make
after last year's second place we're highly motivated &nbsp;to make
some good piece of synthetic biology in 2009. In this year we want to
some good piece of synthetic biology in 2009. In this year we want to
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<br />
<br />
We're looking forward to meeting you on this year's jamboree!<br />
We're looking forward to meeting you on this year's jamboree!<br />
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<h2 class="art-PostHeaderIcon-wrapper"> &nbsp;Project
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Summary<span class="art-PostHeader"></span> </h2>
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Universal Endonuclease &ndash; Cutting Edge Technology</b>
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<p><b>Universal Endonuclease – Cutting Edge Technology</b></p>
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<p>Gene technology is driven by the use of restriction
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<p>Gene technology is driven by the use of restriction endonucleases. Yet, constraints of limited sequence length and variation recognized by available restriction enzymes pose a major roadblock for synthetic biology. We developed the basis for universal restriction enzymes, primarily for routine cloning but also with potential for in vivo applications. We use a nucleotide cleavage domain fused to a binding domain, which recognizes a programmable adapter that mediates binding to DNA and thus cleavage. As adapter we use readily available modified oligonucleotides, as binding domain anticalins and as cleavage domain FokI moieties engineered for heterodimerization and activity. For cloning, this universal enzyme has merely to be mixed with the sequence specific oligonucleotide and the target DNA. Binding and release are addressed with thermocycling. Additionally, we provide concepts for in vivo applications by external adapter delivery, activity regulation by photo-switching, as well as for modifying an argonaute protein towards a DNA endonuclease.
+
endonucleases.
 +
Yet, constraints of limited sequence length and variation recognized by
 +
available restriction enzymes pose a major roadblock for synthetic
 +
biology. We developed the basis for universal restriction enzymes,
 +
primarily for routine cloning but also with potential for in vivo
 +
applications. We use a nucleotide cleavage domain fused to a binding
 +
domain, which recognizes a programmable adapter that mediates binding
 +
to DNA and thus cleavage. As adapter we use readily available modified
 +
oligonucleotides, as binding domain anticalins and as cleavage domain
 +
FokI moieties engineered for heterodimerization and activity. For
 +
cloning, this universal enzyme has merely to be mixed with the sequence
 +
specific oligonucleotide and the target DNA. Binding and release are
 +
addressed with thermocycling. Additionally, we provide concepts for in
 +
vivo applications by external adapter delivery, activity regulation by
 +
photo-switching, as well as for modifying an argonaute protein towards
 +
a DNA endonuclease.
</p>
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<p><a href="https://2009.igem.org/Team:Freiburg_bioware/Team"><span
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alt="The Team" src="https://static.igem.org/mediawiki/2009/f/f6/Freiburg09_Team.gif" /></b></p>
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<p><b>The Team</b><br />
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  style="border: 0px solid ; width: 138px; height: 40px;"
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This year our team consists of 18 undergraduate students and 4 advisors.<br />
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alt="Team"
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<a href="javascript:void(0)">Read more...</a></p>
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  src="https://static.igem.org/mediawiki/2009/f/f6/Freiburg09_Team.gif" /></span></a><br />
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<p></p>
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<b>The Team</b><br />
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In 2009 our team consists of &nbsp;14 undergraduates and 4 advisors.<br />
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  style="width: 147px; height: 49px;" alt="bioss"
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<a href="https://2009.igem.org/Team:Freiburg_bioware/Team">Read
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  src="https://static.igem.org/mediawiki/2009/3/34/Freiburg09_Bioss_portlet.jpg" /></span>
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<p><b>Bioss</b><br />
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We want to thank our main sponsor Bioss for supporting our project.<br />
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<a target="_blank" href="http://www.bioss.uni-freiburg.de">Read
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more...</a></p>
more...</a></p>
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<p><span style="font-weight: bold;"><a
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alt="bioss"
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src="https://static.igem.org/mediawiki/2009/3/34/Freiburg09_Bioss_portlet.jpg" /></a><br />
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Bioss</span><br />
 +
We want to thank our main sponsor Bioss for supporting our project.<br />
 +
<a href="http://www.bioss.uni-freiburg.de">Read more...</a></p>
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Revision as of 13:39, 4 October 2009

Artisteer

an image

Team Freiburg Bioware


The first German team ever to participate in iGEM is back again and after last year's second place we're highly motivated  to make some good piece of synthetic biology in 2009. In this year we want to create an universal restriction enzyme to facilitate labwork and enable new techniques.

We're looking forward to meeting you on this year's jamboree!



Universal Endonuclease – Cutting Edge Technology

Gene technology is driven by the use of restriction endonucleases. Yet, constraints of limited sequence length and variation recognized by available restriction enzymes pose a major roadblock for synthetic biology. We developed the basis for universal restriction enzymes, primarily for routine cloning but also with potential for in vivo applications. We use a nucleotide cleavage domain fused to a binding domain, which recognizes a programmable adapter that mediates binding to DNA and thus cleavage. As adapter we use readily available modified oligonucleotides, as binding domain anticalins and as cleavage domain FokI moieties engineered for heterodimerization and activity. For cloning, this universal enzyme has merely to be mixed with the sequence specific oligonucleotide and the target DNA. Binding and release are addressed with thermocycling. Additionally, we provide concepts for in vivo applications by external adapter delivery, activity regulation by photo-switching, as well as for modifying an argonaute protein towards a DNA endonuclease.

FREiGEM 2009

Team
The Team
In 2009 our team consists of  14 undergraduates and 4 advisors.
Read more...

bioss
Bioss

We want to thank our main sponsor Bioss for supporting our project.
Read more...

Visitors