Difference between revisions of "Team:Virginia/nucleic acids"

 
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             Index:
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         <div>Plasmids and Sequences</div>
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          <svg class="download" fill="none" stroke="none" stroke-linecap="square" stroke-miterlimit="10" version="1.1" viewBox="0.0 0.0 210.41207349081364 277.503937007874" xmlns="http://www.w3.org/2000/svg" xmlns:xlink="http://www.w3.org/1999/xlink"><clipPath id="p.0"><path clip-rule="nonzero" d="m0 0l210.41208 0l0 277.50394l-210.41208 0l0 -277.50394z"></path></clipPath><g clip-path="url(#p.0)"><path d="m0 0l210.41208 0l0 277.50394l-210.41208 0z" fill="#000000" fill-opacity="0.0" fill-rule="evenodd"></path><path d="m85.520996 23.346798l0 0c0 -10.871748 8.813293 -19.68504 19.685043 -19.68504l0 0l0 0c5.2207947 0 10.22776 2.0739536 13.919418 5.765615c3.6916656 3.691661 5.7656174 8.6986265 5.7656174 13.919425l0 164.85039c0 10.87175 -8.813293 19.685043 -19.685036 19.685043l0 0l0 0c-10.87175 0 -19.685043 -8.813293 -19.685043 -19.685043z" fill="#3b3838" fill-rule="evenodd"></path><path d="m40.520252 130.18616l0 0c-7.6748734 -6.4925003 -19.163412 -5.537056 -25.660366 2.1340485l0 0l0 0c-3.1199484 3.683792 -4.648011 8.455261 -4.2480326 13.264709c0.3999796 4.8094635 2.6952362 9.262955 6.3808403 12.380768l75.45092 63.82715c7.6748734 6.492508 19.163414 5.5370636 25.66037 -2.1340485l0 0l0 0c6.496956 -7.671097 5.542061 -19.15297 -2.1328125 -25.645477z" fill="#3b3838" fill-rule="evenodd"></path><path d="m192.26115 243.73228l0 0c8.314713 0 15.055115 6.740402 15.055115 15.05513l0 0l0 0c0 3.992859 -1.5861511 7.822174 -4.4095306 10.645569c-2.8233948 2.8233643 -6.652725 4.409546 -10.645584 4.409546l-174.11023 0c-8.314713 0 -15.055119 -6.7404175 -15.055119 -15.055115l0 0l0 0c0 -8.314728 6.740406 -15.05513 15.055119 -15.05513z" fill="#3b3838" fill-rule="evenodd"></path><path d="m169.89232 130.18658l0 0c7.674698 -6.4927216 19.163086 -5.537445 25.660034 2.133667l0 0l0 0c3.1199493 3.683792 4.648056 8.455292 4.2481384 13.264816c-0.3999176 4.80954 -2.6950989 9.263123 -6.380615 12.3810425l-75.48306 63.85788c-7.6746902 6.4927216 -19.163086 5.537445 -25.660042 -2.133667l0 0l0 0c-6.496956 -7.671097 -5.5422134 -19.153152 2.1324844 -25.645859z" fill="#3b3838" fill-rule="evenodd"></path></g></svg>
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             Please select a sequence from the table below
 
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            <div>General Template Page</div>
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      <br/><br/><br/><br/>
          <div class="sectionTitle" id="Section 1">Section 1</div>
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                The lack of a versatile and reliable way to improve metabolic flux channeling, pathway orthogonality, and product yields is a major impediment to the expanded utilization of biosynthesis for the production of drugs and industrially valuable chemicals. Manifold, a platform technology that addresses this problem, consists of <div class="dict">bacterial microcompartments<span><img src="https://upload.wikimedia.org/wikipedia/commons/thumb/2/25/Carboxysome_and_bacterial_microcompartments.jpg/800px-Carboxysome_and_bacterial_microcompartments.jpg"/>Bacterial microcompartments (BMCs) are organelle-like structures, consisting of a protein shell that encloses enzymes and other proteins. BMCs are typically about 40–200 nanometers in diameter and are entirely made of proteins. The shell functions like a membrane, as it is selectively permeable.</span></div> (BMCs) with encapsulated dsDNA scaffolds <div class="ref">[1]<span>Elbaz, J., Yin, P., &amp; Voigt, C. A. (2016). Genetic encoding of DNA nanostructures and their self-assembly in living bacteria. Nature communications, 7(1), 1-11.</span></div> that sequester and spatially organize, at fixed concentrations, biosynthetic enzymes presented as zinc-finger fusion proteins. Here we deliver the designs for an E. coli cell capable of synthesizing resveratrol using the Manifold platform. The Manifold platform will help lower costs and expand the applications of chemical biosynthesis. The lack of a versatile and reliable way to improve metabolic flux channeling, pathway orthogonality, and product yields is a major impediment to the expanded utilization of biosynthesis for the production of drugs and industrially valuable chemicals. Manifold, a platform technology that addresses this problem, consists of bacterial microcompartments (BMCs) with encapsulated dsDNA scaffolds that sequester and spatially organize, at fixed concentrations, biosynthetic enzymes presented as zinc-finger fusion proteins. Here we deliver the designs for an E. coli cell capable of synthesizing resveratrol using the Manifold platform. The Manifold platform will help lower costs and expand the applications of chemical biosynthesis.
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          <div class="sectionTitle" id="Section 2">Section 2</div>
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              The invention consists of a protein shell comprising one or more proteins, one or more nucleic acid scaffolds of which there can be multiple copies, anabolic and/or catabolic enzymes specific to the desired biosynthesis pathway each containing a nucleic acid binding domain, recognition sequences for the utilized nucleic acid binding domains, nucleic acid spacers, and a linkage between the nucleic acid scaffolds and the protein shell. The protein shell (10) can take the form of any closed or open surface that comprises one or more repeating protein units (12). Examples of valid shells include bacterial microcompartments such as the Pdu, Eut, and carboxysome microcompartments, as well as modified,  but not necessarily closed, surfaces composed of mutated versions of these microcompartment shell proteins. The nucleic acid scaffolds (18) comprise multiple recognition sequences (22) and spacers (32) and can be made from any form of nucleic acid, including: deoxyribonucleic acid, ribonucleic acid, and synthetic nucleic acids such as xeno nucleic acids and peptide nucleic acids among others. These scaffolds are attached to the protein shell. The pathway enzymes are biological proteins whose exact sequences are dependent on the given use case of the invention, but which all contain a nucleic acid binding domain either internal to their structure, or at their N or C terminus.
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              <b>Fig 1.</b> Figure taken from iGEM Tainan 2019 for demo purposes. Notice how the figure is much longer than it is wide, and two images are coupled together to achive this. Try to do that as well so it looks good.
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              Additionally, protein linkers are usually present between this nucleic acid binding domain and the enzyme structure to prevent inhibition of enzyme activity. However the exact linker(s) used,  if any, is(are) also dependent on the specific use case of the invention. These pathway enzymes are attached to the nucleic acid scaffolds via their nucleic acid binding domains. The nucleic acid recognition sequences (22) are unique or semi-unique sequences of nucleic acid monomers on the nucleic acid scaffolds to which the utilized nucleic acid binding domains have some degree of molecular complementarity. These nucleic recognition sequences comprise most of the scaffold and mark the locations to which the DNA binding domains of the pathway enzymes attach to the scaffolds. The nucleic acid spacers (32) are relatively short sequences of nucleic acid monomers that are also present on the nucleic acid scaffolds, between the recognition sequences. The linkage between the nucleic acid scaffolds (18) and protein shell (10) provides a means by which the nucleic acid scaffolds are bound to the protein shell through direct or multi-molecule complementarity. This linkage is found between the nucleic acid scaffolds and the protein shell. One example is through the addition of a nucleic acid binding domain (24) to one or more of the shell proteins forming a nucleic acid binding domain, shell protein fusion (14). Like the pathway enzymes, this nucleic acid binding-domain can be either internal to the shell protein structure or at its N or C terminus, where the exact placement depends on the shell protein being utilized. Alternatively, one or more intermediate proteins can be used to adhere the nucleic acid scaffolds to the shell, where the region of the protein interacting with the shell binds the shell via protein-protein complementarity (28) with a given shell protein, and the region of the protein interacting with the nucleic acid scaffold binds another recognition sequence on the nucleic acid scaffold through another nucleic acid binding domain (30). This forms a shell protein binding, nucleic acid domain fusion (26).<br/><br/><br/>
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Latest revision as of 03:31, 28 October 2020

Manifold

Plasmids and Sequences
Please select a sequence from the table below