Index-2.html

From 2012.igem.org

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             <p class="p1">This year, we accomplished getting pgapz alpha digested to retrieve the part we needed. The vector was gel isolated through gel excision. Following the isolation, the vector was ligated as well as the MCS linker. We then transformed the host into ecoli and colonies were picked. Mini preps were analyzed and a digest was done of pGap. Purification and linearization was done with EcoRI and Pst. We were then able to ligate RFP and pGapz alpha. The vector will then be transformed into Pichia. Future possibilities would include expressing a protein that can be useful as well as advancing uses of Pichia over Ecoli because of its ability to perform post translational modifications which is important in eukaryots. Also, we would like to work on the pPik 9 because of it being inducible. </p>
             <p class="p1">This year, we accomplished getting pgapz alpha digested to retrieve the part we needed. The vector was gel isolated through gel excision. Following the isolation, the vector was ligated as well as the MCS linker. We then transformed the host into ecoli and colonies were picked. Mini preps were analyzed and a digest was done of pGap. Purification and linearization was done with EcoRI and Pst. We were then able to ligate RFP and pGapz alpha. The vector will then be transformed into Pichia. Future possibilities would include expressing a protein that can be useful as well as advancing uses of Pichia over Ecoli because of its ability to perform post translational modifications which is important in eukaryots. Also, we would like to work on the pPik 9 because of it being inducible. </p>
             <h6 class="clr-9 p2">Agro</h6>
             <h6 class="clr-9 p2">Agro</h6>
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             <p class="p1">Agrobacterium tumefaciens is a gram-negative soil bacterium that is the causative agent of Crown-Gall disease in both dicotyledon and monocotyledon plants. The tumors caused by Crown-Gall disease contain segments from the Tumor Inducing (Ti) Plasmid known as the TDNA, which completely integrates with the host's genome. In genetic re-engineering, a binary vector system is used because the Ti plasmid is over 250 kb and is too large to easily manipulate. Binary vectors consist of small plasmids with a cloning site and a selectable maker gene between the left and right border of the TDNA making it easier to manipulate. Modification of a gene of interest and insertion into the Ti Plasmid of A. tumefaciens allows exploitation of the natural ability to A. tumefaciens to transmit DNA. Creation of a binary system containing a gene of interest could potentially be advantageous to both plants and animals.</p>
+
             <p class="p1">Integration of the modified Ti plasmid into plants begins with first creation of a binary system containing a gene of interest could potentially be advantageous to both plants and animals. These modified plasmids will remove the ability of Agrobacterium to produce tumors and introduce genes that could potentially give plants the capability to live and prosper in environments that these plants typically could not live in.
 +
Our goal was to re-engineer the Ti Plasmid by introducing genes that code for red fluorescent protein (RFP) and a advantageous gene of interest. DNA containing pORE Expression Series Vector (20I) and RFP was hydrolyzed and extracted from the 2012 iGEM kit plate. Electrocompetent Escherichia coli cells were first used to manipulate the plasmid due to the relative ease to grow and cultivate E. coli. The RFP gene was successfully inserted into the plasmid of E. coli using electroporation (Figure 3). The transformed E.coli cells were allowed to incubate for 24 hours @ 37ºC (Figure 4). After incubation, plasmid extraction was done using QIAprep Miniprep to remove the plasmid and quantify the purity of their DNA. Restriction digestion using the restriction enzymes EcoR1 and Pst to visually analyze how big the RFP fragment sizes are.
 +
  Due to the time it takes for the plants to grow, verification of the function of our plasmid remains untested. Promptly after sufficient amount of growth occurs, our A. tumefaciens carrying our modified plasmid will trans-infect the Brassica Rapa plants. A positive result will be seen if RFP is expressed in the plants. Further testing will also be done to check how well the plants re-uptake the Ti plasmid.
 +
We recently started working with the pPZP500 cloning vector but as of now we do not have any data collected on this vector. The vector was provided to us by Dr. Holger Bohlmann, and Ali Muhammad Amjad from the University of Natural Resources and Applied Life Sciences in Vienna. </p>
            
            
            
            

Revision as of 23:43, 3 October 2012

Project

Pichia

This year, we accomplished getting pgapz alpha digested to retrieve the part we needed. The vector was gel isolated through gel excision. Following the isolation, the vector was ligated as well as the MCS linker. We then transformed the host into ecoli and colonies were picked. Mini preps were analyzed and a digest was done of pGap. Purification and linearization was done with EcoRI and Pst. We were then able to ligate RFP and pGapz alpha. The vector will then be transformed into Pichia. Future possibilities would include expressing a protein that can be useful as well as advancing uses of Pichia over Ecoli because of its ability to perform post translational modifications which is important in eukaryots. Also, we would like to work on the pPik 9 because of it being inducible.

Agro

Integration of the modified Ti plasmid into plants begins with first creation of a binary system containing a gene of interest could potentially be advantageous to both plants and animals. These modified plasmids will remove the ability of Agrobacterium to produce tumors and introduce genes that could potentially give plants the capability to live and prosper in environments that these plants typically could not live in. Our goal was to re-engineer the Ti Plasmid by introducing genes that code for red fluorescent protein (RFP) and a advantageous gene of interest. DNA containing pORE Expression Series Vector (20I) and RFP was hydrolyzed and extracted from the 2012 iGEM kit plate. Electrocompetent Escherichia coli cells were first used to manipulate the plasmid due to the relative ease to grow and cultivate E. coli. The RFP gene was successfully inserted into the plasmid of E. coli using electroporation (Figure 3). The transformed E.coli cells were allowed to incubate for 24 hours @ 37ºC (Figure 4). After incubation, plasmid extraction was done using QIAprep Miniprep to remove the plasmid and quantify the purity of their DNA. Restriction digestion using the restriction enzymes EcoR1 and Pst to visually analyze how big the RFP fragment sizes are. Due to the time it takes for the plants to grow, verification of the function of our plasmid remains untested. Promptly after sufficient amount of growth occurs, our A. tumefaciens carrying our modified plasmid will trans-infect the Brassica Rapa plants. A positive result will be seen if RFP is expressed in the plants. Further testing will also be done to check how well the plants re-uptake the Ti plasmid. We recently started working with the pPZP500 cloning vector but as of now we do not have any data collected on this vector. The vector was provided to us by Dr. Holger Bohlmann, and Ali Muhammad Amjad from the University of Natural Resources and Applied Life Sciences in Vienna.

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