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| − | <button class="tablinks" onclick="openTab(event, 'Key Achievement')" id="defaultOpen">Key Achievements</button> | + | <button class="tablinks" onclick="openTab(event, 'Key Achievements')" id="defaultOpen">Key Achievements</button> |
| | <button class="tablinks2" onclick="openTab(event, 'biology')">Biology</button> | | <button class="tablinks2" onclick="openTab(event, 'biology')">Biology</button> |
| | <button class="tablinks3" onclick="openTab(event, 'engineering')">Engineering</button> | | <button class="tablinks3" onclick="openTab(event, 'engineering')">Engineering</button> |
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| − | <h2>Results obtained clearly shows that PCR is sensitive up to 0.1 ng/µl, lowest concentration tested, for all three plasmids tested. Visually, all bands appear to be similarly thick, which shows that, despite the changes in concentration, PCR amplified each DNA in a similar manner. | + | <h2>Results obtained clearly shows that PCR is sensitive up to 0.1 ng/µl, lowest concentration tested, for all three plasmids tested. Visually, all bands appear to be similarly thick, which shows that, despite the changes in concentration, PCR amplified each DNA in a similar manner. |
| | </h2> | | </h2> |
| − | <h2>Published research has reported PCR to be sensitive up to 3 pg/µl (6). This shows that PCR is a sensitive technique that is able to amplify DNA even at low DNA concentrations. | + | <h2>Published research has reported PCR to be sensitive up to 3 pg/µl (6). This shows that PCR is a sensitive technique that is able to amplify DNA even at low DNA concentrations. |
| | </h2> | | </h2> |
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| | <h5><i>Specificity (lmo0773, invA and gbpA)</i></h5> | | <h5><i>Specificity (lmo0773, invA and gbpA)</i></h5> |
| − | <h2>Two sets of experiments were carried out to test the specificity of each amplification technique used. In the first set of experiments, the genes used were kept constant, while the primers were varied, while in the second set, the primers were kept constant while the genes were varied. As can be seen in the figure below, PCR was not found to be specific, as the DNA for a specific gene was amplified by primers designed for another gene as well as with primers specific for that gene. | + | <h2>Two sets of experiments were carried out to test the specificity of each amplification technique used. In the first set of experiments, the genes used were kept constant, while the primers were varied, while in the second set, the primers were kept constant while the genes were varied. As can be seen in the figure below, PCR was not found to be specific, as the DNA for a specific gene was amplified by primers designed for another gene as well as with primers specific for that gene. |
| | </h2> | | </h2> |
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| | <img src="https://static.igem.org/mediawiki/2018/4/48/T--NYU_Abu_Dhabi--Results--Biology_2.JPG"class="center"> | | <img src="https://static.igem.org/mediawiki/2018/4/48/T--NYU_Abu_Dhabi--Results--Biology_2.JPG"class="center"> |
| − | <h2><center><i>Figure 2. Agarose gels (1%) corresponding to PCR specificity reactions carried out on three different genes (a) lmo0733, (b) invA and (c) hipO. The first set of reactions for each gene is done by keeping the gene constant while varying the primers, while the second set of reactions are carried out by varying the gene used while keeping the primers constant. | + | <h2><center><i>Figure 2. Agarose gels (1%) corresponding to PCR specificity reactions carried out on three different genes (a) lmo0733, (b) invA and (c) hipO. The first set of reactions for each gene is done by keeping the gene constant while varying the primers, while the second set of reactions are carried out by varying the gene used while keeping the primers constant. |
| | </i></center></h2> | | </i></center></h2> |
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| | <h4><ins>LAMP</ins></h4> | | <h4><ins>LAMP</ins></h4> |
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| − | <h2>Loop-mediated isothermal amplification was performed using primers designed with <a href="http://primerexplorer.jp/lampv5e/index.html">PrimerExplorer</a> for lmo0733, invA, hipO and gbpA. The reaction was run using miniprep DNA and transformed E. Coli colonies to assess if amplification can occur with whole cells. The Agarose gel (1%) shows amplification in all the lanes with miniprep DNA. | + | <h2>Loop-mediated isothermal amplification was performed using primers designed with <a href="http://primerexplorer.jp/lampv5e/index.html">PrimerExplorer</a> for lmo0733, invA, hipO and gbpA. The reaction was run using miniprep DNA and transformed E. Coli colonies to assess if amplification can occur with whole cells. The Agarose gel (1%) shows amplification in all the lanes with miniprep DNA. |
| | </h2> | | </h2> |
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| | <h5><i>Colorimetric Test: Real Sample Swab and Amplification</i></h5> | | <h5><i>Colorimetric Test: Real Sample Swab and Amplification</i></h5> |
| − | <h2>To test the working principles of the <i>Pathogene</i> pathogen project, it had to be established that the intra-lab amplification techniques would be effective on real world samples of contaminated food, water, surfaces etc. Two samples of beef were prepared for the purposes of determining the colorimetric visualization of results for LAMP, in particular the use of NEB WarmStart Colorimetric Mastermix. A sample of untreated store-bought beef was prepared alongside a sample of DH5-alpha cells transformed with the lmo0733 gene from <i>Listeria Monocytogenes</i>. Direct swabs were taken from each sample and used in the LAMP reactions. Reactions lacking the target gene appear a bright red colour whereas reaction mixes containing the amplified gene appear salmon to yellow in colour. | + | <h2>To test the working principles of the <i>Pathogene</i> pathogen project, it had to be established that the intra-lab amplification techniques would be effective on real world samples of contaminated food, water, surfaces etc. Two samples of beef were prepared for the purposes of determining the colorimetric visualization of results for LAMP, in particular the use of NEB WarmStart Colorimetric Mastermix. A sample of untreated store-bought beef was prepared alongside a sample of DH5-alpha cells transformed with the lmo0733 gene from <i>Listeria Monocytogenes</i>. Direct swabs were taken from each sample and used in the LAMP reactions. Reactions lacking the target gene appear a bright red colour whereas reaction mixes containing the amplified gene appear salmon to yellow in colour. |
| | </h2> | | </h2> |
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| | <img src="https://static.igem.org/mediawiki/2018/1/14/T--NYU_Abu_Dhabi--Results--Biology_13.JPG"class="center"> | | <img src="https://static.igem.org/mediawiki/2018/1/14/T--NYU_Abu_Dhabi--Results--Biology_13.JPG"class="center"> |
| − | <h2><center><i>Figure 13. The SYBR Green fluorescence of the <i>hipO</i> serial dilutions represented under <b>(a)</b> UV light (365 nm) <b>(b)</b> Blue light <b>(c)</b> under Blue light with overexposure demonstrates. | + | <h2><center><i>Figure 13. The SYBR Green fluorescence of the <i>hipO</i> serial dilutions represented under <b>(a)</b> UV light (365 nm) <b>(b)</b> Blue light <b>(c)</b> under Blue light with overexposure demonstrates. |
| | </i></center></h2> | | </i></center></h2> |
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| | <h5><i>LAMP Specificity (lmo0773, invA and gbpA)</i></h5> | | <h5><i>LAMP Specificity (lmo0773, invA and gbpA)</i></h5> |
| − | <h2>The same two experiments done with PCR were done with LAMP. The results obtained indicate that LAMP is highly specific as every gene was only amplified by its primers and not by any other primers. LAMP was found to be the only completely specific technique out of PCR, LAMP and RPA. | + | <h2>The same two experiments done with PCR were done with LAMP. The results obtained indicate that LAMP is highly specific as every gene was only amplified by its primers and not by any other primers. LAMP was found to be the only completely specific technique out of PCR, LAMP and RPA. |
| | </h2> | | </h2> |
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| | </i></center></h2> | | </i></center></h2> |
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| − | <h2>The reaction volume for RPA was successfully optimized to a total volume of 25 ul. This allowed for economical use of reagents in lab experiments and for use in microfluidic chips. | + | <h2>The reaction volume for RPA was successfully optimized to a total volume of 25 ul. This allowed for economical use of reagents in lab experiments and for use in microfluidic chips. |
| | </h2> | | </h2> |
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| | </i></center></h2> | | </i></center></h2> |
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| − | <h2>The reaction volume for RPA was successfully optimized to a total volume of 10 µl. The agarose gel (3%) shows brighter bands for <i>gbpA</i> and <i>lmo0733</i> compared to <i>invA</i>. This allowed for economical use of reagents in lab experiments and for use in microfluidic chips. | + | <h2>The reaction volume for RPA was successfully optimized to a total volume of 10 µl. The agarose gel (3%) shows brighter bands for <i>gbpA</i> and <i>lmo0733</i> compared to <i>invA</i>. This allowed for economical use of reagents in lab experiments and for use in microfluidic chips. |
| | </h2> | | </h2> |
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| | <h2>Background fluorescence was observed in the negative controls. However, a clear distinction was observed between positive and negative controls. | | <h2>Background fluorescence was observed in the negative controls. However, a clear distinction was observed between positive and negative controls. |
| − | </h2> | + | </h2> |
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| | <img src="https://static.igem.org/mediawiki/2018/a/a2/T--NYU_Abu_Dhabi--Results--Biology_20.JPG"class="center"> | | <img src="https://static.igem.org/mediawiki/2018/a/a2/T--NYU_Abu_Dhabi--Results--Biology_20.JPG"class="center"> |
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| | <h5><i>Specificity</i></h5> | | <h5><i>Specificity</i></h5> |
| − | <h2>The two specificity experiments were done with RPA for the two genes, <i>lmo0733</i> and <i>invA</i>. The results shown in the Figure below, show that RPA is not as specific as LAMP as amplification of a gene with primers designed for another gene does occur. This could be due to the fact that RPA uses the longest primers out of all three techniques, resulting in a higher possibility of having regions of the primers complementary to different genes. | + | <h2>The two specificity experiments were done with RPA for the two genes, <i>lmo0733</i> and <i>invA</i>. The results shown in the Figure below, show that RPA is not as specific as LAMP as amplification of a gene with primers designed for another gene does occur. This could be due to the fact that RPA uses the longest primers out of all three techniques, resulting in a higher possibility of having regions of the primers complementary to different genes. |
| | </h2> | | </h2> |
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| − | <h2>The heating device provides a platform that sustains the designated temperature under which the RPA, LAMP reaction should run. There are three modes for the device: in the first mode, the | + | <h2>The heating device provides a platform that sustains the designated temperature under which the RPA, LAMP reaction should run. There are three modes for the device: in the first mode, the |
| | green LED light lights up, signaling that the power is connected. The 6 blue LED lights that aids visualization will also be on. In the second mode (for RPA reaction), one red LED light turns on, and the heating board heats up to 40° C. In the third mode (for LAMP reaction), two red LED lights turn on and the heating board heats up to 65° C. A temperature sensor is closely attached to the heating board and helps ensure that the temperature is maintained as desired. A power bank that consists of a 9V rechargeable battery is used as the power supply for the device. The user can just connect the power bank to the device for the device to start operating. | | green LED light lights up, signaling that the power is connected. The 6 blue LED lights that aids visualization will also be on. In the second mode (for RPA reaction), one red LED light turns on, and the heating board heats up to 40° C. In the third mode (for LAMP reaction), two red LED lights turn on and the heating board heats up to 65° C. A temperature sensor is closely attached to the heating board and helps ensure that the temperature is maintained as desired. A power bank that consists of a 9V rechargeable battery is used as the power supply for the device. The user can just connect the power bank to the device for the device to start operating. |
| | </h2> | | </h2> |
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| | </i></center></h2> | | </i></center></h2> |
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| − | <h2>Next, the four RPA reactions were carried out in a 3M chip. For one RPA reaction, 29.5µl of re-hydration buffer was added to one tube of dried reaction, along with 2.4µl forward primers, 2,4 µl backward primers, 8.2µl of water, 5µl of DNA, 1µl of 1000X SBYR Green and 2.5µl of Magnesium acetate. The primers were replaced with an equal volume of water for the two negative control reactions. | + | <h2>Next, the four RPA reactions were carried out in a 3M chip. For one RPA reaction, 29.5µl of re-hydration buffer was added to one tube of dried reaction, along with 2.4µl forward primers, 2,4 µl backward primers, 8.2µl of water, 5µl of DNA, 1µl of 1000X SBYR Green and 2.5µl of Magnesium acetate. The primers were replaced with an equal volume of water for the two negative control reactions. |
| | </h2> | | </h2> |
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| | <h7><ins>Heating Device</ins></h7> | | <h7><ins>Heating Device</ins></h7> |
| | <br><br> | | <br><br> |
| − | <h2>The heating device provides a platform that sustains the designated temperature under which the RPA, LAMP reaction should run. There are three modes for the device: in the first mode, the | + | <h2>The heating device provides a platform that sustains the designated temperature under which the RPA, LAMP reaction should run. There are three modes for the device: in the first mode, the |
| − | green LED light lights up, signaling that the power is connected. The 6 blue LED lights that aids visualization will also be on. In the second mode (for RPA reaction), one red LED light turns on, and the heating board heats up to and maintains at approximately 40°C. In the third mode (for LAMP reaction), two red LED lights turn on and the heating board heats up to and maintains at approximately 65°C. A temperature sensor is closely attached to the heating board and helps ensure that the temperature is maintained as desired. | + | green LED light lights up, signaling that the power is connected. The 6 blue LED lights that aids visualization will also be on. In the second mode (for RPA reaction), one red LED light turns on, and the heating board heats up to and maintains at approximately 40°C. In the third mode (for LAMP reaction), two red LED lights turn on and the heating board heats up to and maintains at approximately 65°C. A temperature sensor is closely attached to the heating board and helps ensure that the temperature is maintained as desired. |
| | </h2> | | </h2> |
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| | <h7><ins>Visualization</ins></h7> | | <h7><ins>Visualization</ins></h7> |
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| − | <h2>Ten NEB LAMP reactions were run, five of which were positive controls with both DNA and primers added, while the other five were negative with DNA added but with no primers. The reactions were run in PCR tubes at 65°C for 30 minutes. The completed reactions were then pipetted into the wells of a ten-well PDMS chip, alternating between positive and negative. | + | <h2>Ten NEB LAMP reactions were run, five of which were positive controls with both DNA and primers added, while the other five were negative with DNA added but with no primers. The reactions were run in PCR tubes at 65°C for 30 minutes. The completed reactions were then pipetted into the wells of a ten-well PDMS chip, alternating between positive and negative. |
| | </h2> | | </h2> |
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| − | The objective of this was to ensure that fluorescence could be observed in the PDMS chip under blue light. Moreover, this was done to illustrate the difference in fluorescence between positive and negative controls. | + | The objective of this was to ensure that fluorescence could be observed in the PDMS chip under blue light. Moreover, this was done to illustrate the difference in fluorescence between positive and negative controls. |
| | </h2> | | </h2> |
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| | </i></center></h2> | | </i></center></h2> |
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| − | <h2>The same process was repeated using 3M chips. 10 reactions, 5 positive and 5 negative were carried out in PCR tubes and pipetted into a 3M chip to check visualization. The results are shown in Figure shown below, as visualized under blue light. | + | <h2>The same process was repeated using 3M chips. 10 reactions, 5 positive and 5 negative were carried out in PCR tubes and pipetted into a 3M chip to check visualization. The results are shown in Figure shown below, as visualized under blue light. |
| | </h2> | | </h2> |
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| | <div class="dropdown-menu" aria-labelledby="navbarDropdown"> | | <div class="dropdown-menu" aria-labelledby="navbarDropdown"> |
| | <a class="dropdown-item" href="https://2018.igem.org/Team:NYU_Abu_Dhabi/Description">Description</a> | | <a class="dropdown-item" href="https://2018.igem.org/Team:NYU_Abu_Dhabi/Description">Description</a> |
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| | <a class="dropdown-item" href="https://2018.igem.org/Team:NYU_Abu_Dhabi/Demonstrate">Demonstration</a> | | <a class="dropdown-item" href="https://2018.igem.org/Team:NYU_Abu_Dhabi/Demonstrate">Demonstration</a> |
| | <a class="dropdown-item" href="https://2018.igem.org/Team:NYU_Abu_Dhabi/Results">Results</a> | | <a class="dropdown-item" href="https://2018.igem.org/Team:NYU_Abu_Dhabi/Results">Results</a> |
