Difference between revisions of "Team:CCU Taiwan/Results"

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             <h2>Conjugations of Primary Amines to the Glass Fiber Membranes</h2>
 
             <h2>Conjugations of Primary Amines to the Glass Fiber Membranes</h2>
             <p>We expressed green fluorescent protein (GFP) as a mock E protein to show that that after modification, the glass fiber membrane can bind to the primary amines (side-chain amines) from a peptide or protein. We appreciate Mingdao iGEM 2020, who generously provided us with a plasmid containing the green fluorescent protein gene (GFPmut1, BBa_K1159311). The modified glass fiber membranes were immersed in GFP supernatant from the culture medium for 30 mins to form amide bonds. To verify that the experiments work, we measured the intensity of the fluorescence from GFP using a Synergy H1 Hybrid Multi-Mode Microplate Reader (also provided by Mingdao iGEM 2020). The intensity of membrane reaction with 0.5x and 1x GFP supernatant are shown in Figure 17(a) and 17(b), respectively. We carefully washed the membranes with double-distilled water after the reaction. The intensity was about twice as strong in the 1x supernatant as the 0.5x one, suggesting the conjugation experiments were successful. We also performed the same experiment with non-modified glass fiber membranes as a control, and the intensity of fluorescence is within the range of measurement error (Figure 17(c)).</p>
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             <p>We expressed green fluorescent protein (GFP) as a mock E protein to show that that after modification, the glass fiber membrane can bind to the primary amines (side-chain amines) from a peptide or protein. We appreciate Mingdao iGEM 2020, who generously provided us with a plasmid containing the green fluorescent protein gene (GFPmut1, BBa_K1159311). The modified glass fiber membranes were immersed in GFP supernatant from the culture medium for 30 mins to form amide bonds. To verify that the experiments work, we measured the intensity of the fluorescence from GFP using a Synergy H1 Hybrid Multi-Mode Microplate Reader (also provided by Mingdao iGEM 2020). The intensity of membrane reaction with 0.5x and 1x GFP supernatant are shown in Figure 17. We carefully washed the membranes with double-distilled water after the reaction. The intensity was about twice as strong in the 1x supernatant as the 0.5x one, suggesting the conjugation experiments were successful. We also performed the same experiment with non-modified glass fiber membranes as a control, and the intensity of fluorescence is within the range of measurement error.</p>
 
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                 <img width="70%" src="https://static.igem.org/mediawiki/2020/c/c6/T--CCU_Taiwan--Results_dl1.png">
 
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                 <p>Figure 17. Fluorescence from (a) modified glass fiber membranes reacting with 1x GFP stock, (b) modified glass fiber membranes reacting with 0.5x GFP stock, and (c) non-modified glass fiber membranes.</p>
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                 <p>Figure 17. Fluorescence from modified glass fiber membranes reacting with 1x GFP stock, modified glass fiber membranes reacting with 0.5x GFP stock, and non-modified glass fiber membranes (control).</p>
 
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                 <img width="70%" src="https://static.igem.org/mediawiki/2020/3/38/T--CCU_Taiwan--Results_dl2.png">
 
                 <img width="70%" src="https://static.igem.org/mediawiki/2020/3/38/T--CCU_Taiwan--Results_dl2.png">
                 <p>Figure 18. The fluorescence spectra of DNA conjugated glass fiber membrane (blue), the control experiment (red), in which DNAs react with non-modified membranes, and the empty well (gray). The spectra were obtained at an excitation of 320 nm.</p>
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                 <p>Figure 18. The fluorescence spectra of DNA conjugated glass fiber membrane (blue), the control experiment (red), in which DNAs react with non-modified membranes, and the empty well (yellow). The spectra were obtained at an excitation of 320 nm.</p>
 
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Revision as of 14:04, 27 October 2020

Results