Team:XMU-China/Project PSystem

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<!--P system-->
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<img id="Project_Psystem_title" class="Project_title" src="https://static.igem.org/mediawiki/2014/4/48/Xmu_project_P_system_zwei.png"/>
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     <span style="font-family: Times New Roman;text-align:center">A reasonable explanation of misfolding GFP under QS oscillation</span>
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     <span style="font-size: 27px; font-weight: 700;">A REASONABLE EXPLANATION OF MISFOLDING GFP UNDER QS OSCILLATION</span>
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     <span style="font-family: Times New Roman;">In</span><span style="font-family: Times New Roman;"> the project </span><span style="font-family: Times New Roman;">of</span><span style="font-family: Times New Roman;"> iGEM</span><span style="font-family: Times New Roman;">13 XMU-China, they</span><span style="font-family: Times New Roman;"> can’t get expected oscillation. H</span><span style="font-family: Times New Roman;">owever</span><span style="font-family: Times New Roman;">,</span><span style="font-family: Times New Roman;"> </span><span style="font-family: Times New Roman;">this year</span><span style="font-family: Times New Roman;"> </span><span style="font-family: Times New Roman;">iGEM14 XMU-China</span><span style="font-family: Times New Roman;"> further </span><span style="font-family: Times New Roman;">investigate the reason of abnormal oscillation. We further review</span><span style="font-family: Times New Roman;"> SDS-PAGE analysis to confirm </span><span style="font-family: Times New Roman;">the circuit </span><span style="font-family: Times New Roman;">at</span><span style="font-family: Times New Roman;"> protein leve</span><span style="font-family: Times New Roman;">l. The SDS-PAGE data is shown in </span><span style="font-family: Times New Roman; font-weight: 700;">Figure 1</span><span style="font-family: Times New Roman;">.</span><span style="font-family: Times New Roman;"> Based on that, we make a reasonable assumption that the unexpected behavior of the LuxR Promoter lead</span><span style="font-family: Times New Roman;">s</span><span style="font-family: Times New Roman;"> to the misfolding proteins </span><span style="font-family: Times New Roman;">hence the</span><span style="font-family: Times New Roman;"> abnormal oscillation.</span>
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     <span style="font-family: Arial,sans-serif;">In</span><span style="font-family: Arial,sans-serif;"> the project </span><a href="https://2013.igem.org/Team:XMU-China" target="_blank">iGEM13_XMU-China</a>, they<span style="font-family: Arial,sans-serif;"> couldn't get expected oscillation. However</span><span style="font-family: Arial,sans-serif;">,</span><span style="font-family: Arial,sans-serif;"> </span><span style="font-family: Arial,sans-serif;">this year</span> <a href="https://2014.igem.org/Team:XMU-China" target="_blank">iGEM14_XMU-China</a><span style="font-family: Arial,sans-serif;"> further </span><span style="font-family: Arial,sans-serif;">investigated the reason of abnormal oscillation. We further reviewed</span><span style="font-family: Arial,sans-serif;"> SDS-PAGE analysis to confirm </span><span style="font-family: Arial,sans-serif;">the circuit </span><span style="font-family: Arial,sans-serif;">at</span><span style="font-family: Arial,sans-serif;"> protein leve</span><span style="font-family: Arial,sans-serif;">l. The SDS-PAGE data is shown in </span><span style="font-family: Arial,sans-serif; font-weight: 700;">Figure 1</span><span style="font-family: Arial,sans-serif;">.</span><span style="font-family: Arial,sans-serif;"> Based on that, we made a reasonable assumption that the unexpected behavior of the LuxR promoter lead</span><span style="font-family: Arial,sans-serif;">s</span><span style="font-family: Arial,sans-serif;"> to the misfolding proteins Hence result in the abnormal oscillation result in the abnormal oscillation.</span>
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                     <img width="612" height="408" style="font-family: Times New Roman;" src="https://static.igem.org/mediawiki/2014/2/22/Xmu_project_p_system01.png"/>
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                     <span style="font-family: Times New Roman; font-weight: 700;">Figure 1</span><span style="font-family: Times New Roman; font-weight: 700;">.</span><span style="font-family: Times New Roman;"> </span><span style="font-family: Times New Roman;">SDS-PAGE analysis of E.</span><span style="font-family: Times New Roman;">coli K strain (</span><span style="font-family: Times New Roman; font-style: italic;">DH5α</span><span style="font-family: Times New Roman;">). </span><span style="font-family: Times New Roman; font-weight: 700;">(a)</span><span style="font-family: Times New Roman;"> Lane 1-2: supernatant and pellet of original </span><span style="font-family: Times New Roman; font-style: italic;">DH5α</span><span style="font-family: Times New Roman;">; Lane 3-4: supernatant and pellet of strain with single plasmid A1 (BBa_K1036003); Lane 5-6: supernatant and pellet of strain with both plasmids A1</span><span style="font-family: Times New Roman;"> </span><span style="font-family: Times New Roman;">(BBa_K1036003) and B</span><span style="font-family: Times New Roman;"> (BBa_K1036000)</span><span style="font-family: Times New Roman;">. The red arrows indicate the </span><span style="font-family: Times New Roman; font-weight: 700;">misfolding</span><span style="font-family: Times New Roman;"> GFP-LVA protein (27.6 kDa) in the precipitation. </span><span style="font-family: Times New Roman; font-weight: 700;">(b)</span><span style="font-family: Times New Roman;"> Lane 1-2: supernatant and pellet of original </span><span style="font-family: Times New Roman; font-style: italic;">BL21</span><span style="font-family: Times New Roman;">; Lane 3-4: supernatant and pellet of strain with single plasmid A1</span><span style="font-family: Times New Roman;"> (BBa_K1036003)</span><span style="font-family: Times New Roman;">; Lane 5-6: supernatant and pellet of strain with both plasmids A1</span><span style="font-family: Times New Roman;"> (BBa_K1036003) </span><span style="font-family: Times New Roman;">and B</span><span style="font-family: Times New Roman;"> (BBa_K1036000)</span><span style="font-family: Times New Roman;">. The blue arrows indicate LuxR (27.5 kDa), GFP-LVA (27.6 kDa) and AiiA-LVA (28.7 kDa) in the supernatant. The orange arrows indicate LuxI-LVA (22.4 kDa) in the supernatant. (The marker of b was not in right position, however, the proteins were confirmed by MALDI-TOF-TOF .)</span>
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                     <span style="font-family: Times New Roman; font-weight: 700;">Figure 1. </span>SDS-PAGE analysis of <em>E. coli</em> K strain (<span style="font-family: Times New Roman;">DH5α</span>). </span><span style="font-family: Times New Roman; font-weight: 700;">(a)</span> Lane 1-2: supernatant and pellet of original </span><span style="font-family: Times New Roman; font-style: ">DH5α</span>; Lane 3-4: supernatant and pellet of strain with single plasmid A1 (<span>BBa_K1036003</span>); Lane 5-6: supernatant and pellet of strain with both plasmids A1</span> </span>(<span>BBa_K1036003</span>) and B</span> (<span>BBa_K1036000</span>)</span>. The red arrows indicate the </span><span style="font-family: Times New Roman; font-weight: 700;">misfolding</span> GFP-LVA protein (27.6 kDa) in the precipitation. </span><span style="font-family: Times New Roman; font-weight: 700;">(b)</span> Lane 1-2: supernatant and pellet of original </span><span style="font-family: Times New Roman; font-style: italic;">BL21</span>; Lane 3-4: supernatant and pellet of strain with single plasmid A1</span> (<span>BBa_K1036003</span>)</span>; Lane 5-6: supernatant and pellet of strain with both plasmids A1</span> (<span>BBa_K1036003</span>) </span>and B</span> (<span>BBa_K1036000</span>)</span>. The blue arrows indicate LuxR (27.5 kDa), GFP-LVA (27.6 kDa) and AiiA-LVA (28.7 kDa) in the supernatant. The orange arrows indicate LuxI-LVA (22.4 kDa) in the supernatant. (The marker of b was not in right position, however, the proteins were confirmed by MALDI-TOF-TOF .)</span>
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     <span style="font-family: Times New Roman;">As the SDS-PAGE show</span><span style="font-family: Times New Roman;">s</span><span style="font-family: Times New Roman;">, a large amount of </span><span style="font-family: Times New Roman;">GFP-LVA and LuxI-LVA </span><span style="font-family: Times New Roman;">appear</span><span style="font-family: Times New Roman;"> in pellet where misfolding proteins often exist. Both protein</span><span style="font-family: Times New Roman;">s</span><span style="font-family: Times New Roman;"> directl</span><span style="font-family: Times New Roman;">y </span><span style="font-family: Times New Roman;">a</span><span style="font-family: Times New Roman;">ffect the oscillation result. </span><span style="font-family: Times New Roman;">And it is critical to find out the reason for misfolding proteins</span><span style="font-family: Times New Roman;">. iGEM14 XMU-China make the following assumption:</span>
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     As the SDS-PAGE shows, a large amount of GFP-LVA and LuxI-LVA appear in pellet where misfolding proteins often exist. Both proteins directly affect the oscillation result. And it is critical to find out the reason for misfolding proteins. <a href="https://2014.igem.org/Team:XMU-China" target="_blank">iGEM14_XMU-China</a> made the following assumption:
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     <span style="font-family: Times New Roman;"> &nbsp; &nbsp;</span>
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     <span style="font-family: Arial,sans-serif;"> &nbsp; &nbsp;</span>
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     <span style="font-family: Times New Roman;">The 2012 published paper</span><span style="font-family: Times New Roman; valign: sup;">[1]</span><span style="font-family: Times New Roman;"> reveals an unexpected behavior of </span><span style="font-family: Times New Roman;">L</span><span style="font-family: Times New Roman;">ux pR</span><span style="font-family: Times New Roman;"> </span><span style="font-family: Times New Roman;">(BBa_R0062).</span><span style="font-family: Times New Roman;"> In the absence of autoinducer 3OC6 (AHL), LuxR binds to Plux</span><span style="font-family: Times New Roman;"> (Lux pR)</span><span style="font-family: Times New Roman;"> and activates backwards transcription (</span><span style="font-family: Times New Roman; font-weight: 700;">Figure 2</span><span style="font-family: Times New Roman;">).</span>
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     The research<sup>[1]</sup> reveals an unexpected behavior of Lux pR (<span>BBa_R0062</span>). In the absence of autoinducer 3OC6 (AHL), LuxR binds to plux (Lux pR) and activates backwards transcription (<strong>Figure 2</strong>).
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                     <img width="540" height="409" style="font-family: Arial,sans-serif;background-color:white;" src="https://static.igem.org/mediawiki/2014/c/c5/Xmu_project_p_system02.png"/>
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                     <span style="font-family: Times New Roman; font-weight: 700;">Figure</span><span style="font-family: Times New Roman; font-weight: 700;"> 2</span><span style="font-family: Times New Roman; font-weight: 700;">.</span><span style="font-family: Times New Roman;"> Relative RFP fluorescence for a control construct designed to measure backwards transcription from </span><span style="font-family: Times New Roman;">Lux pR</span><span style="font-family: Times New Roman;">. Addition of LuxR and 3OC6</span><span style="font-family: Times New Roman;">90 (AHL)</span><span style="font-family: Times New Roman;"> as indicated. Error bars in all panels are one standard deviation.</span>
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                     <span style="font-weight: 700;"><b>Figure 2.</b> Relative RFP fluorescence for a control construct designed to measure backwards transcription from Lux pR. Addition of LuxR and 3OC6 90 (AHL) as indicated. Error bars in all panels are one standard deviation.</span>
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     <span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">The imperfect simplification</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;"> of setting </span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">lux pL</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;"> and </span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">L</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">ux pR</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;"> in the same direction</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">:</span>
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     <strong>The imperfect simplification of setting lux pL and Lux pR in the same direction:&nbsp;</strong>
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     <span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">From the original design by</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">Jeff</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">H</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">asty</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">, Lux pR and Lux pL are </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">set</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> in opposite directions</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> (</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">Figure 3</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">A</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">)</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">.</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">In the absence of AHL</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">, LuxR could activate backward transcription of Lux pR</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> </span><span style="font-family: Times New Roman;">leading to more expression of LuxR which is</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> critical to meet the oscillation conditions. However, present literature don’t consider </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">the backwards transcription which </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">have effect</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> on </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">q</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">uorum sensing oscillation.</span>
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     From the original design by Jeff Hasty, Lux pR and Lux pL were set in opposite directions (<strong>Figure 3A</strong>). In the absence of AHL, LuxR could activate backwards transcription of Lux pR leading to more expression of LuxR which was critical to meet the oscillation conditions. However, present literature did’t consider the backwards transcription which had effect on quorum sensing oscillation.
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                     <span style="font-weight: 700;">A.</span><span style="font-weight: 700;"> </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">Original </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">D</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">esign</span>
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                     <span style="font-weight: 700;">A.</span><span style="font-weight: 700;"> </span><span style="font-family: Arial,sans-serif; font-weight: 400;">Original </span><span style="font-family: Arial,sans-serif; font-weight: 400;">D</span><span style="font-family: Arial,sans-serif; font-weight: 400;">esign</span>
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                     <span style="font-weight: 700;">B.</span><span style="font-weight: 700;"> </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">iGEM13 XMU-China Design</span>
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                     <span style="font-weight: 700;">B.</span><span style="font-weight: 700;"> </span><span style="font-family: Arial,sans-serif; font-weight: 400;"><a href="https://2013.igem.org/Team:XMU-China" target="_blank">iGEM13_XMU-China</a> Design</span>
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                     <span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">Figure 3</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> </span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">A.</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">Top row is the original design by</span><span style="font-size: 14px;"> </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">Jeff Hasty</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">.</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> </span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">B.</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">Bottom row is the simplif</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">ied</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> design which sets lux pL and lux pR in the same direction.</span>
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                     <span style="font-weight: 700;">Figure 3A.</span>Top row is the original design by Jeff Hasty.<span style="font-weight: 700;">B.</span> Bottom row is the simplified design which sets Lux pL and Lux pR in the same direction.
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     <span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">In the simplif</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">ied</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> design (</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">Figure 3B</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">), when LuxR activates the backward transcription, RNA polymerase will be blocked by the terminators B0015. So that thi</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">s simplif</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">ication</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">doesn’t </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">perform as same as</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> original design. Actually, the</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> reverse </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">terminated </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">efficiency </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">of B0015 is 0.295</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">(CC)</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font; valign: sup;">[2]</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> which may lead to leakage transcription. </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">However, the correct sequence of GFP-LAA can’t be transcribed during the backwards transcription, even if the minus-strand of GFP-LAA could be transcribed, the sequence of the RNA is not </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">in </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">the right </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">direction of GFP-LAA, </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">hence incorrect amino acid sequences may be translated, resulting in misfolding GFP just as the SDS-PAGE shows (</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">Figure 1</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">). </span>
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     <span style="font-family: Arial,sans-serif; font-weight: 400;">In the simplif</span><span style="font-family: Arial,sans-serif; font-weight: 400;">ied</span><span style="font-family: Arial,sans-serif; font-weight: 400;"> design (</span><span style="font-family: Arial,sans-serif; font-weight: 700;">Figure 3B</span><span style="font-family: Arial,sans-serif; font-weight: 400;">), when LuxR activates the backwards transcription, RNA polymerase will be blocked by the terminators B0015. So this simplification will not  perform as same as original design. Actually, the reverse terminated efficiency of B0015 is 0.295(CC)<sup>[2]</sup> which may lead to leakage transcription. However, the correct sequence of GFP-LAA couldn’t be transcribed during the backwards transcription, even if the minus-strand of GFP-LAA could be transcribed, the sequence of the RNA is not in the right direction of GFP-LAA, hence incorrect amino acid sequences might be translated, resulting in misfolding GFP just as what the SDS-PAGE shows (</span><span style="font-family: Arial,sans-serif; font-weight: 700;">Figure 1</span><span style="font-family: Arial,sans-serif; font-weight: 400;">). </span>
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     <span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">Because of the </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">imperfect simplified</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> design doesn’t follow the original function completely, the abnormal oscillation is justifiable. </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">M</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">isfolding protein is a</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">n</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> evidence to support our assumption.</span>
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     <span style="font-family: Arial,sans-serif; font-weight: 400;">Because of the </span><span style="font-family: Arial,sans-serif; font-weight: 400;">imperfect simplified</span><span style="font-family: Arial,sans-serif; font-weight: 400;"> design didn’t follow the original function completely, the abnormal oscillation was justifiable. </span><span style="font-family: Arial,sans-serif; font-weight: 400;">M</span><span style="font-family: Arial,sans-serif; font-weight: 400;">isfolding protein were</span><span style="font-family: Arial,sans-serif; font-weight: 400;">n</span><span style="font-family: Arial,sans-serif; font-weight: 400;"> evidence to support our assumption.</span>
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     <span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">iGEM14 XMU-China involved sequence comparison to investigate the difference between the original and </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">the registry parts.</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> We find that</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> the original Lux pR has 20bp overlapping sequence with origin</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">al Lux p</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">R</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">. </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">There is </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">a r</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">estriction e</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">nzyme cutting site (EcoR I)</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> at the 56bp of original Lux pR</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> (</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">Figure 4</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">)</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">.</span>
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     <span style="font-family: Arial,sans-serif; font-weight: 400;"><a href="https://2014.igem.org/Team:XMU-China" target="_blank">iGEM14_XMU-China</a> involved sequence comparison to investigate the difference between the original and </span><span style="font-family: Arial,sans-serif; font-weight: 400;">the registry parts.</span><span style="font-family: Arial,sans-serif; font-weight: 400;"> We found that</span><span style="font-family: Arial,sans-serif; font-weight: 400;"> the original Lux pR had 20bp overlapping sequence with original</span><span style="font-family: Arial,sans-serif; font-weight: 400;">al Lux p</span><span style="font-family: Arial,sans-serif; font-weight: 400;">R</span><span style="font-family: Arial,sans-serif; font-weight: 400;">. </span><span style="font-family: Arial,sans-serif; font-weight: 400;">There was </span><span style="font-family: Arial,sans-serif; font-weight: 400;">a r</span><span style="font-family: Arial,sans-serif; font-weight: 400;">estriction e</span><span style="font-family: Arial,sans-serif; font-weight: 400;">nzyme cutting site (EcoR I)</span><span style="font-family: Arial,sans-serif; font-weight: 400;"> at the 56bp of original Lux pR</span><span style="font-family: Arial,sans-serif; font-weight: 400;"> (</span><span style="font-family: Arial,sans-serif; font-weight: 700;">Figure 4</span><span style="font-family: Arial,sans-serif; font-weight: 400;">)</span><span style="font-family: Arial,sans-serif; font-weight: 400;">.</span>
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                     <span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">Figure 4</span><span style="font-family: Times New Roman; font-weight: 700; styleName: Default Paragraph Font;">.</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> Schematic of original </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">QS promoter</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">.</span>
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                     <span style="font-weight: 700;">Figure 4. </span><span style="font-weight: 400;"> Schematic of original </span><span style="font-weight: 400;">QS promoter</span><span style="font-weight: 400;">.</span>
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    <span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">Parts registry truncate the original Lux pR at 56bp to get the </span><span style="font-family: Times New Roman;">55bp Lux pR</span><span style="font-family: Times New Roman;"> </span><span style="font-family: Times New Roman;">(BBa_R0062). </span><span style="font-family: Times New Roman;">On the contrary, Lux pL</span><span style="font-family: Times New Roman;"> </span><span style="font-family: Times New Roman;">(BBa_R0063) is longer the original Lux pL, and at the end of BBa_R0063 is </span><span style="font-family: Times New Roman;">initial part of </span><span style="font-family: Times New Roman;">41bp </span><span style="font-family: Times New Roman;">LuxR (BBa_C0062). </span><span style="font-family: Times New Roman;">Thus new problems</span><span style="font-family: Times New Roman;"> arise</span><span style="font-family: Times New Roman;">—</span><span style="font-family: Times New Roman;">i</span><span style="font-family: Times New Roman;">s the modification of original </span><span style="font-family: Times New Roman;">QS</span><span style="font-family: Times New Roman;"> </span><span style="font-family: Times New Roman;">promoter </span><span style="font-family: Times New Roman;">reasonable? Does the modification result in the unexpected backward transcription?</span>
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        <span style="font-family: Arial,sans-serif; font-weight: 400;">Parts registry truncated the original Lux pR at 56bp to get the 55bp Lux pR (BBa_R0062). On the contrary, Lux pL (BBa_R0063) is longer than the original Lux pL, and at the end of BBa_R0063 is initial part of 41bp LuxR (BBa_C0062). Thus new problems arised—was the modification of original QS promoter reasonable? Did the modification result in the unexpected backwards transcription?</span>
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     <span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">Quorum sensing system is so widely used in the synthetic biology, we think it’s remarkable to make it clear. We highlight the abnormal phenomenon of QS oscillation which may</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> be caused by imperfect simplification</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> for the very first time. </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">We hope</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> that more </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">effort</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">s</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">could</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> be </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">made</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;"> to figure out the interaction between </span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">QS oscillation parts.</span><span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font; valign: sup;">[3]</span>
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     <span style="font-family: Arial,sans-serif; font-weight: 400;">Quorum sensing system is so widely used in the synthetic biology, we thought it’s remarkable to make it clear. We highlighted the abnormal phenomenon of QS oscillation which might be caused by imperfect simplification for the very first time. We hope that more efforts could be made to figure out the interaction between QS oscillation parts.<sup>[3]</sup></span>
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     <span style="font-family: Arial,sans-serif; font-size: 21px; font-weight: 700;">References</span>
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     <span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">1. </span><span style="background: rgb(255, 255, 255); color: rgb(34, 34, 34); font-family: Arial; font-size: 13px;">Eckdahl T, Sawyer E M, Barta C, et al. </span><span style="background: rgb(255, 255, 255); color: rgb(34, 34, 34); font-family: Arial; font-size: 13px;">Bacterial logic devices reveal unexpected behavior of frameshift suppressor tRNAs[J]. Interdisciplinary Bio Central, 2012, 4(1): 10.</span>
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     <span style="font-size:14px"><a href="http://www.ibc7.org/article/journal_v.php?sid=287" target="_self">1. Eckdahl T, Sawyer E M, Barta C, et al. Bacterial logic devices reveal unexpected behavior of frameshift suppressor tRNAs[J]. Interdisciplinary Bio Central, 2012, 4(1): 10.</a></span>
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    <span style="color: rgb(0, 0, 255); text-decoration: underline; styleName: Default Paragraph Font;">http://www.ibc7.org/article/journal_v.php?sid=287</span>
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    <span style="font-size:14px"> <a href="http://parts.igem.org/Part:BBa_B0015" target="_self">2. http://parts.igem.org/Part:BBa_B0015</a></span>
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     <span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">2. </span><span style="color: rgb(0, 0, 255); text-decoration: underline; styleName: Default Paragraph Font;">http://parts.igem.org/Part:BBa_B0015</span>
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     <span style="font-size:14px"><a href="http://www.nature.com/nature/journal/v463/n7279/full/nature08753.html" target="_self">3. Danino T, Mondragón-Palomino O, Tsimring L, et al.A synchronized quorum of genetic clocks[J]. Nature, 2010, 463(7279): 326-330.</a></span>
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    <span style="font-family: Times New Roman; font-weight: 400; styleName: Default Paragraph Font;">3. </span><span style="background: rgb(255, 255, 255); color: rgb(34, 34, 34); font-family: Arial; font-size: 13px;">Danino T, Mondragón-Palomino O, Tsimring L, et al. </span><span style="background: rgb(255, 255, 255); color: rgb(34, 34, 34); font-family: Arial; font-size: 13px;">A synchronized quorum of genetic clocks[J]. </span><span style="background: rgb(255, 255, 255); color: rgb(34, 34, 34); font-family: Arial; font-size: 13px;">Nature, 2010, 463(7279): 326-330.</span>
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    <span style="color: rgb(0, 0, 255); text-decoration: underline; styleName: Default Paragraph Font;">http://www.nature.com/nature/journal/v463/n7279/full/nature08753.html</span>
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Latest revision as of 03:26, 18 October 2014

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A REASONABLE EXPLANATION OF MISFOLDING GFP UNDER QS OSCILLATION



In the project iGEM13_XMU-China, they couldn't get expected oscillation. However, this year iGEM14_XMU-China further investigated the reason of abnormal oscillation. We further reviewed SDS-PAGE analysis to confirm the circuit at protein level. The SDS-PAGE data is shown in Figure 1. Based on that, we made a reasonable assumption that the unexpected behavior of the LuxR promoter leads to the misfolding proteins Hence result in the abnormal oscillation result in the abnormal oscillation.

 

Figure 1. SDS-PAGE analysis of E. coli K strain (DH5α). (a) Lane 1-2: supernatant and pellet of original DH5α; Lane 3-4: supernatant and pellet of strain with single plasmid A1 (BBa_K1036003); Lane 5-6: supernatant and pellet of strain with both plasmids A1 (BBa_K1036003) and B (BBa_K1036000). The red arrows indicate the misfolding GFP-LVA protein (27.6 kDa) in the precipitation. (b) Lane 1-2: supernatant and pellet of original BL21; Lane 3-4: supernatant and pellet of strain with single plasmid A1 (BBa_K1036003); Lane 5-6: supernatant and pellet of strain with both plasmids A1 (BBa_K1036003) and B (BBa_K1036000). The blue arrows indicate LuxR (27.5 kDa), GFP-LVA (27.6 kDa) and AiiA-LVA (28.7 kDa) in the supernatant. The orange arrows indicate LuxI-LVA (22.4 kDa) in the supernatant. (The marker of b was not in right position, however, the proteins were confirmed by MALDI-TOF-TOF .)

 

As the SDS-PAGE shows, a large amount of GFP-LVA and LuxI-LVA appear in pellet where misfolding proteins often exist. Both proteins directly affect the oscillation result. And it is critical to find out the reason for misfolding proteins. iGEM14_XMU-China made the following assumption:

   

The research[1] reveals an unexpected behavior of Lux pR (BBa_R0062). In the absence of autoinducer 3OC6 (AHL), LuxR binds to plux (Lux pR) and activates backwards transcription (Figure 2).

 

Figure 2. Relative RFP fluorescence for a control construct designed to measure backwards transcription from Lux pR. Addition of LuxR and 3OC6 90 (AHL) as indicated. Error bars in all panels are one standard deviation.

 

The imperfect simplification of setting lux pL and Lux pR in the same direction: 

From the original design by Jeff Hasty, Lux pR and Lux pL were set in opposite directions (Figure 3A). In the absence of AHL, LuxR could activate backwards transcription of Lux pR leading to more expression of LuxR which was critical to meet the oscillation conditions. However, present literature did’t consider the backwards transcription which had effect on quorum sensing oscillation.

 

A. Original Design

B. iGEM13_XMU-China Design

Figure 3A.Top row is the original design by Jeff Hasty.B. Bottom row is the simplified design which sets Lux pL and Lux pR in the same direction.

 

In the simplified design (Figure 3B), when LuxR activates the backwards transcription, RNA polymerase will be blocked by the terminators B0015. So this simplification will not perform as same as original design. Actually, the reverse terminated efficiency of B0015 is 0.295(CC)[2] which may lead to leakage transcription. However, the correct sequence of GFP-LAA couldn’t be transcribed during the backwards transcription, even if the minus-strand of GFP-LAA could be transcribed, the sequence of the RNA is not in the right direction of GFP-LAA, hence incorrect amino acid sequences might be translated, resulting in misfolding GFP just as what the SDS-PAGE shows (Figure 1).

 

Because of the imperfect simplified design didn’t follow the original function completely, the abnormal oscillation was justifiable. Misfolding protein weren evidence to support our assumption.

 

iGEM14_XMU-China involved sequence comparison to investigate the difference between the original and the registry parts. We found that the original Lux pR had 20bp overlapping sequence with originalal Lux pR. There was a restriction enzyme cutting site (EcoR I) at the 56bp of original Lux pR (Figure 4).

 

Figure 4. Schematic of original QS promoter.

 

Parts registry truncated the original Lux pR at 56bp to get the 55bp Lux pR (BBa_R0062). On the contrary, Lux pL (BBa_R0063) is longer than the original Lux pL, and at the end of BBa_R0063 is initial part of 41bp LuxR (BBa_C0062). Thus new problems arised—was the modification of original QS promoter reasonable? Did the modification result in the unexpected backwards transcription?

 

Quorum sensing system is so widely used in the synthetic biology, we thought it’s remarkable to make it clear. We highlighted the abnormal phenomenon of QS oscillation which might be caused by imperfect simplification for the very first time. We hope that more efforts could be made to figure out the interaction between QS oscillation parts.[3]

 

References

1. Eckdahl T, Sawyer E M, Barta C, et al. Bacterial logic devices reveal unexpected behavior of frameshift suppressor tRNAs[J]. Interdisciplinary Bio Central, 2012, 4(1): 10.

2. http://parts.igem.org/Part:BBa_B0015

3. Danino T, Mondragón-Palomino O, Tsimring L, et al.A synchronized quorum of genetic clocks[J]. Nature, 2010, 463(7279): 326-330.