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| | <p class="dropcap">One of the most interesting and complex types of group behaviors in animals is that in which several organisms simultaneously repeat the same activity at regular intervals of time.<sup>1</sup> In ordinary usage, this kind of behavior is called “<strong>synchronous</strong>”. It has been observed in Thailand that male Pteroptyx malaccae fireflies, congregated in trees, flash in rhythmic synchrony with a period of about 560 ± 6 msec (at 28°C). Males of a China’s special species of firefly called <i><b>Qiongyuying</b></i> flash synchronously during mating season. And we also observed that bees crawling in the same small area display a synchrony of wings fluttering in order to scare off intruder,and we filmed a video clip to demonstrate this phenomenon.</p> | | <p class="dropcap">One of the most interesting and complex types of group behaviors in animals is that in which several organisms simultaneously repeat the same activity at regular intervals of time.<sup>1</sup> In ordinary usage, this kind of behavior is called “<strong>synchronous</strong>”. It has been observed in Thailand that male Pteroptyx malaccae fireflies, congregated in trees, flash in rhythmic synchrony with a period of about 560 ± 6 msec (at 28°C). Males of a China’s special species of firefly called <i><b>Qiongyuying</b></i> flash synchronously during mating season. And we also observed that bees crawling in the same small area display a synchrony of wings fluttering in order to scare off intruder,and we filmed a video clip to demonstrate this phenomenon.</p> |
| - | <div style="margin-left:40px"><embed src="http://www.tudou.com/v/VY8BWCd7FSA/&resourceId=0_05_05_99&bid=05/v.swf" type="application/x-shockwave-flash" allowscriptaccess="always" allowfullscreen="true" wmode="opaque" width="600" height="400"></div> | + | <div><embed src="http://www.tudou.com/v/VY8BWCd7FSA/&resourceId=0_05_05_99&bid=05/v.swf" type="application/x-shockwave-flash" allowscriptaccess="always" allowfullscreen="true" wmode="opaque" width="480" height="400"></div> |
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| | <p class="dropcap"> Moreover, synchrony has been described in a range of mammal groups, including <i><b>odontocete cetaceans</b></i> (a kind of toothed whale).<sup>2</sup> The <i><b>odontocete cetaceans</b></i> behave synchronously when they breathe on the surface of water.</p> | | <p class="dropcap"> Moreover, synchrony has been described in a range of mammal groups, including <i><b>odontocete cetaceans</b></i> (a kind of toothed whale).<sup>2</sup> The <i><b>odontocete cetaceans</b></i> behave synchronously when they breathe on the surface of water.</p> |
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| | <p> Light sensor that directly regulates the expression at the transcription level is rarely seen. Bacterial opsins usually appeal as light activated kinases or phosphodiesterases. | | <p> Light sensor that directly regulates the expression at the transcription level is rarely seen. Bacterial opsins usually appeal as light activated kinases or phosphodiesterases. |
| - | BBa_K238013, an exact promoter of the blue light receptor, is a portion of an E.coli constitutive light sensing system. This system consists of a receptor, ycgF, which is responsive to blue light. When blue light strikes, the <img src="https://static.igem.org/mediawiki/2012/b/bb/Ycgz_system.jpg" style="width:60%;margin:15px;float:right">When blue light strikes, the receptor changes conformation and dimerizes driven by the BLUF-domain. This allows it to bind to the ycgE repressor through its EAL-domain, releasing the repressor from the promoter region. In summary, the irradiance of blue light will cause a positive induction, expression downstream | + | BBa_K238013, an exact promoter of the blue light receptor, is a portion of an E.coli constitutive light sensing system. This system consists of a receptor, ycgF, which is responsive to blue light. When blue light strikes, the <img src="https://static.igem.org/mediawiki/2012/b/bb/Ycgz_system.jpg" style="margin:15px;float:right">When blue light strikes, the receptor changes conformation and dimerizes driven by the BLUF-domain. This allows it to bind to the ycgE repressor through its EAL-domain, releasing the repressor from the promoter region. In summary, the irradiance of blue light will cause a positive induction, expression downstream |
| | Light sensing feedback using ycgF-YcgE-YcgZ sensing system.</p><img src="https://static.igem.org/mediawiki/2012/8/85/YcgF.jpg" style="width:45%;margin-left:15px;float:right;margin-bottom:15px"> | | Light sensing feedback using ycgF-YcgE-YcgZ sensing system.</p><img src="https://static.igem.org/mediawiki/2012/8/85/YcgF.jpg" style="width:45%;margin-left:15px;float:right;margin-bottom:15px"> |
| | <p><strong>MG1655 strain</strong><br>The PCR process results that dH5α,the strain we used as normal competent cell, does not contain such endogenous system. The MG1655 strain as a wild type of E.coli K12 was used for the construction of our light sensing design. <a href="http://openwetware.org/wiki/E._coli_genotypes#MG1655"> See MG1655 genotype</a>. </p> | | <p><strong>MG1655 strain</strong><br>The PCR process results that dH5α,the strain we used as normal competent cell, does not contain such endogenous system. The MG1655 strain as a wild type of E.coli K12 was used for the construction of our light sensing design. <a href="http://openwetware.org/wiki/E._coli_genotypes#MG1655"> See MG1655 genotype</a>. </p> |
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| - | <h1><a name="lightsensor">Light Sensor</a></h1> | + | <h1><a name="lightsensor">Sensor protein design</a></h1> |
| - | <p>Pellentesque habitant morbi tristique senectus et netus et malesuada fames ac turpis egestas. Vestibulum tortor quam, feugiat vitae, ultricies eget, tempor sit amet, ante. Donec eu libero sit amet quam egestas semper. Aenean ultricies mi vitae est. Mauris placerat eleifend leo. Quisque sit amet est et sapien ullamcorper pharetra. Vestibulum erat wisi, condimentum sed, commodo vitae, ornare sit amet, wisi. Aenean fermentum, elit eget tincidunt condimentum, eros ipsum rutrum orci, sagittis tempus lacus enim ac dui. Donec non enim in turpis pulvinar facilisis. Ut felis. Praesent dapibus, neque id cursus faucibus, tortor neque egestas augue, eu vulputate magna eros eu erat. Aliquam erat volutpat. Nam dui mi, tincidunt quis, accumsan porttitor, facilisis luctus, metus</p> | + | |
| - | <p> Pellentesque habitant morbi tristique senectus et netus et malesuada fames, Pellentesque habitant morbi tristique senectus et netus et malesuada fames Pellentesque habitant morbi tristique senectus et netus et malesuada fames.</p> | + | <p><strong>Issue</strong><br>By using the YcgZ light inducing system, we have basically completed our gene circuits. But the performance issue is a critical topic to all the endogenous system. |
| | + | </p> |
| | + | <p>With the help of the previous iGEMer, we could have a comprehensive knowledge of the ycgZ performance. Two charts placed here show the promote level of YcgZ and the leaky expression. </p> |
| | + | <img src="http://partsregistry.org/wiki/images/f/f9/Weakness.png" style="width:46%;margin-right:15px" class="myimg"><img src="http://partsregistry.org/wiki/images/e/e8/Light-dark.png" class="myimg" style="width:46%"> |
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| | + | <p>Weak promotion and high level leaky expression may reduce the ratio of signal to noise. More than that, negative feedback requires a repressive domain with in the sensation system. |
| | + | To solve the issue rise above, we have launched the DESIGN (Design of Enhanced Sensor Instead General Negative part) subproject aiming at providing a high sensitivity, low leaky expression and plasmid based light sensation negative regulation system. |
| | + | |
| | + | </p> |
| | + | <p><strong>tetR repressor</strong>TetR act as a repressor is operating by binding to the specific DNA sequence, which is a palindromic sequence. The whole binding structure is classified as the HTH motif containing a |
| | + | <img src="https://static.igem.org/mediawiki/2012/2/2e/TetR_lux.jpg" style="width:90%;align-ment:middle"> |
| | + | |
| | + | <p>helix-turn-helix protein sequence which is the α2 and α3 helixes in the structure image. |
| | + | Using tetR as a repression has several advantages. The tetR has no leaky expression, and the repression can be adjusted by the tetracycline. <br> |
| | + | </p> |
| | + | <p><strong>LOV domain</strong><br>LOV (light, oxygen or voltage) domains are protein photo sensors that are conserved in bacteria, archaea, plants and fungi, and detect blue light via a flavin cofactor (FMN or FAD).<img src="https://static.igem.org/mediawiki/2012/5/54/Lovdomain.PNG" style="width:90%"> |
| | + | </p> |
| | + | <p>Figure 2this cartoon presents just a few examples of the hundreds of LOV domain- containing proteins. The attached domain include: GAF cyclic GMP-specific phosphodiesterases; HTH helix-turn-helix; HK histidine kinase; MASE1 membrane-associated sensor1; PAS PER-ARNT-SIM; REC CheY-like phosphoacceptor (receiver); SpollE sporulation stage II protein E; STAS sulphate transporter anti-σ antagonist; ZnF zinc-finger.</p> |
| | + | <p>In bacteria, LOV proteins generally follow the domain organization that is described in other bacterial signaling proteins. The activation domain could be multifunctional; the chart shows the diversity in LOV-signaling output. Such complex domain arrangements can allow the integration<img src="https://static.igem.org/mediawiki/2012/d/de/Lov_function_lux.PNG">of multiple environmental signals and can provide mechanisms for amplification or attenuation of the light signal. |
| | + | Clearly, LOV domains are versatile photoswitches. But how do LOV domains regulate such a structurally disparate group of proteins? The mechanisms could be simply described by the following chart. The LOV domain transfer the signal by the Jα helix or the dimerization of the Ncap. |
| | + | The properties of LOV domain show us the possibility of designing light switch. We have laid eyes on such two LOV opsins: EL222 and AsLov2. |
| | + | </p> |
| | + | <p><strong>LOV-HTH</strong><br> |
| | + | The LOV-HTH protein design is inspire by the natural protein EL222, a 222amino acid protein isolated from the marine bacterium Erythrobacter litoralis HTCC2594. In addition to an N-terminal LOV<img src="https://static.igem.org/mediawiki/2012/d/dc/HTH_swap.jpg" style="float:left"> |
| | + | domain, EL222 also contains a C-terminal helix-turn-helix (HTH) DNA-binding domain representative of LuxR-type DNA-binding proteins. |
| | + | The EL222 has the naturally light switch and DNA binding activity, but the regulation sequence should be modified into a repressive operon. The tetR operating sequence shows the same HTH motif. So the HTH swap could be processed. The swapped sequence is shown in the image. |
| | + | After the HTH swap, Lov-HTH is transformed into a light sensing domain with the PtetO repressive switch function.</p><img src="https://static.igem.org/mediawiki/2012/b/b1/HTH_swap.png" |
| | + | </p> |
| | + | <p> |
| | + | <strong>LOV-tetR</strong><br> |
| | + | Beside the unfolding and the dimerization, the Jα helix lies directly behind the normal Lov domain could also make the effective signal output by conducting the allosteric signal. This kind of physical mechanical interaction is delivered by the lever arm like helix. This kind of methodology is successful achieved by <img src="https://static.igem.org/mediawiki/2012/3/32/Bluf_water.png" style="width:55%;margin:15px;float:right"class="myimg">Devin Strickland and his colleagues. |
| | + | Under our condition, constructing a lever arm between the As Lov2 domain and the tetR is quite crucial. Our strategy is forming a helix to helix connection. The C-terminal of Lov2 and the N-terminal of tetR is directly linked together by delete the non-helix-forming amino acid sequence at the linker part. The linker itself construct a Jα lever arm. |
| | + | At the dark situation, the Jα delivered allosteric effect make the lov domain become a hindrance of the tetR binding to the DNA. When the protein exposed to a 450nm blue light, Jα can release the LOV domain, DNA binding activity is restored. That trigger the repression switch, expression under the PtetO will be repressed. </p> |
| | + | <img src="https://static.igem.org/mediawiki/2012/4/45/Lov-tetR_text.jpg" class="myimg"></p> |
| | + | |
| | </div> | | </div> |
| | <div> | | <div> |
"
not fit the light sensor which we will discuss later. So we picked another well-known bio illuminator, the Lux operon. It is also presented by 2010 Cambridge. 
blue-green light with a maximum intensity at 490 nm without the requirement of adding exogenous substrate, which was the prime reason why we chose it to be our light source in this study.
When blue light strikes, the receptor changes conformation and dimerizes driven by the BLUF-domain. This allows it to bind to the ycgE repressor through its EAL-domain, releasing the repressor from the promoter region. In summary, the irradiance of blue light will cause a positive induction, expression downstream
Light sensing feedback using ycgF-YcgE-YcgZ sensing system.
of multiple environmental signals and can provide mechanisms for amplification or attenuation of the light signal.
Clearly, LOV domains are versatile photoswitches. But how do LOV domains regulate such a structurally disparate group of proteins? The mechanisms could be simply described by the following chart. The LOV domain transfer the signal by the Jα helix or the dimerization of the Ncap.
The properties of LOV domain show us the possibility of designing light switch. We have laid eyes on such two LOV opsins: EL222 and AsLov2.
domain, EL222 also contains a C-terminal helix-turn-helix (HTH) DNA-binding domain representative of LuxR-type DNA-binding proteins.
The EL222 has the naturally light switch and DNA binding activity, but the regulation sequence should be modified into a repressive operon. The tetR operating sequence shows the same HTH motif. So the HTH swap could be processed. The swapped sequence is shown in the image.
After the HTH swap, Lov-HTH is transformed into a light sensing domain with the PtetO repressive switch function.
Devin Strickland and his colleagues.
Under our condition, constructing a lever arm between the As Lov2 domain and the tetR is quite crucial. Our strategy is forming a helix to helix connection. The C-terminal of Lov2 and the N-terminal of tetR is directly linked together by delete the non-helix-forming amino acid sequence at the linker part. The linker itself construct a Jα lever arm.
At the dark situation, the Jα delivered allosteric effect make the lov domain become a hindrance of the tetR binding to the DNA. When the protein exposed to a 450nm blue light, Jα can release the LOV domain, DNA binding activity is restored. That trigger the repression switch, expression under the PtetO will be repressed. 
