Difference between revisions of "Team:BioIQS-Barcelona/DryLab"
Marc exposit (Talk | contribs) |
Marc exposit (Talk | contribs) |
||
| Line 89: | Line 89: | ||
<h4 class="book orange block-sept comas"><i>Despite what some people may think, DryLab | <h4 class="book orange block-sept comas"><i>Despite what some people may think, DryLab | ||
occasionally may be equal or more important for a project to develop properly than the | occasionally may be equal or more important for a project to develop properly than the | ||
| − | WetLab. Applying this | + | WetLab. Applying this to our project, we decided to study some important |
aspects and evaluate their viability. More specifically, our work in the DryLab | aspects and evaluate their viability. More specifically, our work in the DryLab | ||
consisted on:</i></h4> | consisted on:</i></h4> | ||
| Line 107: | Line 107: | ||
<div class="col-md-12 mx-auto"> | <div class="col-md-12 mx-auto"> | ||
<div class="row"> | <div class="row"> | ||
| − | <h3 class="orange-intense">1st | + | <h3 class="orange-intense">1st: Modeling</h3> |
</div> | </div> | ||
<div class="row block-desc-b"> | <div class="row block-desc-b"> | ||
<div class="col-md-6 right"> | <div class="col-md-6 right"> | ||
<p class="book orange">We had several ideas about how the sensor could work, and | <p class="book orange">We had several ideas about how the sensor could work, and | ||
| − | eventually, one rose up strongly. The first step | + | eventually, one rose up strongly. The first step is having an idea. It may seem simple, but it can take long, as it goes through |
| − | think about | + | think about the idea, understand it and rethink it as many times as it is required. Maybe this reflection |
| − | seems | + | seems intuitive, but constitutes the fundamental part of all |
| − | + | developments. Using mathematical models and computer simulations we have been able to | |
| − | understand the dynamics underlying our sensor, variety of parameters | + | understand the dynamics underlying our sensor. Furthermore, using this model we can tune a huge variety of parameters, |
| − | eventualities | + | test many eventualities and predict the tendency of the sensor.</p> |
| Line 123: | Line 123: | ||
<div class="col-md-6 left center"> | <div class="col-md-6 left center"> | ||
<div class="col-md-12 left"> | <div class="col-md-12 left"> | ||
| − | <p class="book orange">Generally speaking, the bottleneck | + | <p class="book orange">Generally speaking, the bottleneck or critical working point of our idea, |
| − | + | was being able to build up a complex network of gold | |
| − | nano-particles | + | nano-particles. This would enable our sensor to have an easy optical detection system. Understanding |
| − | the implications associated | + | the implications associated in that procedure makes the difference while facing the real design. |
| − | + | How can we detect the interactions between the HLA-DQ protein and gluten-derived peptides? How can this detection be easy and visual? And finally, which are the physical dynamics pervading in the system? | |
| − | + | Go to the <a href="https://2018.igem.org/Team:BioIQS-Barcelona/Model">modeling section</a> if you wish to know the answer to all this questions. </p> | |
| − | + | ||
<div class="row block-desc-b"> | <div class="row block-desc-b"> | ||
| Line 135: | Line 134: | ||
<div class="row block-sept center"> | <div class="row block-sept center"> | ||
<div class="col-md-7 button"> | <div class="col-md-7 button"> | ||
| − | <a class="text-transform" href="https://2018.igem.org/Team:BioIQS-Barcelona/Model" target="_blank"> | + | <a class="text-transform" href="https://2018.igem.org/Team:BioIQS-Barcelona/Model" target="_blank"> Modeling</a> |
</div> | </div> | ||
</div> | </div> | ||
| Line 146: | Line 145: | ||
</div> | </div> | ||
<div class="row"> | <div class="row"> | ||
| − | <h3 class="orange-intense">2nd PCRs standardization</h3> | + | <h3 class="orange-intense">2nd: PCRs standardization</h3> |
</div> | </div> | ||
<div class="row block-desc-b"> | <div class="row block-desc-b"> | ||
<div class="col-md-6 right"> | <div class="col-md-6 right"> | ||
<p class="book orange">One of the strengths of our approach to detect patient-specific | <p class="book orange">One of the strengths of our approach to detect patient-specific | ||
| − | reactive gluten peptides in food is that | + | reactive gluten peptides in food is that we can produce the sensor using only a DNA |
| − | sample | + | sample from the saliva of the patient, which is not invasive. Patient’s HLA-DQ (the protein responsible for |
| − | + | recognizing and triggering the immune response) is then expressed using the <a href="https://2018.igem.org/Team:BioIQS-Barcelona/Basic_Part">PCR protocol</a> | |
| − | + | designed in the WetLab. For this purpose, we use specific primers to amplify the patient’s | |
| − | target genes and thus, it is necessary to evaluate if they | + | target genes and thus, it is necessary to evaluate if they will be useful for all of the |
different celiac-associated genotypes.</p> | different celiac-associated genotypes.</p> | ||
</div> | </div> | ||
| Line 161: | Line 160: | ||
<div class="col-md-12"> | <div class="col-md-12"> | ||
<p class="book orange">A multiple sequence alignment (MSA) on all annotated | <p class="book orange">A multiple sequence alignment (MSA) on all annotated | ||
| − | celiac-associated genomic sequence was performed to evaluate the specific | + | celiac-associated genomic sequence was performed to evaluate the conservation between genotypes of the specific |
| − | primer-binding regions | + | primer-binding regions.</p> |
| − | <p class="book orange"> | + | <p class="book orange">The results demonstrate that this regions are perfectly |
| − | conserved or slightly different for both DQ2 and DQ8 celiac haplotypes | + | conserved or only slightly different for both DQ2 and DQ8 celiac haplotypes. |
This means that either the same primer can be used for amplifying all genotypes or | This means that either the same primer can be used for amplifying all genotypes or | ||
| − | that a specific DQ2- or DQ8-primer has to be used.</p> | + | that a specific DQ2- or DQ8-primer has to be used. The possibility to use the same primers for multiple patients reduces the costs associated in the personalization factor. |
| − | + | Thus, we've created a standard method to achieve the required personalization.</p> | |
<div class="row block-desc-b"> | <div class="row block-desc-b"> | ||
<div class="col-md-12 left"> | <div class="col-md-12 left"> | ||
| Line 185: | Line 184: | ||
</div> | </div> | ||
<div class="row"> | <div class="row"> | ||
| − | <h3 class="orange-intense">3rd Molecular recognition</h3> | + | <h3 class="orange-intense">3rd: Molecular recognition</h3> |
</div> | </div> | ||
<div class="row block-desc-b"> | <div class="row block-desc-b"> | ||
<div class="col-md-6 right"> | <div class="col-md-6 right"> | ||
<p class="book orange">Another aspect that we wanted to evaluate is how the HLA-DQ protein | <p class="book orange">Another aspect that we wanted to evaluate is how the HLA-DQ protein | ||
| − | is able to effectively | + | is able to effectively recognize and bind gluten-derived peptides. Specifically, which |
| − | are the residues that are mediating this recognition and | + | are the residues that are mediating this recognition and if they are conserved among |
celiac haplotypes DQ2 and DQ8.</p> | celiac haplotypes DQ2 and DQ8.</p> | ||
| − | <p class="book orange">To do so, we focused the conservation study to | + | <p class="book orange">To do so, we focused the conservation study to the residues that |
| − | have been suggested to be responsible | + | have been previously suggested to be responsible for the peptide recognition. A multiple alignment |
| − | + | of protein amino acid sequences was performed using all the annotated HLA-DQ proteins so far.</p> | |
</div> | </div> | ||
<div class="col-md-6 left center"> | <div class="col-md-6 left center"> | ||
<div class="col-md-12"> | <div class="col-md-12"> | ||
| − | <p class="book orange"> | + | <p class="book orange">The results demonstrate that three different residues, two in the α chain and one in |
| − | the β chain, | + | the β chain, are conserved among celiac patients and |
| − | absent in healthy people | + | absent in healthy people. This mutated residues strictly need to be present in the HLA-DQ protein in order to molecularly |
| − | + | recognize a gluten peptide and develop the disease. Therefore, we elucidated <a href="https://2018.igem.org/Team:BioIQS-Barcelona/Celiac_disease">which are the residues</a> of the HLA-DQ protein responsible for its interaction with the epitopes involved in celiac disease.</p> | |
| − | + | ||
| − | + | ||
<div class="row block-desc-b"> | <div class="row block-desc-b"> | ||
<div class="col-md-12 left"> | <div class="col-md-12 left"> | ||
Revision as of 23:35, 10 December 2018
Dry Lab | Overview
Have a look!Inner beauty
Despite what some people may think, DryLab occasionally may be equal or more important for a project to develop properly than the WetLab. Applying this to our project, we decided to study some important aspects and evaluate their viability. More specifically, our work in the DryLab consisted on:
1st: Modeling
We had several ideas about how the sensor could work, and eventually, one rose up strongly. The first step is having an idea. It may seem simple, but it can take long, as it goes through think about the idea, understand it and rethink it as many times as it is required. Maybe this reflection seems intuitive, but constitutes the fundamental part of all developments. Using mathematical models and computer simulations we have been able to understand the dynamics underlying our sensor. Furthermore, using this model we can tune a huge variety of parameters, test many eventualities and predict the tendency of the sensor.
Generally speaking, the bottleneck or critical working point of our idea, was being able to build up a complex network of gold nano-particles. This would enable our sensor to have an easy optical detection system. Understanding the implications associated in that procedure makes the difference while facing the real design. How can we detect the interactions between the HLA-DQ protein and gluten-derived peptides? How can this detection be easy and visual? And finally, which are the physical dynamics pervading in the system? Go to the modeling section if you wish to know the answer to all this questions.
2nd: PCRs standardization
One of the strengths of our approach to detect patient-specific reactive gluten peptides in food is that we can produce the sensor using only a DNA sample from the saliva of the patient, which is not invasive. Patient’s HLA-DQ (the protein responsible for recognizing and triggering the immune response) is then expressed using the PCR protocol designed in the WetLab. For this purpose, we use specific primers to amplify the patient’s target genes and thus, it is necessary to evaluate if they will be useful for all of the different celiac-associated genotypes.
A multiple sequence alignment (MSA) on all annotated celiac-associated genomic sequence was performed to evaluate the conservation between genotypes of the specific primer-binding regions.
The results demonstrate that this regions are perfectly conserved or only slightly different for both DQ2 and DQ8 celiac haplotypes. This means that either the same primer can be used for amplifying all genotypes or that a specific DQ2- or DQ8-primer has to be used. The possibility to use the same primers for multiple patients reduces the costs associated in the personalization factor. Thus, we've created a standard method to achieve the required personalization.
3rd: Molecular recognition
Another aspect that we wanted to evaluate is how the HLA-DQ protein is able to effectively recognize and bind gluten-derived peptides. Specifically, which are the residues that are mediating this recognition and if they are conserved among celiac haplotypes DQ2 and DQ8.
To do so, we focused the conservation study to the residues that have been previously suggested to be responsible for the peptide recognition. A multiple alignment of protein amino acid sequences was performed using all the annotated HLA-DQ proteins so far.
The results demonstrate that three different residues, two in the α chain and one in the β chain, are conserved among celiac patients and absent in healthy people. This mutated residues strictly need to be present in the HLA-DQ protein in order to molecularly recognize a gluten peptide and develop the disease. Therefore, we elucidated which are the residues of the HLA-DQ protein responsible for its interaction with the epitopes involved in celiac disease.