Difference between revisions of "Team:Freiburg/Project/Overview"

(new - image is still missing)
Line 479: Line 479:
 
<div class="level1">
 
<div class="level1">
 
<div class="image_box left">
 
<div class="image_box left">
<img align="left" alt="light bulb sketch" src="https://static.igem.org/mediawiki/2015/2/23/Freiburg_light_bulb_sketch.png" width="100px">
+
<img align="left" alt="DiaCHIP_Sabi" src="https://static.igem.org/mediawiki/2015/2/23/Freiburg_DiaCHIP_Sabi.png" width="100px">
 
</div>
 
</div>
 
<p>
 
<p>
 
<!--korrigiert von Philipp05/09/15-->
 
<!--korrigiert von Philipp05/09/15-->
The DiaCHIP is an innovative tool to simultaneously differentially detect antibodies present in blood sera that correspond to infectious diseases. It may greatly simplify broad band screenings, detection of autoimmune diseases and the determination of vaccination status. Essential for our project idea is the combination of on-demand protein synthesis directly in the diagnostic device, that is using a novel and label-free detection system, so simple that it can easily be rebuild and utilized by future iGEM teams.
+
<!--neu von Ramona08/09/15-->
 +
The DiaCHIP is an innovative tool to simultaneously and differentially detect antibodies present in blood sera in response to an infectious disease. It bears the potential to greatly simplify broad band screenings, detection of autoimmune diseases and the determination of vaccination statuses. Especially in case of threatening infections accompanied by similar symptoms fast and reliable differentiation could save lives.
 +
</br>
 +
To account for a disease by verification of corresponding antibodies in a patient’s blood serum is a well-known and routinely used system in modern diagnostics (LINK – diagnostics today). Thus, a simple blood sample is sufficient to perform reliable diagnostics with the DiaCHIP.
 +
</br>
 +
The key feature in the concept of the DiaCHIP is the combination of on-demand protein synthesis and a novel, label-free detection method in one device. This enables to overcome challenges in storage and handling that occur with currently available tests. Additionally, diagnoses can be received faster and in a more cost-efficient way than until now. Nonetheless, the whole device is so simple that it can easily be rebuilt and utilized by future iGEM teams (LINK – new device).
 +
 
 
</p>
 
</p>
 
</div>
 
</div>
 
<!-- EDIT1 SECTION "Project overview: The DiaCHIP" [1-351] -->
 
<!-- EDIT1 SECTION "Project overview: The DiaCHIP" [1-351] -->
<div class="floatbox left">
+
<h2 class="sectionedit2">Step 1: Preparing the DiaCHIP by protein synthesis</h2>
<h2 class="sectionedit2">Preparing the DiaCHIP</h2>
+
<div class="level2">
+
 
<p>
 
<p>
 
<!--korrigiert von Philipp05/09/15-->
 
<!--korrigiert von Philipp05/09/15-->
As the DiaCHIP relies on antibody-antigen interactions, the antigens first have to be synthesized and immobilized inside the device. Given that the whole device is a microfluidic system, it was most convenient to do this directly in the flow-chamber, where detection will finally take place.
+
<!--neu von Ramona08/09/15-->
The flow-chamber consists of two glass surfaces separated by a gap that can be flushed with liquids. On the one surface DNA molecules, which code for the respective antigens. By flushing a cell-free expression mix into the chamber, the respective antigens are transcribed and translated on-demand. Proteins then diffuse until reaching the second surface that specifically captures the proteins encoded by the immobilized DNA. After several washing steps to remove remaining expression-mix the flow-chamber is coated with the immobilized antigens and ready for detection.  
+
Before being able to screen for antibody-antigen interactions, antigens have to be synthesized and immobilized in a microarray arrangement. This is obtained by a copying mechanism transforming a DNA template into a protein microarray by cell-free protein expression. This expression system based on a bacterial lysate prevents the need for genetically engineered organisms to produce every single antigen.  
 +
</br>
 +
The template slide is placed in close proximity to the future protein array enabling the expressed proteins to reach this other surface by diffusion. Complex chemistry ensures that target proteins are specifically immobilized on this surface, while components of the expression mix can be washed away before sample analysis.
 +
To obtain the DNA template, the respective sequences containing transcriptional and translational initiation sites, the antigen coding sequence and terminating regions have to be constructed and labeled with an amino group. An activated PDMS slide provides the basis for immobilization of the DNA by covalent binding of the amino group. Spotting the antigen coding sequences in a distinct pattern enables to retrace a detected binding event to a certain disease.
 +
 
 
</p>
 
</p>
</div>
+
 
</div>
+
 
 
<!-- EDIT2 SECTION "Preparing the DiaCHIP" [352-1230] -->
 
<!-- EDIT2 SECTION "Preparing the DiaCHIP" [352-1230] -->
<div class="floatbox right">
+
<h2 class="sectionedit3">Step 2: Measuring serum samples using iRIf</h2>
<h2 class="sectionedit3">Measuring</h2>
+
<div class="level2">
+
 
<p>
 
<p>
 
<!--korrigiert von Philipp05/09/15-->
 
<!--korrigiert von Philipp05/09/15-->
With the iRIf (Abkürzung) system it is possible to record small changes in layer thickness. The binding of an antibody, present in the blood serum flushed through the chamber, to the according antigen increases the local thickness of the protein surface so that interaction events can be measured label-free and in real-time via the change of the optical properties at this spot.
+
<!--neu von Ramona08/09/15-->
 +
After preparation of the DiaCHIP, a patient’s serum sample can be flushed over the protein array. The binding of antibodies to the protein surface causes a minimal change in the thickness of the slide right at the corresponding antigen spot. This change can be measured without the need for a further label with a new method called iRIf (imaging reflectometric interference). Based on the interference of light beams reflected on different thin layers, binding events can be recorded in real-time.  
 
</p>
 
</p>
 
<p>
 
<p>
But we didn't stop thinking about the device: <a href="https://2015.igem.org/Team:Freiburg/Results">We detected antibodies in our own blood!</a>
+
After weeks of opimizing the different components of the DiaCHIP, we reveal our great results. The highlight of our project was reached with the successful <a href="https://2015.igem.org/Team:Freiburg/Results">detection of antibodies in our own blood!</a>
 
</p>
 
</p>
 
</div>
 
</div>

Revision as of 20:30, 8 September 2015

""

  • Building our own device

    The original measuring device we were using in collaboration with AG Roth is a really expensive machine based on rather simple physics. Therefore, we decided to build our own device in a cost-efficient variant. We performed reliable measurements with it and provide a building plan making label-free proteinarray analysis available for every future iGEM team.

    Want to read more?

  • Communicating science

    Fast and reliable disease diagnostic is a problem of public interest. For this reason we wanted to know what people think about the idea of the DiaCHIP. Although the DiaCHIP is concerned to synthetic biology, which makes people feel rather uncomfortable according to a survey by Leopoldina (national academy of science), we obtained a lot of positive feedback.

    Want to read more?

  • Modeling cellfree expression

    In order to optimize the DiaCHIP for future applications, we modelled the process of cell-free expression and diffusion over time. Making use of xxx parameters and xxx ordinary differential equations, we computed the size of the resulting antigen spots and identified the factors limiting cell-free expression in the DiaCHIP.

    Want to read more?

  • Measuring our own blood

    One of the most notable results we obtained was the detection of anti-tetanus antibodies in human blood serum. Using the DiaCHIP, we were able to distinguish serum samples of a person taken before vaccination and three weeks later. As expected, antibody binding events were shown after vaccination, whereas there was no signal before.

    Want to read more?

Project overview: The DiaCHIP

DiaCHIP_Sabi

The DiaCHIP is an innovative tool to simultaneously and differentially detect antibodies present in blood sera in response to an infectious disease. It bears the potential to greatly simplify broad band screenings, detection of autoimmune diseases and the determination of vaccination statuses. Especially in case of threatening infections accompanied by similar symptoms fast and reliable differentiation could save lives.
To account for a disease by verification of corresponding antibodies in a patient’s blood serum is a well-known and routinely used system in modern diagnostics (LINK – diagnostics today). Thus, a simple blood sample is sufficient to perform reliable diagnostics with the DiaCHIP.
The key feature in the concept of the DiaCHIP is the combination of on-demand protein synthesis and a novel, label-free detection method in one device. This enables to overcome challenges in storage and handling that occur with currently available tests. Additionally, diagnoses can be received faster and in a more cost-efficient way than until now. Nonetheless, the whole device is so simple that it can easily be rebuilt and utilized by future iGEM teams (LINK – new device).

Step 1: Preparing the DiaCHIP by protein synthesis

Before being able to screen for antibody-antigen interactions, antigens have to be synthesized and immobilized in a microarray arrangement. This is obtained by a copying mechanism transforming a DNA template into a protein microarray by cell-free protein expression. This expression system based on a bacterial lysate prevents the need for genetically engineered organisms to produce every single antigen.
The template slide is placed in close proximity to the future protein array enabling the expressed proteins to reach this other surface by diffusion. Complex chemistry ensures that target proteins are specifically immobilized on this surface, while components of the expression mix can be washed away before sample analysis. To obtain the DNA template, the respective sequences containing transcriptional and translational initiation sites, the antigen coding sequence and terminating regions have to be constructed and labeled with an amino group. An activated PDMS slide provides the basis for immobilization of the DNA by covalent binding of the amino group. Spotting the antigen coding sequences in a distinct pattern enables to retrace a detected binding event to a certain disease.

Step 2: Measuring serum samples using iRIf

After preparation of the DiaCHIP, a patient’s serum sample can be flushed over the protein array. The binding of antibodies to the protein surface causes a minimal change in the thickness of the slide right at the corresponding antigen spot. This change can be measured without the need for a further label with a new method called iRIf (imaging reflectometric interference). Based on the interference of light beams reflected on different thin layers, binding events can be recorded in real-time.

After weeks of opimizing the different components of the DiaCHIP, we reveal our great results. The highlight of our project was reached with the successful detection of antibodies in our own blood!