Difference between revisions of "Team:ETH Zurich/Chip"

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<h2>Results and accomplishments</h2>
 
<h2>Results and accomplishments</h2>
<p> Find our results and accomplishments in the<a href="https://2015.igem.org/Team:ETH_Zurich/Results"> Results</a> section.</p>
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<li>We co-cultured bacteria and mammalian cells in the chip successfully.</li>  
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<p> We implemented a testing system for singel cell analysis in a nanowellplate and were able to <a href="https://2015.igem.org/Team:ETH_Zurich/Results#Towards_a_more_sensitive_lactate_dependent_system">detect lactate produced by singel mammalian cells</a>. Also, we co-cultured bacteria and mammalian cells in the chip successfully.<p>  
<li>We measured the lactate production of Jurkat cell in the chip, thanks to our lactate sensing bacteria .</li>  
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<p>Thanks to this experiment, we could show that we can introduce a coherent number of bacteria and mammalian cells into the chip. The aim was to obtain single mammalian cells in the chip with 1000 times more bacteria. The loading of the bacteria and mammalian cells is described <a href="https://2015.igem.org/Team:ETH_Zurich/Experiments#Loading_of_Mammalian_Cells_and_bacteria">elsewhere</a>.</p>
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<p> To visualize the mixture of cells, we used bacteria expressing RFP and 3T3 P65 cells, whose nuclei display green fluorescence.</p>
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<h4>Results</h4>
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<p> We can nicely see that the 3T3 are attaching to the chip.</p>
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Revision as of 15:36, 18 September 2015

"What I cannot create I do not understand."
- Richard Feynmann

Chip Design

Our Different designs

Introduction and first idea

First concept of microfluidic chip

One of the biggest challenges of detecting circulating tumor cells is their scarcity in the blood of patients. To overcome this problem, our first idea was to develop a microfluidic chip in order to perform single cell analysis. The biggest advantage of using a microfluidic chip is its ability to perform high-throughput cell biology. In order to do so, we wanted to produce water-in-oil emulsion droplets, that can then be sorted or analyzed by a machine analogous to FACS, (inspired from [Chiu 2015]). In the droplets, a mixture of bacteria and mammalian cells would be present. And the bacteria would express the green fluorescent protein only in the presence of cancer cells, exhibiting both increased lactate production rate and sensitivity to sTRAIL.

First Design

First design of microfluidic chip: On the figure, the orange layer represents the pressure control of the valves and the red layer represents the flow layer.

However, due to the complexity of this setup, we decided to first explore another design consisting of valves and chambers. Instead of having droplets to isolate single cells, we wanted to have a two-layer microfluidic chip. One of the layer would be the flow layer, where cells are flushed in. The other layer would consist of microfluidic valves, controlled by an external pressure source, and capable of occluding the flow layer. Thus, small chambers separating single cells could be formed. We drew the designs using Autocad.

Realistic and Final Design

Because of time constraints, we did not make the previous chip but instead we designed a "nano-well" plate which represents our proof of principle. Here, there is no flow going through the chip. Characteristics of the chip

  • The volume of every well is 1nL.
  • There are 4992 wells in our chip.

Final design of the microfluidic chip

Results and accomplishments

We implemented a testing system for singel cell analysis in a nanowellplate and were able to detect lactate produced by singel mammalian cells. Also, we co-cultured bacteria and mammalian cells in the chip successfully.

Thanks to this experiment, we could show that we can introduce a coherent number of bacteria and mammalian cells into the chip. The aim was to obtain single mammalian cells in the chip with 1000 times more bacteria. The loading of the bacteria and mammalian cells is described elsewhere.

To visualize the mixture of cells, we used bacteria expressing RFP and 3T3 P65 cells, whose nuclei display green fluorescence.

Results

We can nicely see that the 3T3 are attaching to the chip.

We would like to thank our sponsors