Difference between revisions of "Chip for genomic integrity 2018"
Line 6: | Line 6: | ||
* Treatment of the agarose pads | * Treatment of the agarose pads | ||
* Electrophoresis | * Electrophoresis | ||
− | * | + | * Analyze of the agarose pads |
The chip should be easy to produce (either considering the materials we use or the machinery). It should be reusable. As the chip's users won't be used to work in a lab, the chip will need to be easy to use and handle. | The chip should be easy to produce (either considering the materials we use or the machinery). It should be reusable. As the chip's users won't be used to work in a lab, the chip will need to be easy to use and handle. | ||
Line 12: | Line 12: | ||
== Design == | == Design == | ||
− | We decided to make the chip the size of a microscope slide (25mm height, 75mm long), | + | We decided to make the chip the size of a microscope slide (25mm height, 75mm long), for it to be easily observable under a normal microscope. |
We will make various slides, which will need to be changed according to the step. | We will make various slides, which will need to be changed according to the step. | ||
The chip will be made for 3 pads in total. The original idea is to make one treated pad, one normal and one untreated, but the user will be able to change the conditions however he wants. | The chip will be made for 3 pads in total. The original idea is to make one treated pad, one normal and one untreated, but the user will be able to change the conditions however he wants. | ||
Line 28: | Line 28: | ||
=== Treatment of the agarose pads === | === Treatment of the agarose pads === | ||
− | After having settled, the pads | + | After having settled, the pads must be transferred into a larger well to allow them to float around in liquid. These new wells will be 18x18mm, the size of a coverslip for microscope slide. |
* One bottom slide with 3 wells of 18x18mm, 3 times deeper than the agarose pads. | * One bottom slide with 3 wells of 18x18mm, 3 times deeper than the agarose pads. | ||
− | From the previous step, remove the top slide, and return the two others slide on this step bottom slide. Remove carefully the slides and push gently the pads into their new wells. Then perform the wanted treatment by changing the liquid in the well with a pipette or | + | From the previous step, remove the top slide, and return the two others slide on this step bottom slide. Remove carefully the slides and push gently the pads into their new wells. Then perform the wanted treatment by changing the liquid in the well with a pipette or Paster's pipette. |
''To check: is a top slide needed to perform the treatments'' | ''To check: is a top slide needed to perform the treatments'' | ||
=== Electrophoresis === | === Electrophoresis === | ||
− | + | To make an electrophoresis, we need two electrodes. We also need the agarose pads to be in contact with the liquid. The bottom slide for this test is the most complex of our slides. | |
* One bottom slide with three wells of 18x18mm, XXX µm deep, inside a bigger well less deep XXX µm, flanked by two deeper wells for the electrodes | * One bottom slide with three wells of 18x18mm, XXX µm deep, inside a bigger well less deep XXX µm, flanked by two deeper wells for the electrodes | ||
* One top slide with two holes for the liquid and two for the electrodes. The electrodes will be attached to this slide. The holes will all be above the electrode's wells | * One top slide with two holes for the liquid and two for the electrodes. The electrodes will be attached to this slide. The holes will all be above the electrode's wells | ||
− | Same thing as previous step | + | Same thing as previous step return the slide containing the pads into this step's bottom slide. |
− | === | + | === Analyze of the agarose pads === |
The 18x18mm wells are the size of a common coverslip. Thus, removing the top of the chip, removing most liquid and adding a coverslip over the three 18x18mm wells should permit the observation of the pads under the microscope. | The 18x18mm wells are the size of a common coverslip. Thus, removing the top of the chip, removing most liquid and adding a coverslip over the three 18x18mm wells should permit the observation of the pads under the microscope. | ||
Line 48: | Line 48: | ||
== Challenges & Problems == | == Challenges & Problems == | ||
− | * The chip does not for the moment enable the concentration of the cells into a small volume. We do perform two centrifugations in the lab, we | + | * The chip does not for the moment enable the concentration of the cells into a small volume. We do perform two centrifugations in the lab, we must see if just letting the cells settle down by gravity would be enough. |
* The chip slide would be easily observable under a microscope, but maybe more challenging to do a slide observable with a DIY microscope (like a foldscope). | * The chip slide would be easily observable under a microscope, but maybe more challenging to do a slide observable with a DIY microscope (like a foldscope). | ||
− | * The chip requires movement of the pads from one slide to another, maybe we should at least label the slides a certain way to make sure not to mix the pads by | + | * The chip requires movement of the pads from one slide to another, maybe we should at least label the slides a certain way to make sure not to mix the pads by inadvertence. |
Revision as of 08:15, 28 August 2018
Goals
As many steps of the comet cell assay should be carried out on the chip.
- Concentration of the cells by centrifugation
- Creation of the agarose pads
- Treatment of the agarose pads
- Electrophoresis
- Analyze of the agarose pads
The chip should be easy to produce (either considering the materials we use or the machinery). It should be reusable. As the chip's users won't be used to work in a lab, the chip will need to be easy to use and handle.
Design
We decided to make the chip the size of a microscope slide (25mm height, 75mm long), for it to be easily observable under a normal microscope. We will make various slides, which will need to be changed according to the step. The chip will be made for 3 pads in total. The original idea is to make one treated pad, one normal and one untreated, but the user will be able to change the conditions however he wants.
Concentration of the cells by centrifugation
This step is not implemented in the device yet.
Creation of the agarose pads
For this first step, we thought about using 3 slides. A top one, a middle one and a bottom one.
- The top one will contain 6 holes, 2 for each pad (entry and exit hole if overflow)
- The middle one will be thin (if possible 50µm or 100µm thick), and contain three holes of 15x15mm for the three pads
- The bottom one will be a full normal slide
To check: is the top pad really necessary
Treatment of the agarose pads
After having settled, the pads must be transferred into a larger well to allow them to float around in liquid. These new wells will be 18x18mm, the size of a coverslip for microscope slide.
- One bottom slide with 3 wells of 18x18mm, 3 times deeper than the agarose pads.
From the previous step, remove the top slide, and return the two others slide on this step bottom slide. Remove carefully the slides and push gently the pads into their new wells. Then perform the wanted treatment by changing the liquid in the well with a pipette or Paster's pipette.
To check: is a top slide needed to perform the treatments
Electrophoresis
To make an electrophoresis, we need two electrodes. We also need the agarose pads to be in contact with the liquid. The bottom slide for this test is the most complex of our slides.
- One bottom slide with three wells of 18x18mm, XXX µm deep, inside a bigger well less deep XXX µm, flanked by two deeper wells for the electrodes
- One top slide with two holes for the liquid and two for the electrodes. The electrodes will be attached to this slide. The holes will all be above the electrode's wells
Same thing as previous step return the slide containing the pads into this step's bottom slide.
Analyze of the agarose pads
The 18x18mm wells are the size of a common coverslip. Thus, removing the top of the chip, removing most liquid and adding a coverslip over the three 18x18mm wells should permit the observation of the pads under the microscope.
Challenges & Problems
- The chip does not for the moment enable the concentration of the cells into a small volume. We do perform two centrifugations in the lab, we must see if just letting the cells settle down by gravity would be enough.
- The chip slide would be easily observable under a microscope, but maybe more challenging to do a slide observable with a DIY microscope (like a foldscope).
- The chip requires movement of the pads from one slide to another, maybe we should at least label the slides a certain way to make sure not to mix the pads by inadvertence.