Team:Valencia/WetLab/YeastTeam/Results

From 2009.igem.org

(Difference between revisions)
(Experimental results)
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== '''Experimental results''' ==
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='''Experimental results'''=
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Our ultimate goal was to make a bio-screen made with cellular pixels (LECs). But, before to be able to build this iLCD, we had to study the behaviour of one single LEC. Therefore, we focused on the electrical excitation of our transformed yeasts.
Our ultimate goal was to make a bio-screen made with cellular pixels (LECs). But, before to be able to build this iLCD, we had to study the behaviour of one single LEC. Therefore, we focused on the electrical excitation of our transformed yeasts.
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This is the behaviour that stands as the cornerstone of our project. With a serie of voltage inputs, we acomplished a series of light emissions. No exciting light was needed, only aequorin, coelenterazine and Ca<sub>2+</sub>.
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This is the behaviour that stands as the cornerstone of our project. With a serie of voltage inputs, we acomplished a series of light emissions. No exciting light was needed, only aequorin, coelenterazine (the prosthetic group) and Ca<sup>2+</sup>.
graph continu amb dos pics
graph continu amb dos pics
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We have investigated a set of different voltages and times in order to precisely know how is the reaction of our system to electric current. Knowing this, we could control it properly. Therefore, we have taken advantage of the different experimental designs we had at a glance: we had several calcium channel knock outs (''mid1'' and ''ch1''), as well as functional inhibitors of the calcium channels (KCl) and divalent ion quelant (EDTA).
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We have investigated a set of different voltages and times in order to precisely know how is the reaction of our system to electric current. Knowing this, we could control it properly.  
We will show and explain here the major results, for a thorough description of the behaviour of the aequorin light emission system please refer to the [https://2009.igem.org/Team:Valencia/Parts/Characterization Characterization page] or to the [http://partsregistry.org/wiki/index.php?title=Part:BBa_K222000 Registry].
We will show and explain here the major results, for a thorough description of the behaviour of the aequorin light emission system please refer to the [https://2009.igem.org/Team:Valencia/Parts/Characterization Characterization page] or to the [http://partsregistry.org/wiki/index.php?title=Part:BBa_K222000 Registry].
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===Controls===
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In every little step in a molecular biology laboratory, one has to bear in mind the use of negative controls for every logical step of the hypothesis.
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Therefore, we have taken advantage of the different experimental designs that were available: we had several calcium channel knock outs (''mid1'' and ''ch1''), as well as functional inhibitors of the calcium channels (KCl) and divalent ion quelant (EDTA).
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 +
All these designs were used in order to reject the idea of looking to an artifact.
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[[Image:Comparació_disc.jpg|700 px]]
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This graph shows the behaviour of a set of designs after tha supply of a 4V shock.
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* '''WT''' is our wild type luminiscent cell, with coelenterazine and fully working calcium channels
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* '''Mid1''' is a knock out for a calcium channel. Light is not observed because Ca2+ can’t enter into the cell and bind to the aequorin-coelenterazine complex.
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* '''Cch1''' is another knock out mutant for a calcium channel, so the absence of light can be explainned in the same way.
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* '''EDTA''' is a divalent ion quelant, so Ca2+ is quenched and not useful for the light emission, although every compound necessary for the reaction is present.
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* '''SD +coe''' is growth media with coelenterazine, just to be sure that without cells we had no light.
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* '''SD''' is plain growth media.
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* '''yeast -coe''' is our wild type luminiscent cell, without coelenterazine, the prosthetic group that is needed for the light emission.
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===Voltage===
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Varying exciting time and voltage we can have a variety of responses (arrows indicate electric current supply):
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{|
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|[[Image:1,5V 10s.jpg|center|400px]]
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|[[Image:4,5V 5s.jpg|center|400px]]
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</center>
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===Supply time===
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[[Image:Manteniment resposta disc.jpg|center|thumb|700px| Here, we can see that the process can be repeat consecutively]]
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[[Image:Manteniment resposta disc.jpg|center|thumb|700px| Here, we can see that the process can be repeat consecutively]]
[[Image:Manteniment resposta disc.jpg|center|thumb|700px| Here, we can see that the process can be repeat consecutively]]
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<!-- [[Image:Combinació.jpg|center|thumb|700px| Comparation of the repetibility between our yeasts, our yeasts without coelenterazine, medium whit coelenterazine and mutants]]
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[[Image:Combinació.jpg|center|thumb|700px| Comparation of the repetibility between our yeasts, our yeasts without coelenterazine, medium whit coelenterazine and mutants]]
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Revision as of 17:37, 21 October 2009




Experimental results


Our ultimate goal was to make a bio-screen made with cellular pixels (LECs). But, before to be able to build this iLCD, we had to study the behaviour of one single LEC. Therefore, we focused on the electrical excitation of our transformed yeasts.

This is the behaviour that stands as the cornerstone of our project. With a serie of voltage inputs, we acomplished a series of light emissions. No exciting light was needed, only aequorin, coelenterazine (the prosthetic group) and Ca2+.

graph continu amb dos pics

We have investigated a set of different voltages and times in order to precisely know how is the reaction of our system to electric current. Knowing this, we could control it properly.

We will show and explain here the major results, for a thorough description of the behaviour of the aequorin light emission system please refer to the Characterization page or to the [http://partsregistry.org/wiki/index.php?title=Part:BBa_K222000 Registry].

Controls

In every little step in a molecular biology laboratory, one has to bear in mind the use of negative controls for every logical step of the hypothesis. Therefore, we have taken advantage of the different experimental designs that were available: we had several calcium channel knock outs (mid1 and ch1), as well as functional inhibitors of the calcium channels (KCl) and divalent ion quelant (EDTA).

All these designs were used in order to reject the idea of looking to an artifact. Comparació disc.jpg This graph shows the behaviour of a set of designs after tha supply of a 4V shock.

  • WT is our wild type luminiscent cell, with coelenterazine and fully working calcium channels
  • Mid1 is a knock out for a calcium channel. Light is not observed because Ca2+ can’t enter into the cell and bind to the aequorin-coelenterazine complex.
  • Cch1 is another knock out mutant for a calcium channel, so the absence of light can be explainned in the same way.
  • EDTA is a divalent ion quelant, so Ca2+ is quenched and not useful for the light emission, although every compound necessary for the reaction is present.
  • SD +coe is growth media with coelenterazine, just to be sure that without cells we had no light.
  • SD is plain growth media.
  • yeast -coe is our wild type luminiscent cell, without coelenterazine, the prosthetic group that is needed for the light emission.

Voltage

Varying exciting time and voltage we can have a variety of responses (arrows indicate electric current supply):

1,5V 10s.jpg
4,5V 5s.jpg

Supply time

Here, we can see that the process can be repeat consecutively


characterize the cell light emission if we wanted to control it better. We thought about two possible ways to make cells produce light: First, the producion of light with a chemical imput and, second, making the cells glow with electricity. we choose the calcium signaling because it is the fastest known modality of signaling in biology, and will allow for a fast refreshing rate of the screen.

Chemical input


In order to make our yeasts produce light, we firstly reproduce experiments made by Viladevall et al, after a lot of different trials, we finally could characterize the luminiscence curve in a discontinuos luminometer.

Comparació koh.jpg

As we can see in the graph, a peak of light is emited about 450 seconds after the addition 60 microliters of KOH to 170 microliters of medium with WT transformed yeasts. Although we were almost sure that the mechanism that triggered that flash of light was the expected, we preferred to make the same experiment with different kind of controls and make sure we were not observing any artiffact:

  • Mid1: one knock out mutant for a Calcium channel. Light is not observed because Ca2+ can’t enter into the cell and bind to the aequorin-coelenterazine complex.
  • Cch1: another knock out mutant for Calcium channel, so the absence of light can be explainned in the same way.
  • EDTA: Although every compound necessary for the reaction is present (including Ca2+ channels) light is not emited because EDTA is a divalent ion quelant, so Ca2+ is quenched and not useful for the emission.
  • KCl: another negative control. The absence of the -OH group prevents the opening of calcium channels and makes yeast produce no light.


We wanted to characterize in detail this kind of response. To complete the work with the chemical input, we though KOH amounts could influence in the quantity of emitted light, so we repited the experiment with different concentrations of KOH.

Light emission under diferent concentrations of the chemical input

As we can see, the volume of KOH added (from 15 microliters to 120) is related to the luminiscent peak. Although there is not linearly proportional, luminiscence intensity is increased when we increase the quantity of KOH we put in the sample (always 170 microliters of medium with yeasts).

Characterising the response to the KOH we also found interesting to determinate the reproducibility of the process.


Repetibilitat KOH.jpg


By adding 30 microliters of KOH at certain times (arrows), we discovered that after the first peak, cells couldn’t return to the basals levels, and every new shock make yeasts produce light in higher levels than the last one.

Electrical input


When the experiments with an alkali input showed us that yeasts were able to produce light because of their transformation, we tried our ambitious goal: stimulate calcium channels with an electrical input.

We use two luminometers, one luminometer discontinuous and the other is continuous. Each luminometer uses different units, depends on the manufacturer. For this reasons we can't compare directly the results obtained with one luminometer with the results of the other. According this, when we only compare results in the same graph if they were obtained with the same luminometer. However, an increase (or not) in the luminosity, means the same at two luminometers and the experiments are complementary and reaffirms our conclusions.

We reproduced the mentionated Viladevall et al's protocol, incubating the transformed yeasts with coelenterazine, but changing the KOH by electricity. Surprisingly, we found that light was also produced in a very similar way. We tried with different times and voltages in order to find the optim conditions for a big peak of light. Some of our graphics are theese:

Light emitted when 1,5V are applicated during 5 seconds
Light emitted when 1,5V are applicated during 10 seconds
Light emitted when 4,5V are applicated during 5 seconds
Light emitted when 10V are applicated during 1 second
Light emitted when 10V are applicated during 2 seconds
Light emitted when 24V are applicated during 0,5 seconds

We realised that the time of exposure to the electrical stimulus was crucial, even more that the aplied voltage. That means, if we increased the voltage at very short times, cells could produce a more abrupt peak of light. But if we increased the time of exposure to the electricity, we observe a less defined response, with more flattened peaks.

That’s probably because a big exposure time of electrical input damages and killes the yeasts, making them to release their components to the medium, including the aequorin-coelenterazine-Ca2+ complex, so the emission of light is more uniform in time, instead of the production of the flash produced by the Calcium enetering in the cell.

In the case of very little voltages (like 1,5V) this observation is not carried out by our yeasts. The reason must be that the electrical input is too low, so yeasts don’t die so easily as with more elevated voltage, and a better response is produce with a more prolongated electrical shock.

6V variats disc.jpg

This graph clearly show us that using a same voltage, we obtain a better response with the shortest time of the electrical input.

Our controls discard the idea of an artifact. For example, light could be made by a spark produced during the discharge. It was not very probable, because the peak observed was produce near 400 seconds after the stimulus. But, another time, when cells without coelenterazine or mutants are used, we see no light.

Our yeasts with coelentrazine
Our yeastse without coelenterazine
Medium with coelenterazine
Mutant yeasts, deficients in calcium channels
Comparison of the results


Studying the repetibility of the process, this is a little different from the chemical stimulus, but the system has a similar behaviour, and we can stimulate several times the same sample getting a response. However, every next shock produces a fewer peak of light. We hace two hypothesis: one of them is that a part of our yeasts die meanwhile the electrical stimulus. The other one is that coelenterazine is not reusable, so a proportion of it runs down in every emission of light.

Here, we can see that the process can be repeat consecutively
Comparation of the repetibility between our yeasts, our yeasts without coelenterazine, medium whit coelenterazine and mutants