Team:Valencia/Parts/UCP76deleted

From 2008.igem.org

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(UCP 76 deleted)
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[[Image:Sequence UCP 76 deleted.jpg]]
[[Image:Sequence UCP 76 deleted.jpg]]
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''' Graphic about the growth of four different strains of Saccharomyces cerevisiae transformed with four kinds of UCP genes:'''
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</div>
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</div>
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<h3> Strains growth </h3>
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Apart from monitoring temperature evolution, we also characterized O.D. variations of each of our strains. We took O.D. measures every one a half hours for nine hours. We carried out this experiment both  in Erlenmeyer flasks in the 30ºC shaking stove and in our LCCs.
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This measurements were useful in order to determine some parameters for our Black Box Model. Besides, we were able to prove that the UCP was indeed being produced even though we could not see the temperature increase. Since our mutant strains Gly175Δ and Gly76Δ  do not have the same growing rate as UCP+ when they are expressing the protein, the difference between the results in the strains showed that the reason for our lack of temperature increase was that we had not found the optimum conditions yet. This results made us keep on working until we obtained successful results.
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[[Image:Creixement.jpg]]
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Strains growth equations:
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{|
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Y axis = Population in OD (optic density) units.
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|[[Image:UCP_grf_negativo.jpg|left|450px]]
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X axis = Time in hours.
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|[[Image:UCP+++.PNG|right|450px]]
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|-
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</div>
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|[[Image:UCP_mas.jpg|left|450px]]
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</div>
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|[[Image:175tumadre.PNG|right|450px]]
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|}

Revision as of 05:15, 27 October 2008




UCP 76 deleted

The uncoupling protein UCP 76 deleted is a proton carrier which is obtaines from the direct mugenesis of the Ucp1 gene. Ucp 76 has a deletion in the triplet the encodes for the Glycine 76. The mutant shows a generation time and an heat up capacity higher than UCP1. UCP 76 deleted uncouples the respiratory chain of ATP production, converting the metabolic energy in heat. The mutant shows a generation time and an heat up capacity higher than UCP1.


UCP function in mitochondria


UCP 76 deleted is a 33kd protein. The protein has a tripartite structure. The structure displays an around 100 residues region which is three times repeated. Each part encodes for two transmembrane segments and one long hydrophilic loop.The functional carrier unit is an homodimer.

Structure.jpg


The main difference between UCP 76 deleted and most of the proteins with a nuclear codification is the lack of the importation targeting to the mitochondria in UCP 76 deleted proteins.

The condition that determines the mitochondria as the protein target lays in the first loop which protudes in the mitochondrial matrix.

The second loop of the matrix is essential for the insertion of the protein in the inner mitochondrial matrix.

That protein is without direct regulation and its generation time depends on the inner activity the protein.


Sequence:

Sequence UCP 76 deleted.jpg

Strains growth

Apart from monitoring temperature evolution, we also characterized O.D. variations of each of our strains. We took O.D. measures every one a half hours for nine hours. We carried out this experiment both in Erlenmeyer flasks in the 30ºC shaking stove and in our LCCs. This measurements were useful in order to determine some parameters for our Black Box Model. Besides, we were able to prove that the UCP was indeed being produced even though we could not see the temperature increase. Since our mutant strains Gly175Δ and Gly76Δ do not have the same growing rate as UCP+ when they are expressing the protein, the difference between the results in the strains showed that the reason for our lack of temperature increase was that we had not found the optimum conditions yet. This results made us keep on working until we obtained successful results.

Strains growth equations:

UCP grf negativo.jpg
UCP+++.PNG
UCP mas.jpg
175tumadre.PNG