Team:Valencia/Project/Lab work/2 experiments

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2.-Demonstration that thermogenin-expressing yeast strains can heat their own broth medium.

Materials

In our experiments we worked with the the following Saccharomyces cerevisiae strains kindly handed by Eduardo Rial :

UCP+ : UCP1 gene with Gal7 promoter.
UCP- : UCP1 antisense gene with Gal7 promoter. It is used as control strain.
Gly175Δ : UCP1 mutant sequence, Glycine 175 has been deleted.
Gly76Δ : UCP1 mutant sequence, Glycine 76 has been deleted. These two strains have increased uncoupling activity and do not need fatty acids to be functional.

We used plasmid pYeDP as our vector in Saccharomyces cerevisiae.

Method of culturing UCP1-producing yeast strains for heat production

Each of our experiments entails the following steps:

We prepare a 30ml inoculum for each strains in 100ml Erlenmeyer flasks with SD medium. We leave it overnight in the 28ºC stove.
We prepare a second inoculum for each strain, this time 100ml SP medium in 1L Erlenmeyer flasks. The initial O.D. of this second inoculum is adjusted to 0.2. We leave it several hours in the 28ºC stove.

The objective of this two-step protocol is to be able to start the experiment with a higher O.D. in a medium with little or no glucose. In summary: first, we grow our strains in a liquid medium with glucose (SD medium), in which they have a better growth rate. Second, we use SP medium because it has a really small amount of glucose.
We start the experiment in the LCCs with a volume of 100ml of SP medium, adjusted to O.D. of 0.6. We heat the medium up to aproximately 28ºC inside the LCC.
We add 1% galactose to each of the LCCs containing the four yeast strains. This sugar is the UCP1 gene Gal7 promoter inductor and it is therefore needed for the production of UCP1.
We monitor the temperature evolution in the LCCs thanks to our LCC system.

Experiment results

August_15th		Volume: 100 ml SP medium 250 rpm and slightly tilt. Initial OD: 0,2 O.D measured each one a a half hours during the first 9 hours (We observe each of the moments we opened LCCs for measurements. Induction at the beginning with galactose 1%. Plus extra shot at 9 hours. Left during two days.
September_24th		Volume: 100 ml SP medium 275 rpm and slightly tilt. Initial OD: 0,6 Induction at the beginning with galactose 1%.

Strains growth

Besides monitoring temperature evolution, we also compared the growth of the cultures. For this purpose, we measured O.D. of the cultures. O.D. was measured every ninety minutes for a nine hours period. We carried out this experiment both under normal culture conditions ( Erlenmeyer flasks shaken at 30ºC ) and in our thermally isolated LCCs.

This measurement was useful in order to determine the growing parameters used in the modeling of our system. Culture growth characterization through O.D. indirectly confirmed the expression and functional activity of UCP1. As expected, mutant strains (Gly175Δ and Gly76Δ) exhibited a delayed growth kinetics indicating that uncoupling activity was present. UCP- and UCP+ grew faster.The former does not produce functional thermogenine whereas the later is not functional in absence of fatty acids. These results, indicating the expression of active thermogenine, confirm those on temperature increases we found with the LCC.

Strains growth equations:

Troubleshooting

In order to establish the final conditions and protocols, we have gone through many different experiments.

Low shaking speed, large volume and low initial O.D.

We did not obtain any encouraging results.
Besides, we obtained weird oscillations in most of our experiments (as described in the LCC troubleshooting).

Media variations

YPKAc Medium : In this medium containing acetate, yeast is supposed to only respire rather than ferment. We tried it just in case the problem was that electron transport chain was inhibited.
Palmitate: although our Gly175Δ and Gly76Δ mutants do not need this compound for thermogenine activation, we tried and added it in case it made any difference for UCP+ strain. We tried and added it to both SP medium and YPKAc medium.
We did not obtain any encouraging results either.

Increased shaking speed and reduced volume

We obtained temperature increases for the first time.
Besides, the weird oscillations observed before disappeared.

Higher O.D.

In order to do so, we designed the two inoculum protocol described above. With this protocol, we intend to reach an high O.D. without having too much glucose. We used SP medium for the inoculum in order to avoid adding too much glucose (SD medium is glucose rich) to the LCCs.
We obtained temperature increases and we were able to reproduce it.
We tried and began the experiment with an even higher O.D. but we have not obtained the encouraging results yet.

Initial temperature

We put a lot more effort in starting at the same temperature every time.
Nevertheless, this temperature inside the calorimeter depends on the room temperature. And room temperature can significantly change depending on the outside temperature.

Here you can see a summary of our experiments and the different conditions for them.

LCC content	Conditions	Results and Observations
UCP+ UCP- Gly175Δ Gly76Δ	Volume: 300 ml SP medium 150 rpm Initial OD: 0,05 Induction at 3 hours (approximate OD 0.15) with galactose 0.4%	No conclusions Weird oscillations Actual O.D. at the moment of induction different for the strains and different from predicted.
UCP+ UCP- Gly175Δ Gly76Δ	Volume: 300 ml YPKAc medium 150 rpm Initial OD: 0,05 Induction at different times with 0.4% galactose and no induction	No difference between induction times No difference between induction and no induction Weird oscillations
UCP+ UCP- Gly175Δ Gly76Δ	Volume: 300 ml SP medium 150 rpm Initial OD: 0,2 Induction after 5 hours with galactose 0.4%. Actual OD between 0,8 – 1,6	No conclusions
UCP+ UCP- Gly175Δ Gly76Δ	Volume: 100 ml SP medium 250 rpm and slightly tilt. Initial OD: 0,2 Induction at the beginning with galactose 1%. Plus extra shot at 9 hours. Left during two days.	We obtained temperature increase for the first time, after a lot of hours of experiment. We were not able to reproduce it.
UCP+ UCP- Gly175Δ Gly76Δ	Volume: 100 ml SP medium 275 rpm and slightly tilt. Initial OD: 0,2 Induction after 3 hours with galactose 1%. Aprox OD 0.4	Temperature increase after a lot of hours. But thermocouples not working properly.
UCP+ UCP- Gly175Δ Gly76Δ	Volume: 100 ml SP medium 275 rpm and slightly tilt. Initial OD: 0,6 Induction at the beginning with galactose 1%.	Temperature increase. We were able to reproduce it. System very sensitive to initial temperature.
UCP+ UCP- Gly175Δ Gly76Δ	Volume: 100 ml SP medium 275 rpm and slightly tilt. Initial OD: 2 Induction at the beginning with galactose 1%.	No results. Probably, O.D. at 2 is too high to begin with.

1.LCC Construction << 2.Hot Yeast Experiments >> 3.Modeling

@@ Line 78: / Line 78: @@
 <h3> Troubleshooting </h3>
-In order to establish the final conditions and protocol, we have gone trough a lot of different experiments.
+In order to establish the final conditions and protocols, we have gone through many different experiments.
 <ol>'''Low shaking speed, large volume and low initial O.D.''' <br>
-At the beginning this were the conditions for our experiment. However,we did not want to add the inductor at such lower O.D., so we used to wait three hours of experiment before induction. <br>
+At the beginning these were the conditions for our LCC. However, since the induction should be done at higher cell densities, we had to wait three hours before induction. <br>
 *We did not obtain any encouraging results.
 *Besides, we obtained weird oscillations in most of our experiments (as described in the [[Team:Valencia/Project/Lab_work#Troubleshooting|LCC troubleshooting]]).
@@ Line 87: / Line 87: @@
-<ol>'''Medium variations''' <br>
+<ol>'''Media variations''' <br>
-As we were obtaining any results we desperately tried other mediums.
+As we were not obtaining any results, we desperately tried other culture broths.
-*[[Team:Valencia/Notebook/Protocols#YPKAc Medium | YPKAc Medium ]]: In this medium containing acetate, yeast is suppose to only breath rather than fermenting. We try it in case the problem was that electron transport chain was inhibited.
+*[[Team:Valencia/Notebook/Protocols#YPKAc Medium | YPKAc Medium ]]: In this medium containing acetate, yeast is supposed to only respire rather than ferment. We tried it just in case the problem was that electron transport chain was inhibited.
-*Palmitate: although our Gly175Δ and Gly76Δ mutants do not need this compound, we tried and added it in case it made any difference for UCP+ strain. We tried and added it to both SP medium and YPKAc medium.
+*Palmitate: although our Gly175Δ and Gly76Δ mutants do not need this compound for thermogenine activation, we tried and added it in case it made any difference for UCP+ strain. We tried and added it to both SP medium and YPKAc medium.
 *We did not obtain any encouraging results either.
 </ol>
@@ Line 96: / Line 96: @@
 <ol>'''Increased shaking speed and reduced volume'''<br>
-In other to allow proper respiration the yeast culture in the LCCs, we tried and increase the revolutions per minute of of shaker. Besides, we reduced the volume for the yeast culture to have more oxygen available.
+In other to allow proper respiration of the yeast culture in the LCCs, we tried to increase the speed of shaker. Additionally, we reduced the volume for the yeast culture to have more oxygen available.
-*We obtained temperature increase temperature increase for the first time.
+*We obtained temperature increases for the first time.
-*We were not able to reproduce it.
 *Besides, the weird oscillations observed before disappeared.
 </ol>
@@ Line 104: / Line 103: @@
 <ol>'''Higher O.D.'''<br>
-Instead of starting the experiment at a lower O.D. and waiting several hours before inducing, we thought it would be better to start at a higher O.D. Besides, we would make sure that the O.D. at the time of induction was the same for the four strains.
+Instead of starting the experiment at a lower O.D. and waiting several hours before inducing, we thought it would be better to start at a higher O.D. This way, we would be sure that the O.D. at the time of induction was the same for the four strains.
-*In order to do that, we design the two inoculum protocol described above. With this protocol, we intend to reach an elevated O.D. without having a medium with too much glucose. We added a SP medium inoculum so as to avoid adding too much SD medium (glucose rich) to the LCC.
+*In order to do so, we designed the two inoculum protocol described above. With this protocol, we intend to reach an high O.D. without having too much glucose. We used SP medium for the inoculum in order to avoid adding too much glucose (SD medium is glucose rich) to the LCCs.
-*We obtained temperature increase and we were able to reproduce it.
+*We obtained temperature increases and we were able to reproduce it.
-*We tried and begin the experiment with an even higher O.D. but we have not obtained the encouraging results in yet.
+*We tried and began the experiment with an even higher O.D. but we have not obtained the encouraging results yet.
 </ol>
 <ol>'''Initial temperature'''<br>
-Even after obtaining results that shown mutants increased culture temperature, we obtained obtained weird results were none of the strains behaved as wished. We realized those experiments where the initial temperature of the culture was higher correspond to those were we obtained weird results.
+Even after obtaining results showing that mutants increased the temperature of the culture,  we obtained weird results since none of the strains behaved as wished. We realized the disturbing factor of those experiments was the initial temperature of the culture, higher than that corresponding to the successful experiments.
 *We put a lot more effort in starting at the same temperature every time.
 *Nevertheless, this temperature inside the calorimeter depends on the room temperature. And room temperature can significantly change depending on the outside temperature.