Team:Leicester/August2012

From 2012.igem.org

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<p>(9:30 am) Several members of the team are given wrong start times, so only 1 student arrived in the lab at 9:30, however with the work needed to be done all the rest of the team are quickly on their way.</p>
<p>(9:30 am) Several members of the team are given wrong start times, so only 1 student arrived in the lab at 9:30, however with the work needed to be done all the rest of the team are quickly on their way.</p>
<p>(10:30 am) With everyone now in the lab it turns out a lot of the work planned for today has to wait until tomorrow. This is due to the ''Pseudomonas'' strains needed to be grown in a rich luria broth before we can spin it into a pellet and then run the DNA extraction.</p>
<p>(10:30 am) With everyone now in the lab it turns out a lot of the work planned for today has to wait until tomorrow. This is due to the ''Pseudomonas'' strains needed to be grown in a rich luria broth before we can spin it into a pellet and then run the DNA extraction.</p>
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<p>(11:40 am) With all the bacteria placed in the 15ml corning tubes, and placed in the orbital shaker all of today's labwork is complete. Now the team is going to finish the recording for the rockethub video as some scenes need to be retaken, then go home for individual research/work.</p>
+
<p>(11:40 am) With all the bacteria placed in the 15ml corning tubes, and placed in the orbital shaker all of today's labwork is complete. Now the team is going to finish the recording for the rockethub video as some scenes need to be retaken, then do some individual research/work.</p>
 +
<p>(13:30 pm) After consulting with a supervisor and having a long meeting over lunch the team has decided several directions that is needed to go in. One member is testing the cooling times of a water bath that will be used in the hybridizing process of making our DNA libraries, and to start selecting out of the DNA genes that are in both our Pseudomonas and the NB26 strain that definitely degrades polystyrene. A couple of members are looking through protocol and methods to use with the DNA extraction.</p>
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Revision as of 12:57, 1 August 2012

    Wednesday 1st August 2012

(9:30 am) Several members of the team are given wrong start times, so only 1 student arrived in the lab at 9:30, however with the work needed to be done all the rest of the team are quickly on their way.

(10:30 am) With everyone now in the lab it turns out a lot of the work planned for today has to wait until tomorrow. This is due to the ''Pseudomonas'' strains needed to be grown in a rich luria broth before we can spin it into a pellet and then run the DNA extraction.

(11:40 am) With all the bacteria placed in the 15ml corning tubes, and placed in the orbital shaker all of today's labwork is complete. Now the team is going to finish the recording for the rockethub video as some scenes need to be retaken, then do some individual research/work.

(13:30 pm) After consulting with a supervisor and having a long meeting over lunch the team has decided several directions that is needed to go in. One member is testing the cooling times of a water bath that will be used in the hybridizing process of making our DNA libraries, and to start selecting out of the DNA genes that are in both our Pseudomonas and the NB26 strain that definitely degrades polystyrene. A couple of members are looking through protocol and methods to use with the DNA extraction.

    Thursday 2nd August 2012

(9:30 am) Today the team is going to start creating a DNA library of the ''Pseudomonas. sp'' so that once the NB26 strain arrives it can be compared straight away to give an idea which genes could be involved in the degredation of polystyrene and to help start narrowing our search.

To create the library a few things need to be known: Is the bacteria gram positive or negative? Is the DNA chromosomal or plasmid? How much DNA is going to be extracted? All ''Pseudomonas'' is gram negative, and the team wants to extract as much of the plasmid DNA as possible, as this is where the team thinks the polystyrene degredation enzyme is located. With all these answered the group can collect the right DNA extraction kit and start working.

    Friday 3rd August 2012

No entry for this date.

    Saturday 4th August 2012

No entry for this date.

    Sunday 5th August 2012

No entry for this date.

    Monday 6th August 2012

No entry for this date.

    Tuesday 7th August 2012

No entry for this date.

    Wednesday 8th August 2012

No entry for this date.

    Thursday 9th August 2012

No entry for this date.

    Friday 10th August 2012

No entry for this date.

    Saturday 11th August 2012

No entry for this date.

    Sunday 12th August 2012

No entry for this date.

    Monday 13th August 2012

No entry for this date.

    Tuesday 14th August 2012

No entry for this date.

    Wedesnday 15th August 2012

No entry for this date.

    Thursday 16th August 2012

No entry for this date.

    Friday 17th August 2012

No entry for this date.

    Saturday 18th August 2012

No entry for this date.

    Sunday 19th August 2012

No entry for this date.

    Monday 20th August 2012

No entry for this date.

    Tuesday 21st August 2012

No entry for this date.

    Wedesnday 22nd August 2012

No entry for this date.

    Thursday 23rd August 2012

No entry for this date.

    Friday 24th August 2012

No entry for this date.

    Saturday 25th August 2012

No entry for this date.

    Sunday 26th August 2012

No entry for this date.

    Monday 27th August 2012

No entry for this date.

    Tuesday 28th August 2012

No entry for this date.

    Wednesday 29th August 2012

No entry for this date.

    Tuesday 30th August 2012

No entry for this date.

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