Difference between revisions of "Team:Cardiff Wales/projectdescription"

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<h4 align="center"> The expression system bit </h4>
 
<h4 align="center"> The expression system bit </h4>
 
<p align="center"> Our other aim was to create a transient gene expression system in <i>Nicotiana benthamiana</i>. For this, we isolated regions of four plant promoters found in <i> Arabidopsis thaliana </i>. These were constructs with inducible promoters, which were tested using the luciferase expression system. The same promotors were also used to try and create a high abundance of TSHantag. These constructs can be seen in the diagram below.</p>
 
<p align="center"> Our other aim was to create a transient gene expression system in <i>Nicotiana benthamiana</i>. For this, we isolated regions of four plant promoters found in <i> Arabidopsis thaliana </i>. These were constructs with inducible promoters, which were tested using the luciferase expression system. The same promotors were also used to try and create a high abundance of TSHantag. These constructs can be seen in the diagram below.</p>
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<p align="center">The four promoters used were PDF1, PR2, GST6, and WRKY30. PDF1 is induced by jasmonic acid, PR2 and GST6 by salicylic acid, and WRKY30 by damage associated molecular patterns (DAMPs) which in this case was the presence of cellulose. </p>
 
<p align="center">The four promoters used were PDF1, PR2, GST6, and WRKY30. PDF1 is induced by jasmonic acid, PR2 and GST6 by salicylic acid, and WRKY30 by damage associated molecular patterns (DAMPs) which in this case was the presence of cellulose. </p>
 
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Revision as of 21:04, 1 September 2017

The Project

Our project has several components. The idea was to create a potentially economically viable production platform in Nicotiana benthamiana, testing various Arabidopsis thaliana promoters that respond to different stimuli. The production platform was to be ideally used to produce high levels of therapeutic products, with the appropriate post-translational modifications (PTMs) that makes using plants as a production system more favourable than bacteria. The therapeutic product that we tried to produce was an antagonist to thyroid stimulating hormone, with the aim that this would be able to treat hyperthyroid disorders such as Graves’ disease.




The therapeutic bit

Hyperthyroidism is the name given to a group of conditions that result in an overactive thyroid gland. Both sexes can suffer from the disease but hyperthyroidism is, according to the NHS, about 10 times more common in women than in men, with the condition usually starting between 20 and 40 years of age. The increased abundance of thyroid hormones can be serious if their levels rise too much, but general symptoms include nervousness, anxiety and irritability, mood swings, fatigue, heat sensitivity, goitre, heart palpitations, trembling, twitching and weight loss. If left untreated, the condition can cause problems with the eyes (bulging and double vision), pregnancy complications such as pre-eclampsia, premature birth or miscarriage, and a potentially life threatening ‘thyroid storm’ when symptoms accumulate rapidly and unexpectedly.

Graves’ disease is an autoimmune disorder that causes the body to attack the thyroid, causing hyperthyroidism as antibodies bind to, and activate, the thyroid gland. The disease is partly heritable, with some associated genes identified, and some environmental factors such as smoking or stress increasing the risk of the disease. The antibody that attacks the thyroid gland is called thyroid stimulating immunoglobulin (TSI), which has a similar effect to thyroid stimulating hormone (TSH). Our project aims to create an antagonist (TSHantag) to these molecules, which will also bind to the thyroid gland, but will not activate it. This will prevent the native TSH and TSI binding to the thyroid, and thus should decrease the levels of thyroid hormones in the body, treating the hyperthyroidism. This should be preferable to the current treatment, which is the use of radioactive iodine which destroys the thyroid and renders patients dependent on thyroid medication for the rest of their lives.

The expression system bit

Our other aim was to create a transient gene expression system in Nicotiana benthamiana. For this, we isolated regions of four plant promoters found in Arabidopsis thaliana . These were constructs with inducible promoters, which were tested using the luciferase expression system. The same promotors were also used to try and create a high abundance of TSHantag. These constructs can be seen in the diagram below.


The four promoters used were PDF1, PR2, GST6, and WRKY30. PDF1 is induced by jasmonic acid, PR2 and GST6 by salicylic acid, and WRKY30 by damage associated molecular patterns (DAMPs) which in this case was the presence of cellulose.