Difference between revisions of "Team:Uppsala/Worm Culturing"

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<h1>Introduction</h1>
 
<h1>Introduction</h1>
         <p id="Over">The main goal of our project has been the creation of a diagnostic tool for detecting the level of infestation of small strongyles (or <i>cyathostomins</i>) in horse faeces. For this purpose, transcriptomics and phage display analysis have been performed. These techniques, however, require large amounts of clean sterilized strongyles.<br>
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         <p id="Over">The main goal of our project has been the creation of a diagnostic tool for detecting the level of infestation of small strongyles (or <i>cyathostomins</i>) in horse feces. For this purpose, transcriptomics and phage display analysis have been performed. These techniques, however, require large amounts of clean sterilized strongyles.<br>
 
For this reason, the first part of our project has been the recovery and the processing of the nematodes, to obtain samples usable for the following segments of the project. The co-culturing between nematodes and <i>E. coli</i> has then been performed with the obtained strongyles. This process requires, in fact, the presence of only strongyles and bacteria.<br>
 
For this reason, the first part of our project has been the recovery and the processing of the nematodes, to obtain samples usable for the following segments of the project. The co-culturing between nematodes and <i>E. coli</i> has then been performed with the obtained strongyles. This process requires, in fact, the presence of only strongyles and bacteria.<br>
 
     While dealing with this task, however, many times our group has faced one problem: the lack of information. Not much, in fact, has been published about strongyles and techniques to handle them. For this reason, this first part of the project often involved the adaptation of a pre-existing protocol or the creation of entirely new ones.</p>
 
     While dealing with this task, however, many times our group has faced one problem: the lack of information. Not much, in fact, has been published about strongyles and techniques to handle them. For this reason, this first part of the project often involved the adaptation of a pre-existing protocol or the creation of entirely new ones.</p>
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                           <p>In order to establish the protocols for the recovery of the nematodes from the faeces, a process of trial and error has proven necessary. This has lead to the process being divided in 4 main steps: </p>
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                           <p>In order to establish the protocols for the recovery of the nematodes from the feces, a process of trial and error has proven necessary. This has lead to the process being divided in 4 main steps: </p>
  
 
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     <p>From the faecal samples provided by Vidilab we needed to extract the worms in order to perform experiments on them later. For each extraction, approximately 20 g of faeces are used.</p><br>       
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     <p>From the faecal samples provided by Vidilab we needed to extract the worms in order to perform experiments on them later. For each extraction, approximately 20 g of feces are used.</p><br>       
                 <p>The first step is the incubation of the faeces in a plastic cup in a 29 degree oven for one week. During this time the eggs hatch and the nematodes reach the third larval stage. This is the infectious stage of the strongyles and the end of its development in the faeces/grass.</p>   
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                 <p>The first step is the incubation of the feces in a plastic cup in a 29 degree oven for one week. During this time the eggs hatch and the nematodes reach the third larval stage. This is the infectious stage of the strongyles and the end of its development in the feces/grass.</p>   
 
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                             <p><b>Figure 2.</b> Measurement of faeces for incubation.<br></p>
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                             <p><b>Figure 2.</b> Measurement of feces for incubation.<br></p>
 
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Revision as of 01:46, 18 October 2018