Difference between revisions of "Team:ShanghaitechChina/Biofilm"

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         <h3 class="bg">Principles of methods of characterization</h3>
 
         <h3 class="bg">Principles of methods of characterization</h3>
 
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         <button type="button" id="1"><p><b>Congo Red Assay:</b></p></button>
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         <p><button type="button" id="1"><b>Congo Red Assay:</b></button></p>
 
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Congo Red dye is a classic method to detect amyloid protein [2]. Amyloid can be visualized and quantified through the staining of Congo Red because Congo Red molecules obtain an oriented arrangement on amyloid fibrils. This property can be ascribed to the hydroxyl groups on the amyloid and hydrogen bonding on the Congo Red [3]. It only takes approximately 20 minutes to dye so it is indeed a good practice in lab to crudely test the expression of biofilms.<p></p></div>   
 
Congo Red dye is a classic method to detect amyloid protein [2]. Amyloid can be visualized and quantified through the staining of Congo Red because Congo Red molecules obtain an oriented arrangement on amyloid fibrils. This property can be ascribed to the hydroxyl groups on the amyloid and hydrogen bonding on the Congo Red [3]. It only takes approximately 20 minutes to dye so it is indeed a good practice in lab to crudely test the expression of biofilms.<p></p></div>   
<button type="button" id="2"><p ><b>Crystal Violet Assay:</b></p></button>
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<p ><button type="button" id="2"><b>Crystal Violet Assay:</b></button></p>
 
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Crystal violet is a triarylmethane dye used as a histological stain to classify biomass. This is a simple assay practical and useful for obtaining quantitative data about the relative quantity of cells which adhere to multi-wells cluster dishes. After solubilization, the amount of dye taken up by the monolayer can be quantitated in a plate reader. [4]<p></p>
 
Crystal violet is a triarylmethane dye used as a histological stain to classify biomass. This is a simple assay practical and useful for obtaining quantitative data about the relative quantity of cells which adhere to multi-wells cluster dishes. After solubilization, the amount of dye taken up by the monolayer can be quantitated in a plate reader. [4]<p></p>
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<p style="text-align:center"><b>Fig 1. </b> Crystal violet and Congo Red reagent.</p>
 
<p style="text-align:center"><b>Fig 1. </b> Crystal violet and Congo Red reagent.</p>
 
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<button type="button" id="3">        <p><b>Transmission Electron Microscope(TEM):</b></p></button>
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<p><button type="button" id="3">        <b>Transmission Electron Microscope(TEM):</b></button></p>
 
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In order to visualize the formation and different appearance of biofilm nanowire network, we utilize transmission electron microscope to directly look into the microscopic world. TEM can visualize nano-structure with the maximal resolution of 0.2nm which is beyond the range of optical microscope. <p></p>
 
In order to visualize the formation and different appearance of biofilm nanowire network, we utilize transmission electron microscope to directly look into the microscopic world. TEM can visualize nano-structure with the maximal resolution of 0.2nm which is beyond the range of optical microscope. <p></p>
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<p style="text-align:center"><b>Fig 2. </b> TEM device at the National Center for Protein Science Shanghai.</p></div>   
 
<p style="text-align:center"><b>Fig 2. </b> TEM device at the National Center for Protein Science Shanghai.</p></div>   
<button type="button" id="4">       <p ><b>Quantum Dots Binding Assay:</b></p></button>
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<p ><button type="button" id="4">       <b>Quantum Dots Binding Assay:</b></button></p>
  
 
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Revision as of 19:38, 19 October 2016

igem2016:ShanghaiTech