Difference between revisions of "Team:Pasteur Paris/Science"

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In order to test whether we can detect mosquito-borne pathogens by <B>immunodetection</B>, we tested antibody-antigen recognition onto <B>PVDF commercial membranes</B> by using E2 envelope protein of Chikungunya virus (<B>E2/CHIKV</B>) and <B>monoclonal E2-specific antibody 3E4</B>.  Single E2/CHIKV was conjugated with horseradish peroxydase (<B>HRP</B>) and efficiency of the detection method was tested (Fig. 7A). Then, specificity test was assessed by performing detection of conjugated E2/CHIKV among an excess of conjugated BSA (Fig. 7B). After that, since <B>mosquito proteins</B> can interfere with the E2/CHIKV recognition, we substituted BSA with conjugated <B>mosquito lysate</B> proteins (Fig. 7C). Finally, <B>"real-world" test</B> was performed by detecting <B>17D vaccine strain of Yellow Fever virus (YFV)</B> into infected mosquitoes (Fig. 7D) by a coach with the required safety access to an Institut Pasteur BHSL facility. </br></br>
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In order to test whether we can detect mosquito-borne pathogens by <B>immunodetection</B>, we tested antibody-antigen recognition onto <B>PVDF commercial membranes</B> by using E2 envelope protein of Chikungunya virus (<B>E2/CHIKV</B>) and <B>monoclonal E2-specific antibody 3E4</B>.  Single E2/CHIKV was conjugated with horseradish peroxydase (<B>HRP</B>) and efficiency of the detection method was tested (Fig. 7A). Then, specificity test was assessed by performing detection of conjugated E2/CHIKV among an excess of conjugated BSA (Fig. 7B). After that, since <B>mosquito proteins</B> can interfere with the E2/CHIKV recognition, we substituted BSA with conjugated <B>mosquito lysate</B> proteins (Fig. 7C). Finally, <B>"real-world" test</B> was performed by detecting <B>17D vaccine strain of Yellow Fever virus (YFV)</B> into infected mosquitoes (Fig. 7D) by a coach with the required safety access to an Institut Pasteur BHS facility. </br></br>
  
  
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We made the <B>composite protein-cellulose-based patch</B> by mixing cellulose powder and the pre-silicated fusion protein, and <B>compressing it<B> on a Darragon SE 10 (200 bars, 100 kN, 10T). To check the rigidity gain of the silicated patch, we can characterize the rigidity in <B>traction</B> and <B>compression</B> by measuring the <B>Young’s modulus</B> and the rigidity in shearing by measuring the <B>shear modulus</B>. Then, we coated specific antibodies to CHIKV onto the composite patch, allowing us the detection of <B>purified CHIKV envelope protein</B>.  
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We made the <B>composite protein-cellulose-based patch</B> by mixing cellulose powder and the pre-silicated fusion protein, and <B>compressing it</B> on a Darragon SE 10 (200 bars, 100 kN, 10T). To check the rigidity gain of the silicated patch, we can characterize the rigidity in <B>traction</B> and <B>compression</B> by measuring the <B>Young’s modulus</B> and the rigidity in shearing by measuring the <B>shear modulus</B>. Then, we coated specific antibodies to CHIKV onto the composite patch, allowing us the detection of <B>purified CHIKV envelope protein</B>.  
  
  

Revision as of 14:05, 19 October 2016