Difference between revisions of "Team:CityU HK/Experiments"

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<div class="paragraph" style="text-align:left;"><font size="3"><span style="">To determine the level of &beta;-galactosidase encoded by <em style="">lacZ</em>, ONPG assay was performed.</span><br /><br /><span style=""></span>  <span style=""><strong>ONPG assay:</strong></span><span style="">&nbsp;<a href="https://2015.igem.org/Team:CityU_HK/Protocol#characterization" style="color: #000000"><b><u>(Link to the protocol)</u></b></a></span><br /><span style=""></span><br /><span style=""></span>  <span style="">Besides lactose, ONPG (ortho-Nitrophenyl-&beta;-galactoside) is also a substrate of &beta;-galactosidase. ONPG is digested into galactose and ortho-nitrophenol (ONP) which is yellow in colour. Chloroform was used to lyse the cells and the enzymes were released into the surrounding. By measuring the O.D. at 420 nm after lysing the cells, the level of the &beta;-galatosidase was determined.</span></font><br /><span style=""></span><br /><span style=""></span></div>
 
<div class="paragraph" style="text-align:left;"><font size="3"><span style="">To determine the level of &beta;-galactosidase encoded by <em style="">lacZ</em>, ONPG assay was performed.</span><br /><br /><span style=""></span>  <span style=""><strong>ONPG assay:</strong></span><span style="">&nbsp;<a href="https://2015.igem.org/Team:CityU_HK/Protocol#characterization" style="color: #000000"><b><u>(Link to the protocol)</u></b></a></span><br /><span style=""></span><br /><span style=""></span>  <span style="">Besides lactose, ONPG (ortho-Nitrophenyl-&beta;-galactoside) is also a substrate of &beta;-galactosidase. ONPG is digested into galactose and ortho-nitrophenol (ONP) which is yellow in colour. Chloroform was used to lyse the cells and the enzymes were released into the surrounding. By measuring the O.D. at 420 nm after lysing the cells, the level of the &beta;-galatosidase was determined.</span></font><br /><span style=""></span><br /><span style=""></span></div>
  
<h2 class="wsite-content-title" style="text-align:left;"><span "font-size:12.0pt;mso-bidi-font-size:11.0pt;font-family:&quot;calibri&quot;,&quot;sans-serif&quot;;="" mso-ascii-theme-font:minor-latin;mso-fareast-font-family:&#26032;&#32048;&#26126;&#39636;;mso-fareast-theme-font:="" minor-fareast;mso-hansi-theme-font:minor-latin;mso-bidi-font-family:&quot;times="" roman&quot;;="" mso-bidi-theme-font:minor-bidi;mso-ansi-language:en-us;mso-fareast-language:="" zh-tw;mso-bidi-language:ar-sa"=""><font size="5">pL8-UV5 characterization</font></span></h2>
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<h2 class="wsite-content-title" style="text-align:left;"><span "font-size:12.0pt;mso-bidi-font-size:11.0pt;font-family:&quot;calibri&quot;,&quot;sans-serif&quot;;="" mso-ascii-theme-font:minor-latin;mso-fareast-font-family:&#26032;&#32048;&#26126;&#39636;;mso-fareast-theme-font:="" minor-fareast;mso-hansi-theme-font:minor-latin;mso-bidi-font-family:&quot;times="" roman&quot;;="" mso-bidi-theme-font:minor-bidi;mso-ansi-language:en-us;mso-fareast-language:="" zh-tw;mso-bidi-language:ar-sa"=""><font size="5">PL8-UV5 characterization</font></span></h2>
  
<div class="paragraph" style="text-align:left;"><span style=""><font size="3">pL8-UV5 is a regulated promoter which can be induced by either lactose or the analog IPTG. To characterize the inducible property of the pL8-UV5 promoter, pL8-UV5 was engineered upstream of the GFP gene. The GFP will be transcribed and translated after the promoter is induced. GFP fluorescent signal will be given by GFP. By measuring the GFP fluorescent signal after adding different concentration of IPTG to the bacteria, the inducible property of pL8-UV5 promoter can be determined.</font></span><br /><span style=""></span><br /><span style=""></span></div>
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<div class="paragraph" style="text-align:left;"><span style=""><font size="3">L8-UV5 is a regulated promoter which can be induced by either lactose or the analog IPTG. To characterize the inducible property of the L8-UV5 promoter, PL8-UV5 was engineered upstream of the GFP gene. The GFP will be transcribed and translated after the promoter is induced. GFP fluorescent signal will be given by GFP. By measuring the GFP fluorescent signal after adding different concentration of IPTG to the bacteria, the inducible property of L8-UV5 promoter can be determined.</font></span><br /><span style=""></span><br /><span style=""></span></div>
  
 
<h2 class="wsite-content-title" style="text-align:left;"><font size="5">Lysis cassette characterization</font><br /><span style=""></span></h2>
 
<h2 class="wsite-content-title" style="text-align:left;"><font size="5">Lysis cassette characterization</font><br /><span style=""></span></h2>

Revision as of 15:03, 18 September 2015

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