Team:UESTC-China/result

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<p style="color:#1b1b1b;">Tobacco was transformed essentially using the leaf disk co-cultivation protocol of Horsch. This protocol includes three stages, co-cultivation (Fig.4A), screening cultivation (Fig.4B) and rooting cultivation (Fig.4C). We have successfully transformed each vector into babacco. Table 1 is the statistical result of quantity of each transgenic line. And we have got PCR positive plantlet of every transgenic line.</p>
<p style="color:#1b1b1b;">Tobacco was transformed essentially using the leaf disk co-cultivation protocol of Horsch. This protocol includes three stages, co-cultivation (Fig.4A), screening cultivation (Fig.4B) and rooting cultivation (Fig.4C). We have successfully transformed each vector into babacco. Table 1 is the statistical result of quantity of each transgenic line. And we have got PCR positive plantlet of every transgenic line.</p>
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<strong>Fig.4</strong>
<strong>Fig.4</strong>
Transform piGEM003, piGEM004, piGEM005, piGEM006, piGEM007, piGEM008, piGEM009, piGEM010 and piGEM011 into tobacco. Co-cultured for 48 hours(A); Screening cultivation for one month(B); Rooting cultivation for one month(C).
Transform piGEM003, piGEM004, piGEM005, piGEM006, piGEM007, piGEM008, piGEM009, piGEM010 and piGEM011 into tobacco. Co-cultured for 48 hours(A); Screening cultivation for one month(B); Rooting cultivation for one month(C).
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<h1 class="SectionTitles" style="width:1140px; ">Expression of four key enzymes in tobacco</h1><br/>
<h1 class="SectionTitles" style="width:1140px; ">Expression of four key enzymes in tobacco</h1><br/>
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<p style="color:#1b1b1b;">We extracted DNA from tobacco plantlets. And then we used specific primers to amplify the target gene to verify the kan-resistant seedlings (Fig.5). Next we extracted RNA from tobacco leaves which are PCR positive. We used  RT-PCR to detect whether target gene was expressed <i style="color: red;">(Fig.6)</i>.</p>
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<p style="color:#1b1b1b;">We extracted DNA from tobacco plantlets. And then we used specific primers to amplify the target gene to verify the kan-resistant seedlings (Fig.5). Next we extracted RNA from tobacco leaves which are PCR positive. We used  RT-PCR to detect whether target gene was expressed (Fig.6).</p>
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<p style="position:relative; left:0px; padding:15 5px; font-size:20px; font-family: calibri, arial, helvetica, sans-serif; font-style: calibri; text-align:left; width:650px; color:#1b1b1b;"><strong>Fig.6</strong>
<p style="position:relative; left:0px; padding:15 5px; font-size:20px; font-family: calibri, arial, helvetica, sans-serif; font-style: calibri; text-align:left; width:650px; color:#1b1b1b;"><strong>Fig.6</strong>
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<strong>Fig.6</strong>RT-PCR verification of positive transgenic tobacco seedlings.<br/>
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M: DNA marker; 1-8: 6 individual lines; 9: plasmid
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Revision as of 01:22, 14 October 2014

UESTC-China