Team:USTC CHINA/Project/Results
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<img src="https://static.igem.org/mediawiki/igem.org/9/9a/2013ustc-china_xianlu%28GFP%29.png"> | <img src="https://static.igem.org/mediawiki/igem.org/9/9a/2013ustc-china_xianlu%28GFP%29.png"> | ||
<div><p>Using GFP to prove the validity of a newly designed circuit is a classical way to verify the expressing of this circuit. As expressions in E.coli involve neither secretory nor sequential problems, we hoped to verify the practicality of our locus by the expression of TD1-GFP. Thus we selected pET22b,which is a common recombinant vector for plasmid construction, as our recombinant vector and E.coli BL21 as engineered bacteria . We fused sequence TD1-GFP with T7 promoter from pET22b downstream and succeeded in expressing fusion protein TD1-GFP, induced by IPTG. </p></div> | <div><p>Using GFP to prove the validity of a newly designed circuit is a classical way to verify the expressing of this circuit. As expressions in E.coli involve neither secretory nor sequential problems, we hoped to verify the practicality of our locus by the expression of TD1-GFP. Thus we selected pET22b,which is a common recombinant vector for plasmid construction, as our recombinant vector and E.coli BL21 as engineered bacteria . We fused sequence TD1-GFP with T7 promoter from pET22b downstream and succeeded in expressing fusion protein TD1-GFP, induced by IPTG. </p></div> | ||
+ | <img src="https://static.igem.org/mediawiki/igem.org/2/2a/2013ustc-china_jiaotu-gfp.png"> | ||
<div><p>*****一天到晚@人!!!但这里还是有三张图片!!!我*****</p></div> | <div><p>*****一天到晚@人!!!但这里还是有三张图片!!!我*****</p></div> | ||
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Revision as of 01:16, 26 September 2013