Difference between revisions of "Part:BBa K1074006:Experience"
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[[Image:USTC_China_iGEM13_BBa_K1074006_4.png|thumb|right|300px|figure 2 SDS-PAGE of N-terminal TD1 modified LTB and HBsAg]] | [[Image:USTC_China_iGEM13_BBa_K1074006_4.png|thumb|right|300px|figure 2 SDS-PAGE of N-terminal TD1 modified LTB and HBsAg]] | ||
[[Image:USTC_China_iGEM13_BBa_K1074006_2.JPG|thumb|left|600px|figure 3 Fluorescence detection of N-terminal TD1 modified GFP expression with and without IPTG induction]] | [[Image:USTC_China_iGEM13_BBa_K1074006_2.JPG|thumb|left|600px|figure 3 Fluorescence detection of N-terminal TD1 modified GFP expression with and without IPTG induction]] | ||
− | [[Image:USTC_China_iGEM13_BBa_K1074006_5.jpg|thumb|left| | + | [[Image:USTC_China_iGEM13_BBa_K1074006_5.jpg|thumb|left|400px|figure 4 ELISA test transdermal function of N-terminal TD1 modified antigen HBsAg ]] |
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Revision as of 13:13, 27 September 2013
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how you used this part and how it worked out.
Applications of BBa_K1074006
User Reviews
UNIQe97e005497bb5e12-partinfo-00000000-QINU UNIQe97e005497bb5e12-partinfo-00000001-QINU
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USTC_China iGEM13 |
In our project, we construct other four gene circuits based on this part. In these gene circuits, GFP is replaced by HBsAg, Ag85b, PAD4, LTB respectively. We transformed the recombinant Plasmids both in BL21 and Bacillus Subtilis WB800N and induced expression with IPTG . Results analyzed by SDS-page , mass spectrum and ELISA were proved positive. But proteins expressed in WB800N were far less than those in BL21. The antigenicity and transdermal function of N-terminal TD1 modified antigen HBsAg was also tested positive by ELISA. |