Difference between revisions of "Part:BBa K515107:Experience"

Latest revision as of 06:15, 16 October 2018

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SCAU-China

The main goal of this characterization is to find out which pH value is the most effective among the 6 pH values in order to obtain a suitable culture condition for the expression of Dendar2.We further found that the part which expressed the protein Dendar2 worked well in E.coli strain DH10B, like in the DH5 alpha.

Result and Findings

1.pH 4.5 is found to be the best pH that is suitable for the expression of Dendar2 .

2.Thered fluorescence from Dendar2 after photoconversion showed stronger fluorescent intensity than before.

3.Compared with the the expression pattern of Dendar2 as showed previously in DH5α, we concluded that the expression of Dendar2 works in both E.coli strains.

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-The main goal of this characterisation was to find out which pH value condition was the most effective among 6 level pH value to obtain a suitable culture condition for the expression of Dendar2.We also found that the part which expressed the Dendar2 can work well in E.coli strain DH10B, and just like in the DH5 alpha mentioned in main page.
+The main goal of this characterization is to find out which pH value is the most effective among the 6 pH values in order to obtain a suitable culture condition for the expression of Dendar2.We further found that the part which expressed the protein Dendar2 worked well in E.coli strain DH10B, like in the DH5 alpha.
-Experiment
-We wanted to test 6 pH value gradients that easily used in lab : 4.5/5.8/6.2/7.2/8,2/9,1, to see, in a 360 min culturing time, which one would be the best pH value culture condition for the DH10B to growth and express the Dendar2.
-We used the bacterial stock of our own, coming from commercial bacteria cultured and made competent using our protocol a few weeks before the experiment and conserved at -80°C.
-We made an electric shock transformation of 30ng BBa_K515107 part into 50μL bacteria and culture in LB plate, then picked the colony to 250μL LB broth medium for one hour. We prepared different pH level LB medium in 6 gradients(4.5/5.8/6.2/7.2/8,2/9,1), and add 25μL cultured medium from the 250μL LB broth medium to 1 mL different pH level LB medium, still culture to 360 min.
-Very 20 min time point, we collect 10μL bacterial culture medium and measure the green fluorescence as well as the red fluorescence after photoconversion using photon stimulation at UV wavelength.
-ImageJ was used to analysize the intensity of Dendar2 fluorescence.
-[[File:Scau-china-2018-7.png|800px|thumb|center| Figure 1 The fluorescence signal of Dendar2 in t=100min and t=300min time point, pH=4.5 and pH=9.1.The part work well in DH10B and the we found that the alkaline condition have a negative influence on the expression of Dendar2 in DH10B. ]]
-[[File:Scau-china-2018-8.png|800px|thumb|center|Figure 2 The measurement of Dendar2, green fluorescence signal before photoconversion changed in different pH value gradients during 360 min.]]
-[[File:Scau-china-2018-9.png|800px|thumb|center| Figure 3 The measurement of Dendar2, red fluorescence signal after photoconversion changed in different pH value gradients during 360 min.]]
 Result and Findings
-.The acid condition is suitable for the expression of Dendar2 When pH =4.5, the part can have a better working condition .
-.There red fluorescence we observed after photoconversion have stronger intensity than the green fluorescence before photoconversion.
+.pH 4.5 is found to be the best pH that is suitable for the expression of Dendar2 .
-.Compared with the characterisation show before in the DH5α stain, we made conclusion the expression of Dendar2 can be well in those two E. coli strain.|
+.Thered fluorescence from Dendar2 after photoconversion showed stronger fluorescent intensity than before.
+.Compared with the  the expression pattern of Dendar2 as showed previously in DH5α, we concluded that the expression of Dendar2 works in both E.coli strains.
+|
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