Difference between revisions of "Part:BBa K4255000:Experience"

(Applications of BBa_K4255000)
 
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===Applications of BBa_K4255000===
 
===Applications of BBa_K4255000===
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This year our project is focused on the synthesis of anthocyanin, which has a lot of research and reporting on this canonical pathway. But due to anthocyanins are ubiquitous in plants, therefore, each enzyme can find multiple homologous proteins. To get the better yeild, we first compared enzymes in different species and selected the most suitable sequence for E.coli expression, we constructed several new parts, which has been submitted this year.
 
This year our project is focused on the synthesis of anthocyanin, which has a lot of research and reporting on this canonical pathway. But due to anthocyanins are ubiquitous in plants, therefore, each enzyme can find multiple homologous proteins. To get the better yeild, we first compared enzymes in different species and selected the most suitable sequence for E.coli expression, we constructed several new parts, which has been submitted this year.
 
[[Image:SHSBNU.1.gif|center|700px|thumb|'''Fig. 1: Metabolism pathway for anthocyanin synthesis''']]
 
[[Image:SHSBNU.1.gif|center|700px|thumb|'''Fig. 1: Metabolism pathway for anthocyanin synthesis''']]
 
The first new part we uploaded this year is to express F3 '5'H, which is enzyme working to catalyze dihydrokaempferol into dihydromyricetin. The sequence we submitted here was come from (物种). And we has done codon optimization for E.coli expression.
 
The first new part we uploaded this year is to express F3 '5'H, which is enzyme working to catalyze dihydrokaempferol into dihydromyricetin. The sequence we submitted here was come from (物种). And we has done codon optimization for E.coli expression.
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Protocol we use:
 
Protocol we use:
 
We asked biological company to synthesize the sequence at first. And we constructed it into pETDUET plasmid. Next, we transformed the plasmids into E. coli BL21(DE3).
 
We asked biological company to synthesize the sequence at first. And we constructed it into pETDUET plasmid. Next, we transformed the plasmids into E. coli BL21(DE3).

Latest revision as of 09:57, 8 October 2022


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Applications of BBa_K4255000

This year our project is focused on the synthesis of anthocyanin, which has a lot of research and reporting on this canonical pathway. But due to anthocyanins are ubiquitous in plants, therefore, each enzyme can find multiple homologous proteins. To get the better yeild, we first compared enzymes in different species and selected the most suitable sequence for E.coli expression, we constructed several new parts, which has been submitted this year.

Fig. 1: Metabolism pathway for anthocyanin synthesis

The first new part we uploaded this year is to express F3 '5'H, which is enzyme working to catalyze dihydrokaempferol into dihydromyricetin. The sequence we submitted here was come from (物种). And we has done codon optimization for E.coli expression.

Protocol we use: We asked biological company to synthesize the sequence at first. And we constructed it into pETDUET plasmid. Next, we transformed the plasmids into E. coli BL21(DE3). After the colony has grown up on the plate, we picked a single colony by a sterile tip and added it into 4 ml LB medium with the corresponding antibiotic. Later, we added 1 mM IPTG for induction and shook at 16℃ overnight. We also set a control group and didn’t add IPTG into it. Finally, we centrifuged the bacterial solution at 12000 g, discard the supernatant, and used RIPA as a lysis buffer. we added loading buffer to the supernatant which contains the protein extract, and after heating at 96℃ for 10 min, we underwent SDS-PAGE and Coomassie brilliant blue staining for expression test. We could see a clear band at the position of (请老师补充分子量大小)kD, which only appeared in the group with IPTG. The molecular weight of this band was in line with the expectation, and it was under the condition of induction, so we believed that we had successfully expressed F3 '5'H gene. (需要补充载体设计图与表达结果图)

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