Difference between revisions of "Part:BBa K1694025"
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After assembling the DNA sequences from the basic parts, we recombined each Pcons+RBS+Lpp-OmpA-N+ScFv gene to pSB1C3 backbones and conducted a PCR experiment to check the size of each parts. The DNA sequence length of these parts is around 1100~1300 bp. In this PCR experiment, the PCR products' size should be near at 1300~1500 bp. The '''Fig.2''' showed the correct size of this part, and proved that we successfully ligated the sequence onto an ideal backbone. | After assembling the DNA sequences from the basic parts, we recombined each Pcons+RBS+Lpp-OmpA-N+ScFv gene to pSB1C3 backbones and conducted a PCR experiment to check the size of each parts. The DNA sequence length of these parts is around 1100~1300 bp. In this PCR experiment, the PCR products' size should be near at 1300~1500 bp. The '''Fig.2''' showed the correct size of this part, and proved that we successfully ligated the sequence onto an ideal backbone. | ||
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− | [[File:PROH.png|600px|thumb| | + | [[File:PROH.png|600px|thumb|center|'''Fig.3''' Pcons+RBS+Lpp-OmpA-N+ScFv(anti-HER2)]] |
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'''2.Cell staining experiment'''<br> | '''2.Cell staining experiment'''<br> | ||
After cloning the part of anti-HER2, we were able to co-transform anti-HER2 with different fluorescent protein into our ''E. coli''. <br> | After cloning the part of anti-HER2, we were able to co-transform anti-HER2 with different fluorescent protein into our ''E. coli''. <br> |
Latest revision as of 10:46, 22 September 2015
Pcons+B0034+Lpp-OmpA-N+scFv(Anti-HER2)
Introduction:
By ligating the constitutive promoter (BBa_J23101), strong ribosome binding site (BBa_B0034) and Lpp-OmpA
(BBa_K1694002)
connected to Anti-HER2
(BBa_K1694005) , we were able to display the Anti-EGFR on the E. coli outer membrane continuously.
This year we want to supply a customized platform. We provide two plasmids libraries of Pcon+RBS+OmpA-scFv and Pcons+RBS+Fluorescence+Ter for customers. Therefore,customers can choose any scFv and fluorescent proteins combination they want. We will co-transform the two plasmids, which helps us tailor our product to the wishes of our customers.
Introduction of basic parts:
Lpp-OmpA-N
Anti-HER2
Experiment
1.Cloning
After assembling the DNA sequences from the basic parts, we recombined each Pcons+RBS+Lpp-OmpA-N+ScFv gene to pSB1C3 backbones and conducted a PCR experiment to check the size of each parts. The DNA sequence length of these parts is around 1100~1300 bp. In this PCR experiment, the PCR products' size should be near at 1300~1500 bp. The Fig.2 showed the correct size of this part, and proved that we successfully ligated the sequence onto an ideal backbone.
2.Cell staining experiment
After cloning the part of anti-HER2, we were able to co-transform anti-HER2 with different fluorescent protein into our E. coli.
The next step was to prove that our co-transformed product have successfully displayed ScFv of anti-HER2 and expressed fluorescent protein.
To prove this, we conducted the cell staining experiment by using the co-transformed E. coli to detect the HER2 in the cancer cell line.
Modeling:
In the modeling part, we discover optimum protein expression time by using the genetic algorithm (GA) in Matlab.
We want to characterize the actual kinetics of this Hill-function based model that accurately reflects protein expression time.
By using the differential function which was derived from these optimum parameters which were calculated by GA can help us to simulate the optimum protein expression.
When we have the simulated protein expression rate, the graph of protein expression versus time can be drawn.Thus, we can find the optimum protein expression time. However, the simulated protein expression curve is slower than the experimental curve by one hour. Therefore, to find the most exact optimum protein expression time, we infer that subtracting one hour of the optimum protein expression time would be correct.
Co-transform
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12INCOMPATIBLE WITH RFC[12]Illegal NheI site found at 7
Illegal NheI site found at 30 - 21INCOMPATIBLE WITH RFC[21]Illegal BglII site found at 741
- 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal NgoMIV site found at 451
- 1000COMPATIBLE WITH RFC[1000]