Part:BBa_K4516019
hFoxO1-F.luciferase-R.luciferase:a platform to screen a small molecule FoxO1 antagonist
Profile
Name: hFoxO1-F.luciferase-R.luciferase
Base Pairs: 6187 bp
Origin: HepG2 cell genome
Properties: expression plasmid that can duplicate both in E.coli and HepG2 cells
Contribution
FoxO1, as a transcription factor, plays an important role in the regulation of blood glucose balance. FoxO1 in the liver can promote the expression of key gluconeogenesis enzyme genes, and an important mechanism of insulin regulation of blood sugar is to increase the phosphorylation of FoxO1, promote its nuclear export, and then reduce its transcriptional activation activity. According to this theory, we constructed a human FoxO1 full-length plasmid, used Firefly luciferase and Renilla luciferase as a reporter gene, established a FoxO1 transcriptional activation screening platform, and used this platform to screen out active compounds that inhibit FoxO1 transcriptional activation activity.
In order to construct a FoxO1 expression plasmid that can shuttle both in E.coli and HepG2 cells, we designed the DNA sequences of hFoxO1 to be inserted into the XhoI and KpnI sites of the pcDNA3.1 vector (Fig.1), and transfected the HepG2 cells with the recombinant plasmid to set up our experiment platform.
Engineering Success
How we design our plasmid
In order to construct a FoxO1 expression plasmid that can duplicate both in E.coli and HepG2 cells, we designed the DNA sequences of hFoxO1 to be inserted into the XhoI and KpnI sites of the pcDNA3.1 vector (Fig.1), and transfect the HepG2 cells with the recombinant plasmid and set up our experiment platform.
How we build our plasmid
To build the plasmid, we use PCR to amplify the hFoxO1 gene from template DNA (HepG2 cell genome), and extract the target fragment (Fig.2). At the same time, we did the plasmid extraction to obtain the plasmid pcDNA3.1. The second step was double-enzyme digestion with XhoI and KpnI. The goal of digestion was to get the linearized pcDNA3.1 vector and inserted DNA fragments of hFoxO1. The third step was to ligate the inserts and linearized vector and transfer the ligation product into DH5α competent.
(A)Lane 1 is the hFoxO1 target band. We send the constructed recombinant plasmid to a sequencing company for sanger sequencing. The returned sequencing comparison results showed that the plasmid was successfully constructed (Fig.3). Then we extract the recombinant plasmid from E.coli DH5α and transfect it into HepG2 cells to express hFoxO1 proteins.
How we test our hFoxO1
a) Protein expression and verification In order to verify if hFoxO1 protein was successfully expressed in HepG2 cells which were transfected with the correct recombinant plasmid after 12 hours, we did Western blot (Fig.4). The result shows that the protein expression level of hFoxO1 increased accompanied by the increase of plasmid concentration, indicating that hFoxO1 was expressed successfully in the cell.
improvement of an existing part
Our composite component, BBa_K4516019, is a platform to screen small molecule FoxO1 antagonists that can be used to treat type 2 diabetes. As early as 2020, the iGEM20_XDFYZ team was committed to developing a drug screening platform (BBa_K3522013) for the treatment of type 2 diabetes. They found candidate drug molecules by screening FXR antagonists. Based on their work, by reading literature and consulting experts in related fields, we found that in addition to the FXR target, there are also a FoxO1 target that plays an important role in the regulation of blood glucose balance. Therefore, we further optimized the diabetes drug screening platform and constructed a new composite part BBa_K4516019 to screen more kinds of drug molecules that can be used to treat type 2 diabetes. In order to prove the function of our new composite part hFoxO1-F. luciferase-R. luciferase, we transferred the recombinant plasmid into HepG2 to establish a transcriptional activation screening platform, and screened a totally new compound 355, which has an inhibitory effect on the transcriptional activation activity of FoxO1. Then, by detecting the effect of 355 active compounds on hepatic gluconeogenesis and the mRNA levels of key enzymes in hepatic gluconeogenesis, it was further confirmed that 355 compounds have the effect of inhibiting hepatic gluconeogenesis, thereby achieving the effect of lowering blood sugar.
Results of Compounds Screening Using this Platform To regulate the expression of hFoxO1, we used small molecular compounds from the database to examine their effects on gluconeogenesis (Table1). Compound 335 was found to have a significant role in reducing glucose concentrations in HepG2 cells. Table 1. The effects of different small molecular compounds on gluconeogenesis.
In Fig.6, in the third column of the histogram, the luciferase activity level was low in the presence of the hFoxO1 transcriptional activator under the action of compound 355, so it could be concluded that compound 355 has an obvious inhibitory effect on hFoxO1 transcriptional activation.
c) Detection of the 355 compounds on hepatic gluconeogenesis After screening for compound 355 by luciferase activity detection (Fig.6), compound 355 was also used to inhibit both glucose concentration in HepG2 cells and mRNA abundance of key enzymes of gluconeogenesis. In Fig7A, we can find that with the gradual increase of the concentration of compound 355, the glucose level showed a counter gradient change and was concentration-dependent, indicating that compound 355 could significantly inhibit gluconeogenesis in hepatocytes.
G6Pase is an enzyme that releases glucose into the blood by hydrolyzing glucose-6-phosphate in liver tissue. PEPCK is a gluconeogenic enzyme that allows hepatic parenchymal cells to produce glucose from pyruvate derived from amino acid metabolism. In Fig.7 B and 7C, when the volume of compound 355 increases gradually, the mRNA levels of G6pase and PEPCK gradually decreased in a counter gradient and were also concentration-dependent, indicating that compound 355 could significantly reduce the mRNA levels of key enzymes in gluconeogenesis.
Future plan
We have already collected the data and figures from our experiments. hFoxO1 plays a role in regulating downstream genes, especially in gluconeogenesis. And we find out that within a certain range, we could see a gradient of luciferin activity and concentration dependence. After expressing hFoxO1 protein in HepG2 cells, we can easily detect the downstream gene expression through a fluorescence reporting system. By the way, when we compared these data with the positive control group, we find that the activity of the hFoxO1 is easily regulated by special small components. Because of the great effect of the hFoxO1, we believe that if we can regulate the expression of hFoxO1 in the future and promote it in the market, it will become a great power to fight against type 2 diabetes, and it may be applied to clinical disease treatment, improve the quality of life of patients, and even reduce the number of diabetes patients. Reference 1.IDF., Diabetes Atlas. 10th Edition, 2021. 2.Choi, H.E., et al., Novel FoxO1 inhibitor, JY-2, ameliorates palmitic acid-induced lipotoxicity and gluconeogenesis in a murine model. Eur J Pharmacol, 2021. 899: p. 174011. 3.Oh, K.J., et al., CREB and FoxO1: two transcription factors for the regulation of hepatic gluconeogenesis. BMB Rep, 2013. 46(12): p. 567-74. 4.Zhao, Y., Y. Wang, and W.G. Zhu, Applications of post-translational modifications of FoxO family proteins in biological functions. J Mol Cell Biol, 2011. 3(5): p. 276-82. 5.Nagashima, T., et al., Discovery of novel forkhead box O1 inhibitors for treating type 2 diabetes: improvement of fasting glycemia in diabetic db/db mice. Mol Pharmacol, 2010. 78(5): p. 961-70. 6.Ohtake, F., et al., Modulation of oestrogen receptor signalling by association with the activated dioxin receptor. Nature, 2003. 423(6939): p. 545-50.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12INCOMPATIBLE WITH RFC[12]Illegal NotI site found at 518
Illegal NotI site found at 527 - 21INCOMPATIBLE WITH RFC[21]Illegal BglII site found at 783
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- 1000INCOMPATIBLE WITH RFC[1000]Illegal BsaI.rc site found at 4363
Illegal SapI.rc site found at 3273
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