Difference between revisions of "Part:BBa K5375006"
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+ | The part sequence we have registered is its corresponding DNA sequence, which needs to be transcribed into RNA sequence for use. The following sequences are siRNA sequences. | ||
siHSP70-1 is cultivated through oligonucleotides with a nucleic acid synthesizer. Two complementary oligonucleotides are chemically synthesized, representing the sense and antisense strands of the siRNA: | siHSP70-1 is cultivated through oligonucleotides with a nucleic acid synthesizer. Two complementary oligonucleotides are chemically synthesized, representing the sense and antisense strands of the siRNA: | ||
- Oligo Sequence for siHSP70-1-SS: CCUUCAAGGUCAUCGAGAAGG | - Oligo Sequence for siHSP70-1-SS: CCUUCAAGGUCAUCGAGAAGG | ||
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- Oligo Sequence for siHSP70-1-AS: UUCUCGAUGACCUUGAAGGGG | - Oligo Sequence for siHSP70-1-AS: UUCUCGAUGACCUUGAAGGGG | ||
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= Measurement and Characterization = | = Measurement and Characterization = | ||
+ | In this project, we utilized RT-qPCR technology to assess the expression levels of the target gene. We employed a relative quantification method that standardizes the expression of the target gene across different samples using a reference gene. Specifically, we compared the Ct values of the target gene in experimental samples with those in control samples, with the results expressed as the ratio or fold change in the target gene expression between the experimental and control samples. | ||
+ | In our experiments, we selected β-actin as the reference gene for normalization. By normalizing the expression levels, we derived the fold change of the target gene expression in the experimental samples relative to the control samples. The normalized expression level of the target gene in the control samples was set to "1", while the normalized expression levels in the experimental samples were reported as the fold increase or decrease compared to the control. This calculation was performed using the 2^-(∆∆Ct) method, which effectively reflects the relative expression levels of the target gene across different samples. | ||
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= Reference = | = Reference = | ||
Latest revision as of 07:44, 30 September 2024
siHSP70-1
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000COMPATIBLE WITH RFC[1000]
Contents
Origin
Synthesized by company.
Properties
Inhibition of Heat Shock Protein 70 expression.
Usage and Biology
siHSP70-1 inhibits the target gene HSP70 as a small interfering RNA (siRNA). HSP70 can induce IgE-mediated hypersensitivity reactions and T-cell responses in allergic individuals (Fagotti et al., 2022). Further discussion of it as a pan-allergen can be found in part BBa_K2619011. siRNA is a key component of the RNAi process, a powerful gene silencing mechanism. Once introduced into the target cells, it is recognized and loaded into the RNA-Induced Silencing Complex (RISC). The siRNA’s antisense strand binds to the complementary target mRNA molecule, triggering the RISC complex into cleaving the target mRNA. This prevents the target mRNA from being translated into a functional protein (Agrawal et al., 2003). The silencing effect typically lasts around 12 days for this part.
Its potential lies in applications to plant cells, where it successfully inhibits the expression of the pan-allergen HSP70, alleviating and reducing allergic symptoms for *Populus tomentosa* pollen allergy.
Cultivation and Purification
The part sequence we have registered is its corresponding DNA sequence, which needs to be transcribed into RNA sequence for use. The following sequences are siRNA sequences.
siHSP70-1 is cultivated through oligonucleotides with a nucleic acid synthesizer. Two complementary oligonucleotides are chemically synthesized, representing the sense and antisense strands of the siRNA:
- Oligo Sequence for siHSP70-1-SS: CCUUCAAGGUCAUCGAGAAGG
- Oligo Sequence for siHSP70-1-AS: UUCUCGAUGACCUUGAAGGGG
The oligonucleotides are then mixed under appropriate buffer conditions to anneal and form a double-stranded siRNA molecule. The resulting siRNA is purified using high-performance liquid chromatography (HPLC) (Sohail et al., 2003). To enhance siRNA delivery into plant cells, carbon dots (CDs) were incorporated with Polyethyleneimine (PEI) through the microwave method, allowing the negatively charged siRNA to bind to the CDs via electrostatic adsorption.
Measurement and Characterization
In this project, we utilized RT-qPCR technology to assess the expression levels of the target gene. We employed a relative quantification method that standardizes the expression of the target gene across different samples using a reference gene. Specifically, we compared the Ct values of the target gene in experimental samples with those in control samples, with the results expressed as the ratio or fold change in the target gene expression between the experimental and control samples.
In our experiments, we selected β-actin as the reference gene for normalization. By normalizing the expression levels, we derived the fold change of the target gene expression in the experimental samples relative to the control samples. The normalized expression level of the target gene in the control samples was set to "1", while the normalized expression levels in the experimental samples were reported as the fold increase or decrease compared to the control. This calculation was performed using the 2^-(∆∆Ct) method, which effectively reflects the relative expression levels of the target gene across different samples.
The chart shows the performance of siHSP70-1 in inhibiting HSP70 expression. Results indicate that siHSP70-1 was unable to repress HSP70 and caused minor fluctuations. Thus, siHSP70-1 was deemed unsuccessful, while siHSP70-2 and -3 demonstrated better performance.
RT-qPCR results for siRNA injection in tobacco leaves. siHSP70-1 and CDs@siHSP70-1 columns indicate the performance of siHSP70-1. Data shows that combining siHSP70-1 with CDs was unsuccessful in repressing HSP70 expression.
RT-qPCR results for siRNA delivery through trunk injection in osmanthus trees. Some success in inhibiting HSP70 expression was observed with the combination of CDs, but further trials are required to validate the efficacy.
Further trials and improvements will be needed for siHSP70-1 to ensure optimal quality and efficacy in target gene repression.
Reference
Agrawal N. N., Dasaradhi P. V., Mohmmed A., Malhotra P., Bhatnagar R. K., & Mukherjee S. K. (2003). RNA Interference: Biology, Mechanism, and Applications. *Microbiology and Molecular Biology Reviews*, 67(4), 657-685. [1](https://doi.org/10.1128/MMBR.67.4.657-685.2003)
Fagotti A., Lucentini L., Simoncelli F., La Porta G., Brustenga L., Bizzarri I., Trio S., Isidori C., Di Rosa I., & Di Cara G. (2022). HSP70 upregulation in nasal mucosa of symptomatic children with allergic rhinitis and potential risk of asthma development. *Scientific Reports*, 12(1), 1-10. [2](https://doi.org/10.1038/s41598-022-18443-x)
Sohail M., Doran G., Riedemann J., Macaulay V., & Southern E. M. (2003). A simple and cost-effective method for producing small interfering RNAs with high efficacy. *Nucleic Acids Research*, 31(7), e38.