Production and Expression Optimization of Heterologous Serratiopeptidase

Q: How can I download an article?

To download an article from SID, first log in to the site, search for the article title, and click on the 'Download Article' option.

Q: How can I download an ISI article?

To download an ISI article on SID, enter the keyword or article title in the search bar, view the relevant results, click on the desired article, and select the 'Download Article' option.

Q: How can I access the SID database?

To access the SID database, visit SID.ir, create an account, and log in to access scientific resources.

Q: Is downloading articles from SID free?

Some articles on SID are available for free, while others require payment. Details are specified on the article's page.

ROUHANI MARYAM; VALIZADEH VAHIDEH; MOLASALEHI SARA; NOROUZIAN DARIUSH

مرکز اطلاعات علمی Scientific Information Database (SID) - Trusted Source for Research and Academic Resources

Journal Paper

Paper Information

Journal: Iranian Journal of Public Health Year:2020 | Volume:49 | Issue:5 Page(s): 931-939

Download Full-Text

View:

224

Download:

Cites:

Information Journal Paper

Title

Production and Expression Optimization of Heterologous Serratiopeptidase

Author(s)

ROUHANI MARYAM | VALIZADEH VAHIDEH | MOLASALEHI SARA | NOROUZIAN DARIUSH | Issue Writer Certificate

Keywords

Serratiopeptidase

Cloning

Expression optimization

Abstract

Background: Serratiopeptidase is a bacterial metalloprotease, which is useful for the treatment of pain and inflammation. It breaks down fibrin, thins the fluids formed during inflammation and acts as an anti-biofilm agent. Because of medicinally important role of the enzyme, we aimed to study the Cloning and the Expression optimization of Serratiopeptidase. Methods: The heat-stable Serratiopeptidase (5d7w) was selected as the template. Cloning into pET28a expression vector was performed and confirmed by colony PCR and double restriction enzyme digestion. The recombinant protein was expressed in Esherichia coli BL21 and confirmed by SDS-PAGE and Western blot analysis. Different parameters such as expression vector, culture media, post-induction incubation temperature, inducer concentration, and post-induction incubation time were altered to obtain the highest amount of the recombinant protein. Results: Serratiopeptidase was successfully cloned and expressed under optimized conditions in E. coli which confirmed by western blot analysis. The optimal conditions of expression were determined using pQE30 as vector, cultivating the host bacteria in Terrific Broth (TB) medium, at 37º C, induction by IPTG concentration equal to 0. 5 mM, and cells were harvested 4 h after induction. Conclusion: As Serratiopeptidase is a multi-potent enzyme, the expressed recombinant protein can be considered as a valuable agent for pharmaceutical applications in further studies.

Cites

No record.

References

No record.

Cite

APA: Copy

ROUHANI, MARYAM, VALIZADEH, VAHIDEH, MOLASALEHI, SARA, & NOROUZIAN, DARIUSH. (2020). Production and Expression Optimization of Heterologous Serratiopeptidase. IRANIAN JOURNAL OF PUBLIC HEALTH, 49(5), 931-939. SID. https://sid.ir/paper/740128/en

Vancouver: Copy

ROUHANI MARYAM, VALIZADEH VAHIDEH, MOLASALEHI SARA, NOROUZIAN DARIUSH. Production and Expression Optimization of Heterologous Serratiopeptidase. IRANIAN JOURNAL OF PUBLIC HEALTH[Internet]. 2020;49(5):931-939. Available from: https://sid.ir/paper/740128/en

IEEE: Copy

MARYAM ROUHANI, VAHIDEH VALIZADEH, SARA MOLASALEHI, and DARIUSH NOROUZIAN, “Production and Expression Optimization of Heterologous Serratiopeptidase,” IRANIAN JOURNAL OF PUBLIC HEALTH, vol. 49, no. 5, pp. 931–939, 2020, [Online]. Available: https://sid.ir/paper/740128/en

Related Journal Papers

No record.

Related Seminar Papers

No record.

Related Plans

No record.

Recommended Workshops