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Adv Pharm Bull. 2019;9(4): 655-661.
doi: 10.15171/apb.2019.076
PMID: 31857971
PMCID: PMC6912177
Scopus ID: 85075825369
  Abstract View: 1556
  PDF Download: 840

Research Article

Cloning and Overexpression of Strictosidine β-D-Glucosidase Gene Short Sequence from Catharanthus roseus in Escherichia coli

Ahmed Saeed Arafa 1 ORCID logo, Amany Elsayed Ragab 1* ORCID logo, Abdel-Rahim Sayed Ibrahim 1 ORCID logo, Wael Saad Abdel-Mageed 2,3 ORCID logo, Mahmoud Emam Nasr 2 ORCID logo

1 Pharmacognosy Department, Faculty of Pharmacy, Tanta University, Tanta, Egypt, 31527.
2 Molecular Biology Department, Genetic Engineering and Biotechnology Research Institute, Sadat City University, Sadat City, Egypt, 32897.
3 Genetics Department, Faculty of Agriculture, Beni-Suef University, Beni-Suef, Egypt, 62511.
*Corresponding Author: Email: amany.ragab@pharm.tanta.edu.eg

Abstract

Purpose: Strictosidine-β-D-glucosidase (SGD) is considered as a key enzyme in the production of bisindole alkaloids in Catharanthus roseus. The present study illustrated the production of a short sequence of this enzyme in Escherichia coli without codon optimization.

Methods: Strictosidine-β-D-glucosidase (sgd) gene short sequence (1434 bp), which lacks the conserved sequence KGFFVWS and the localization peptide sequence at the C-terminal, was amplified from cDNA of C. roseus leaves, cloned and expressed in Escherichia coli. The activity of the produced protein in cell free lysate was tested using total alkaloid extract of C. roseus leaves.

Results: HPLC and LC-MS analysis of the assay mixture revealed the disappearance of the strictosidine peak.

Conclusion: SGD short sequence can be produced in Escherichia coli in active form without codon optimization.


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Submitted: 05 Nov 2018
Revision: 07 Jun 2019
Accepted: 15 Jun 2019
ePublished: 24 Oct 2019
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