Open AccessIdentification and cloning of putative water clarification genes of Moringa peregrina (Forssk.) Fiori in E. coli Xl1blue cells
Author(s) -
Reihaneh Ghodsi,
Hamid Mirmohammad Sadeghi,
Gholamreza Asghari,
Sara Torabi
Publication year - 2014
Publication title -
advanced biomedical research
Language(s) - English
Resource type - Journals
ISSN - 2277-9175
DOI - 10.4103/2277-9175.125807
Subject(s) - moringa , cloning (programming) , complementary dna , gene , polymerase chain reaction , microbiology and biotechnology , biology , genetics , food science , computer science , programming language
Background: Water purification processes include the use of chemical compounds despite the concern that they may induce diseases. An ecological solution to this dilemma can come from the use of plant seeds for this purpose. Moringa peregrina (Forssk.) Fiori seeds have water clarification ability. Therefore, the aim of this work was to look for certain water clarification genes in M. peregrina.Materials and Methods: After preparation of M. peregrina callus, mRNA was extracted from these cells. After application of reverse transcriptase, the obtained cDNA (s) were used for PCR amplification of the desired genes using primers based on MO 2.1 gene of Moringa oleifera. DNA amplification products were cloned in E. coli Xl 1 blue cells and DNA sequences were compared with Mo 1,2 gene in M. oleifera.Results: We obtained 3 PCR products (approximately 200, 300, and 400 bps). Conclusion: After comparison of the sequences of 300bp band obtained from M. peregrina with Mo 1,2 gene in M. oleifera, it seems that 300bp band is a good candidate to investigate regarding its potential flocculent activity