Objective: To assess two kinds of extraction (aqueous and methanolic) for Calendula officials using flowers, leaves
and stems and studying their antibacterial activity against five different bacteria.
Methodology: Calendula officials were selected to carry out this study. Flowers, leaves and stems were collected from
local markets in Baghdad then dried in shade for 7 days and grinded to fine powder. Aqueous hot extracts for 2hr. at
(100c˚) and alcoholic extracts for 48 hrs at (80c˚) were performed using flowers, leaves and stems then studied
antibacterial effect against five different bacterial genuses by using well diffusion technique.
Results: This study showed that hot aqueous extracts for 2hr. to all parts of Calendula officials indicated no
antibacterial activity. While, methanolic extracts of flowers, leaves and stems for 48hrs had antibacterial activity and
the highest values for inhibition zone shown in staphylococcus aureus and Escherichia coli.
Recommendations: The present study has been suggested to use Calendula officials flowers extract as alternative
medical therapy for microorganisms which may resist conventional treatment. This study is a first step for another
future studies. It is necessary to use various extraction methods to give active materials with high percentage,
although different organic solvents to be used with Calendula officials plant to obtain extracts used for testing
different kinds of microorganisms which have highly resistance to conventional treatment.
Over the past decades, several studies have examined the subcellular localization of the cauliflower mosaic virus (CaMV) P6 protein by tagging it with GFP (P6-GFP). These investigations have been essential in the development of models for inclusion body formation, nuclear transport, and microfilament-associated intracellular movement of P6 inclusion bodies for delivery of virions to plasmodesmata. Although it was shown early on that the translational transactivation function of P6-GFP was comparable to wild type P6, it has not been possible to incorporate a P6-GFP gene into an infectious clone of CaMV. Consequently, it has not been possible to formally prove that a P6-GFP fusion is comparable in function to the unmodified P6 protein. Here w
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