This study was performed to evaluate the total phenols, flavonoids, and antioxidant activities of twenty-four propolis samples from different regions of Morocco. In addition, two samples were screened regarding the antibacterial effect against four Staphylococcus aureus strains. Gas chromatography coupled to mass spectra (GC-MS) analysis was done for propolis samples used in antibacterial tests. The minimum inhibitory and minimum bactericidal concentration (MIC, MBC) were determined. The potential to acquire the resistance after sequential exposure of bacterial strains and the impact of adaptation to propolis on virulence using the Galleria mellonella were evaluated. Additionally, the effects of propolis extract on the bacterial adherence ability and its ability to inhibit the quorum sensing activity were also examined. Among the twenty-four extracts studied, the samples from Sefrou, Outat el Haj, and the two samples marketed in Morocco were the best for scavenging DPPH, ABTS, NO, peroxyl, and superoxide radicals as well as in scavenging of hydrogen peroxide. A strong correlation was found between the amounts of phenols, flavonoids, and antioxidant activities. Propolis extract at the MIC value (0.36 mg/mL) significantly reduced (p < 0.001) the virulence potential of S. aureus ATCC 6538 and the MRSA strains without leading to the development of resistance in the sequence of continuous exposure. It was able to impair the bacterial biofilm formation. The results have revealed that sample 1 reduces violacein production in a concentration dependent manner, indicating inhibition of quorum sensing. This extract has as main group of secondary metabolites flavonoids (31.9%), diterpenes (21.5%), and phenolic acid esters (16.5%).
The aim of this study was to evaluate the adaptation response of Staphylococcus aureus, methicillin-resistant S. aureus (MRSA), and Listeria monocytogenes to the essential oil (EO), eugenol, and citral. The minimum inhibitory concentration of eugenol and citral was determined by agar dilution and microdilution. Adaptation to eugenol and citral was done by sequential exposure of the pathogens to increasing concentrations of the essential oils. The M2-A9 standard was used to determine the antibiotic susceptibility. The effect of eugenol and citral on the adherence ability was evaluated by the crystal violet assay. The impact of adaptation to eugenol on virulence was estimated using the Galleria mellonella model. No development of resistance to the components and antibiotics was observed in the adapted cells of S. aureus, MRSA, and L. monocytogenes. Eugenol and citral at subinhibitory concentration reduced the bacterial adherence. Adaptation to subinhibitory concentration of eugenol affected the virulence potential of S. aureus, MRSA, and L. monocytogenes. Eugenol and citral do not pose a risk of resistance development in a continuous mode of use. These EO components showed a high efficacy as antistaphylococcal and antilisterial biofilm agents. Adaptation at subinhibitory concentration of eugenol protected the larvae against listerial and staphylococcal infection.
The Algarve Region (AR) in southern Portugal, which is an
international tourist destination, has been considered an endemic region of
zoonotic leishmaniasis caused by Leishmania infantum since the
1980s. In the present study, phlebotomine and canine surveys were conducted to
identify sandfly blood meal sources and to update the occurrence of
Leishmania infection in vectors and dogs. Four sandfly
species were captured: Phlebotomus perniciosus,
Phlebotomus ariasi, Phlebotomus sergenti
and Sergentomyia minuta. In one P. perniciosus
female, L. infantum DNA was detected. Blood meal tests showed
that this species had no host preferences and was an opportunistic feeder. An
overall canine leishmaniasis (CanL) seroprevalence of 16.06% was found; the
seroprevalence was 3.88% in dogs housed in kennels and 40.63% in dogs that
attended veterinary clinics. The simultaneous occurrence of dogs and P.
perniciosus infected with L. infantum in the AR
indicates that the region continues to be an endemic area for CanL. Our results
reinforce the need for the systematic spatial distribution of phlebotomine
populations and their Leishmania infection rates and the need
to simultaneously perform pathogen monitoring in both invertebrate and
vertebrate hosts to investigate the transmission, distribution and spreading of
Leishmania infection.
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