Four postharvest pathogens were used to assess the antimicrobial activity of the prepared spice extracts. Aspergillus niger Tiegh. (Ascomycota), Fusarium sambucinum Fuckel (Ascomycota), Pythium sulcatum R.G. Pratt & J.E. Mitch. (Oomycota), and Rhizopus stolonifer (Ehrenb.:Fr.) Vuill. (Zygomycota) were maintained on potato dextrose agar (PDA; Becton Dickinson, Sparks, MD, USA) at 24°C.

Extracts were prepared from cinnamon bark (Cinnamomum verum J. Presl), ginger rhizome (Zingiber officinale Roscoe), horseradish powder (Armoracia rusticana P.G. Gaertn., B. Mey. & Scherb), and nutmeg seed (Myristica fragrans Houtt.). Dried cinnamon bark sticks and nutmeg seed were reduced to a fine powder in a spice grinder. Ginger rhizomes were surface sterilized for 5 min in 70% ethanol, washed with water, and lyophilized prior to being reduced to powder using a mortar and pestle. Extracts were prepared by suspending 10 to 100 g of each dried powdered spice in 100 mL of sterile distilled water at 24°C for 36 h. The extracts were recovered by filtering the suspensions on Whatman paper (#1) followed by centrifugation at 3,100 x g for 15 min. The supernatant was recovered and cold sterilized through a 0.45 µm filter unit (Nalgene, Rochester, NY, USA).

To determine their effect on A. niger, F. sambucinum, P. sulcatum and R. stolonifer mycelial growth, the produced extracts were incorporated into PDA. In an initial trial, spice extracts (cinnamon, ginger, horseradish and nutmeg) were incorporated at 0.05 g mL^‑1 into warm (45°C) sterile PDA prior to pouring into Petri dishes. PDA without spice extracts served as controls. In a second trial, cinnamon and ginger extracts were incorporated into PDA (as described above) at the following concentrations: 0 (control), 0.05, 0.10 and 0.15 g mL^‑1. Concentrations of extracts are expressed as the quantity of dried spice (in grams) per mL of PDA. Agar plugs (0.5 cm diam) covered with actively growing mycelia of the four pathogens were individually inoculated on the media and incubated for 2 (for R. stolonifer), 3 (for A. niger) or 4 d (for F. sambucinum and P. sulcatum) in the dark at 24°C. After the incubation period, mycelial growth of each pathogen was measured as the average of two perpendicular diam of the colony minus 0.5 cm (diam of the agar plug). All experiments were conducted according to a completely randomized design with five replications.

To determine the inhibitory effect of cinnamon and ginger extracts on potato dry rot and carrot cavity spot, the extracts were sprayed on artificially inoculated potato tubers and mature carrot roots. In dry rot experiments, potato tubers (Solanum tuberosum L. var. Superior) were surface sterilized with a 0.5% solution of sodium hypochlorite for 15 min, rinsed with distilled water, and air dried. Wounds (0.5 cm diam, 4 mm deep) were performed on each tuber using a cork borer as previously described by Mecteau et al. (2008). Agar plugs (0.5 cm diam) covered with actively growing mycelia of F. sambucinum were placed in each wound. Agar plugs containing no fungi mycelia served as non-inoculated controls. In cavity spot experiments, mature carrot roots (Daucus carota L. cv. Caropak) were surface sterilized with a 0.5% solution of sodium hypochlorite for 5 min, rinsed with distilled water, and air dried. Wounding was performed on each carrot root by gently scraping the epidermis with a sterile razor blade according to Benard and Punja (1995). Agar plugs (0.5 cm diam) covered with actively growing mycelia of P. sulcatum were placed directly on the wounded carrot epidermis. Agar plugs containing no P. sulcatum mycelia served as non-inoculated controls. The inoculated and non-inoculated potato tubers and carrot roots were individually transferred to plastic containers lined with moistened paper towels. Each potato tuber and carrot root was sprayed with 2 mL of cinnamon or ginger extracts at concentrations of 0.05, 0.10 and 0.15 g mL^‑1. Sterile distilled water (2 mL) served as the control. Dry rot and cavity spot severity was measured as the average of two perpendicular diam of the lesions after a 7-d incubation period at 24°C or a 10-d incubation period at 15°C for dry rot and cavity spot, respectively. The experimental unit consisted of one potato tuber or one carrot root in an individual plastic container. The experiment was conducted according to a completely randomized design with four replications.

Analysis of variance (ANOVA) was carried out with the GLM procedure of SAS (SAS Institute Inc. 1999) and, when significant (P < 0.05), treatment means were compared using Fisher's protected least significant difference (LSD) test.

In the initial in vitro trial, the four spice extracts (cinnamon, ginger, horseradish and nutmeg) were tested at a concentration of 0.05 g L^‑1 against the four postharvest pathogens. At this concentration, cinnamon extract caused 100% inhibition of mycelial growth in A. niger whereas the other extracts did not inhibit the growth of this pathogen (Table 1). In F. sambucinum, only the cinnamon extract significantly inhibited mycelial growth when compared to the control (Table 1). Cinnamon and ginger extracts completely inhibited the growth of P. sulcatum. Nutmeg extract also significantly inhibited the growth of P. sulcatum, albeit to a lesser extent (28%) (Table 1). In R. stolonifer, cinnamon and ginger extracts caused the highest inhibition of mycelial growth relative to the control. Nutmeg extract also inhibited R. stolonifer growth, though significantly less so than cinnamon and ginger extracts (Table 1). At a concentration of 0.05 g mL^‑1, horseradish extract did not cause a significant inhibition in any of the tested fungi or oomycota.

In a second in vitro trial, cinnamon and ginger extracts were assayed at different concentrations to assess their inhibitory effect on the tested pathogens. Significant statistical interactions between extracts and concentrations were found and the data are therefore presented for each extract. In general, cinnamon and ginger extracts inhibited the pathogens in a dose-dependent manner for F. sambucinum and R. stolonifer. Indeed, increasing the concentration in the medium from 0.05 to 0.15 g mL^‑1 caused a significant decrease in mycelial growth in these two fungi (Tables 2 and 3). Results from this trial confirmed that 0.05 g mL^‑1 of cinnamon extract was necessary to completely inhibit A. niger and P. sulcatum, whereas 0.10 and 0.15 g L^‑1 were required to totally inhibit F. sambucinum and R. stolonifer, respectively (Table 2). Conversely, 0.05 g mL^‑1 of ginger extract was necessary to completely inhibit P. sulcatum and 0.15 g mL^‑1 was necessary to completely inhibit R. stolonifer. A concentration of 0.15 g mL^‑1 of ginger extract significantly inhibited F. sambucinum, albeit by only 29%. None of the tested concentrations of ginger extract significantly inhibited the mycelial growth of A. niger (Table 3).

Various concentrations of cinnamon and ginger extracts were further tested to determine their suppression of potato dry rot (F. sambucinum) and carrot cavity spot (P. sulcatum). Significant statistical interactions between extracts and concentrations were found and the data are therefore presented for each extract. Cinnamon extract provided significant control of dry rot (approximately 20% relative to the water control) at 0.10 g mL^‑1. A concentration of 0.15 g mL^‑1 of cinnamon extract afforded the highest suppression of both dry rot and cavity spot, reducing lesions by 51 and 31%, respectively (Fig. 1). Ginger extracts did not suppress dry rot at any of the tested concentrations (Fig. 2). A ginger concentration of 0.15 g mL^‑1 significantly reduced cavity spot lesions by 35%.