1. Introduction
Entomopathogenic fungi are among the important biological control agents of insect pests, by causing lethal infections and regulating insect and mite populations in nature by epizootics [1] - [3] . These biocontrol agents infect a wide range of insect orders including Hemiptera, Coleoptera and Lepidoptera which are of great concern in worldwide agriculture but some strains of these fungi could be host specific with a very low risk of attacking non-target organisms or beneficial insects [4] .
The entomopathogenic as comycete, Beauveria bassiana (Balsamo) Vuillemin is an important pathogen of insects and it has been developed as a microbial insecticide for use against many major arthropod pests [5] [6] . It has been developed as a microbial insecticide for use against many major pests, including lepidopterans. It is reported to be non-toxic to humans and other vertebrates, so it can be applied on commodities [7] .
Plodia interpunctella (Hübner) (Lepidoptera: Pyralidae), is a serious pest of raw and processed food products worldwide [8] - [11] . Some reports have pointed out to the promising control effects of B. bassiana on Indian meal moth [12] [13] . However the fungi encountered some limiting factors to show adequate level of pest control.
The use of B. bassiana alone for the control of many stored product pests requires a high application rates. The action of fungal penetration to the host integument is dependent to physicochemical properties of cuticle including thickness, sclerotization, and presence of fatty acids as well as cuticle destroying enzymes [14] - [16] .
The presence of cuticular lipids in insect integument could protect the insect from pathogenic microorganisms. If any agent could damage this barrier, greater penetration and higher pathogen virulence would be expected.
Diatomaceous Earth (DE), a natural product composed of the fossils of diatoms, can exhibit such role with its special properties like integument scarification and adsorbing wax from cuticle layer [17] , causing the release of subcuticular compounds that have a synergistic effect on conidial attachment and virulence of entomopathogenic fungi [18] [19] .
Several studies document that DE formulations are very effective against a wide range of stored products pests, persist on the product for a long period and can be easily removed from the grains [20] - [22] .
It is generally accepted that these materials act as desiccants on insect cuticle, and that insects exposed to DE particles die from rapid water loss [17] [23] [24] . Low mammalian toxicity is another important characteristic of DE [25] , rendering it a potential and safe method for pest control.
Our objective in this study was to determine the effects of B. bassiana and DE, alone or in combination, on the Indian meal moth larvae as well as clarify interactions of these two agents.
2. Materials and Methods
2.1. Insect Rearing
Indian meal moth, P. interpunctella was acquired from a laboratory population at the Department of Plant Protection, University of Tehran and reared under laboratory conditions (25˚C ± 1˚C, 65% ± 10% RH and 16:8 L:D) in Polyethylene boxes (30 × 20 × 15 cm) covered with a piece of fine cloth.
Artificial diet including wheat bran, yeast, honey, and glycerol, prepared by the method described by Sait et al. [26] , was used for insect rearing. No antibiotic or fungicide was added to the diet.
2.2. Fungal Isolate and Cultures
The isolate used in this study was B. bassiana ETU105, originally isolated from soil using Galleria-bait and preserved in Laboratory of Biological Control at the Department of Plant Protection, University of Tehran. Fungal isolate was grown on Sabouraud dextrose agar plus 1% yeast extract (SDAY) in 9 cm diameter Petri dishes (Figure 1) and incubated under conditions of 25˚C ± 1˚C, 75 ± 10 RH and 16:8 L:D for 14 days. Colony was preserved at 4˚C.
Fungal conidia were collected by scraping conidial layer using sterilized scalpel into 0.02% Tween 80. The conidial concentration was estimated using a haemocytometer. Each mg of collected conidia contained 4.5 × 108 spores. Five serial concentrations 103 - 107 conidia mg−1 diet were prepared by mixing adequate conidia with artificial diet. An electric mixer was used for 5 min to prepare an even mixture.
2.3. Diatomaceous Earth
Diatomaceous Earth (DE) was prepared from Kimia Sabz Avar Company located in Iran. It was oven-dried initially at 60˚C for two hours, and then two concentrations of 500 and 2000 mg/kg were prepared by adding sufficient DE to artificial diet. These two concentrations were selected based on the results of our preliminary test.
(a) (b)
Figure 1. Beauveria bassiana, (a) Fully sporulated on SDAY medium; (b) Scanning electron micrograph of conidiophores and conidia clusters (original, bar = 10 µm).
2.4. Bioassay
There were 17 treatments: five fungal dose rates alone, five fungal dose rates in combination with each of the two DE dose rates and the two DE rates alone. Five serial dose rates of fungal conidia were 103 - 107 con. mg−1 diet. Fifteen g of diet containing treatments were placed in series of glass Petri dishes with 9 cm in diameter. An additional series of dishes containing untreated diet served as a control.
After the preparation of the dishes, 15 third instar larvae of P. interpunctella were introduced into each dish. The dishes were placed in incubators set up at temperature of 25˚C ± 1˚C and RH of 65% ± 5% for a week. All the experiments were repeated four times. Larval mortality was assessed daily until 7 days after exposure.
2.5. Statistical Analysis
Mortality counts were corrected by using Abbott’s formula [27] . The experiment was designed and conducted in a factorial Complete Randomized Design (CRD). The pooled data were analyzed separately for each treatment category (Fungus alone, DE alone, DE 500+ fungus, DE 2000+ fungus), by submitting the mortality counts to ANOVA’s for dose rate. Means were separated using the Tukey test at P < 0.05. SAS software version 9.1 was used for statistical analysis. The LC50 values were estimated with probit analysis using POLO-Plus [28] .
3. Results
3.1. Effect of B. bassiana on P. interpunctella Larvae
Mortality rates of third instar larvae of P. interpunctella treated with B. bassiana increased with increasing conidial concentration and time of exposure. Differences among lethal effects established by different conidial concentrations of fungal isolate were significantly different (F = 72.49, df = 5, P < 0.0001).
The LC50 value of fungus at 7 d after treatment on P. interpunctella larvae was 9.8 × 105 con. mg−1 diet. Comparative virulence of B. bassiana isolate against L3 instar of P. interpunctella indicated that mortality of larvae began at the third day after exposure and reached to 61.7% at the day 7. The LT50 value of fungus at 1 × 107 con. mg−1 was 6.59 d (6.23 - 7.12 days lower and upper 95% C.I., respectively).
3.2. Effect of Diatomaceous Earth on P. interpunctella Larvae
Larval mortality reached to a maximum of 28.3% and 71.7% after 7 d exposure to 500 and 2000 mg/kg DE concentrations, respectively. There were highly significant differences in larval mortality resulting from different concentrations of DE (F = 121.13, df = 2, P < 0.0001). Larval mortality ranged from 1.7 to a maximum of 71.7% over the range of tested concentrations.
3.3. Combination of B. bassiana and DE
Data on comparative virulence of B. bassiana isolate in combination with DE against L3 instar of P. interpunctella is brought in Table 1. These results showed that there was a synergistic relationship between fungus and DE targeting larvae of P. interpunctella.
The LC50 value for B. bassiana plus DE 500 mg/kg was 4.6 × 104 con. mg−1 diet and with DE 2000 mg/kg was 1.65 × 103 con. mg−1 diet in contrast to the LC50 of 9.8 × 105 con. mg−1 diet for B. bssiana alone (Table 2). There were significant differences among these treatments (F = 72.49, df = 5, P < 0.0001).
The combination treatment of fungus with DE caused the highest mortality at 7d after treatment which was significantly greater than all other treatments. With concentration of 500 ppm DE, mortality of larvae began at the second day after exposure to 1 × 107 con. mg−1 of fungus and reached to 100% at the day 7.
With DE 500, LT50 value for fungus with concentration of 1 × 105 con. mg−1, diminished to 3.9 d which was significantly lower than that of fungus alone with 6.6 d (F = 11.48, df = 26, P < 0.0001). This value showed a greater reduction when DE 2000 was applied, such that it was reduced to 2.1 d. The log-probit regression lines of LC50 had slopes of 0.34 without DE, 0.65 with DE 500 and 0.64 with DE 2000. These parameters for LT50s were 8.21, 6.54 and 5.35, respectively (Table 3).
4. Discussion
Results from bioassays on P. interpunctella larvae showed that the B. bassiana isolate ETU105 was virulent against the pest, however, a relatively high concentration of 9.8 × 105 conidia mg−1 diet needs to cause 50% mortality during 7 d. These results stand somewhat in agreement with that of Buda and Pečiulytė [29] who found that after treatment with concentration of 2.6 × 106 conidia mg−1 of B. bassiana, larval mortality of the species, was reached to 50% during 5 days.
Many of the important pests in grain storage have proven to be susceptible to B. bassiana, but its high production costs and high application rates make it economically unreachable [30] - [36] .
Table 1. Mean percent mortalities of P. interpunctella third instar larvae caused by B. bassiana in combination with diatomaceous earth.
Table 2. LC50 values of B. bassiana alone or in combination with two diatomaceous earth doses based on experiments with 3rd instar larvae of P. interpunctella.
Number of treated larvae = 360.
Table 3. Values of LT50 for B. bassiana at 1 × 107 con. mg−1 diet alone or in combination with two doses of diatomaceous earth based on experiments with 3rd instar larvae of P. interpunctella.
Number of treated larvae = 360; df = 26.
The concentration of 500 ppm of DE, caused 28.3% mortality of P. interpunctella larvae with increasing the DE concentration to 2000 ppm could enhance the mortality rate to 71.7 percent. This result approved the finding of Sabbour et al. [13] , however, the LC50 of fungus in their study was 1.29 × 109 con. mg−1 which was much greater than that of our finding, 1 × 105 con. mg−1 diet. This difference may be related to fungus isolate or population of P. interpunctella.
Our results also are in conformity with findings of Akbar et al. [18] who found that DE increased the efficacy of B. bassiana against Tribolium castaneum larvae. Also Michalaki et al. [19] found that the effectiveness of entomopathogenic fungus, Metarhizium anisopliae can be benefitted by the presence of DE against T. confusum larvae.
DE does not leave any toxic residue because of its physical effects; however, regarding the possible health issues, lower concentrations should be preferred. Low concentration of DE does not leave any harmful residue on stored commodities. If it could be prepared from good quality and suitable resources, would have very low effect on human breathing system. Also, using suitable breathing mask, such effects could be greatly diminished.
Fast and stable effectiveness, make DE an appropriate choice to substitute chemical compounds for stored product protection. Moisture increase of environment can lead to less effectiveness of DE, so it is more successful in control of stored product pests. Moreover such pests are little in size, have a higher body surface to body volume ratio, and encountered to low water content of commodities. The lack of insect resistance against DE is another important prominence which enhances its capability for use as a part of integrated pest management program.
DE does not have any significant effect on stored products by own itself and can be removed easily with air blowing or washing. This can decrease applying chemical pesticides in grain deposit. Using DE at concentration of 500 ppm, the LC50 value of B. bassiana was significantly decreased on P. interpunctella larvae.
The exact mechanisms by which DE interacts with B. bassiana are not clear but may involve a combination of increased availability of water and other nutrients, removal or mitigation of inhibitory materials, alteration of adhesive properties, and physical disruption of the cuticular barrier [18] . Lord [12] [34] proposed that lipid removal may contribute to the synergistic interaction between B. bassiana and DE against some stored grain pests.
Akbar et al. [18] showed the number of B. bassiana conidia attached to the larval cuticle of Tribolium castaneum was significantly greater with DE presence than without it. The mean counts of conidia were 212.7 with DE and 90.9 without DE.
Michalaki et al. [19] revealed that DE benefits the fungal efficacy only when conidial concentration exceeds a certain “active threshold”. Below this “threshold”, a considerable amount of conidia may be damaged by the presence of DE, or DE particles may partially lose their desiccant capacity.
5. Conclusion
Finally, this study clearly indicated that simultaneous use of B. bassiana and DE against larvae of P. interpunctella, not only reduced the required concentration of fungus or DE, but it would also shorten the time need for showing their effects. On the other hand, the greatest factor in the loss of inoculum viability of entomopathogenic fungi under field conditions is inactivation caused by UV light [37] [38] , but grain storage environment does not have such disadvantage, thus it could be a suitable environment for integrated application of B. bassiana and DE.
NOTES
*Corresponding author.