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Susceptibility of Elasmopalpus lignosellus (Lepidoptera: Pyralidae) larvae to entomopathogenic nematodes (Rhabditida)1 1 This work is part of the dissertation defended by the first author, Maria Eduarda Berlatto Magnabosco, in the Graduate Program in Qualidade Ambiental at the Universidade Federal de Uberlândia.

ABSTRACT

The cornstalk borer, Elasmopalpus lignosellus (Lepidoptera: Pyralidae), reduces the productive potential of maize crops and is a difficult pest to manage. A management program using different methods could improve the control of E. lignosellus. Considering the potential of entomopathogenic nematodes (EPN) in reducing insect pest populations in soil, the objective of this study was to evaluate the virulence of these EPN and adjust their concentration for controlling E. lignosellus larvae under laboratory and greenhouse conditions. In the laboratory, the virulence of five EPN populations was tested; then, Heterorhabditis amazonensis MC01 was tested at four concentrations. In the greenhouse, H. amazonensis MC01 was tested at four concentrations and was applied to vessels containing maize plants and six larvae. After five days, mortality was evaluated, and means were compared using Tukey’s test (p-value < 0.05). Heterorhabditis amazonensis MC01 and S. carpocapsae All were equally virulent, reducing the larva population by more than 90%. The concentration of H. amazonensis MC01 that caused the highest mortality of larvae in the laboratory was 182 infective juveniles (IJ) larva-1. In the greenhouse, the nematode was also considered virulent to E. lignosellus since all concentrations tested caused larval mortality greater than 70%.

Keywords
biological control; Heterorhabditis ; lesser cornstalk borer; plant protection; Steinernema

INTRODUCTION

The lesser cornstalk borer, Elasmopalpus lignosellus (Zeller) (Lepidoptera: Pyralidae), feeds on several plant species of high economic value. The larvae penetrate the base of the plant in the initial stages of development of the culture, just below the ground, creating a gallery in the stem that can cause the breakage and death of the plants, resulting in stand reduction. Chemical control is the main method that has been used with seed treatment, but it is not always effective to reduce pest populations (Vieira et al., 2020Vieira ECS, Ávila CJ, Vivan LM, Silva GF, Silva IF, Vieira MCS & Silva PG (2020) Controle da lagarta Elasmopalpus lignosellus (Zeller, 1848) (Lepidoptera: Pyralidae) com diferentes inseticidas aplicados em tratamento de sementes na cultura da soja. In: Pereira AIA (Ed.) Coletânea Nacional sobre Entomologia 2. Ponta Grossa, Atena Editora. p.43-50.).

The larvae typically occur inside the seedlings or in cocoons made of web and soil particles, and they remain close to the stem, which makes handling them difficult. In the 1980s, new management strategies using natural enemies for the lesser cornstalk borer were developed (Jham et al., 2005Jham GN, Silva AA, Lima ER & Viana PA (2005) Identificação (GC e GC-MS) de acetatos insaturados em Elasmopalpus lignosellus e sua atividade biológica (GC-EAD e EAG). Journal of Separation Science, 28:281-285.; 2007Jham GN, Silva AA, Lima ER & Viana PA (2007) Identification of acetates in Elasmopalpulus lignosellus pheromone glands using a newly created mass spectral database and kóvats retention indices. Química Nova, 30:916-919.). Nevertheless, chemical control is still the most used method, even though its incorrect use may cause problems such as the development of resistant populations, reduction of natural enemies, and outbreaks of secondary pests (Neri et al., 2005Neri DKP, Moraes JC & Gavino MA (2005) Interação silício com inseticida regulador de crescimento da lagarta-do-cartucho Frugiperda de Spodoptera (JE Smith, 1797) (Lepidoptera: Noctuidae) em milho. Ciência e Agrotecnologia, 29:1167-1174.).

Among the organisms studied for E. lignosellus population control, entomopathogenic nematodes (EPN) have potential, as they inhabit the soil and have the ability to maintain their viability and remain active, controlling larvae in different instars (Grewal et al., 2001Grewal PS, de Nardo EAB & Aguillera MM (2001) Entomopathogenic nematodes: potential for exploration and use in South America. Neotropical Entomology, 30:191-205.). Moreover, they have a symbiotic association with bacteria that are released into the hemolymph of the insect, causing its death (Cagnolo et al., 2004Cagnolo SR, Donari YM, & di Rienzo JA (2004) Existence of infective juveniles in the offspring of first and second generation adults of Steinernema rarum (OLI strain): evaluation of their virulence. Journal of Invertebrate Pathology 85:33-39.; Dolinski, 2006Dolinski C (2006) Nematoides como agentes do controle biológico de insetos. In: Oliveira Filhos EC & Monnera RG (Eds.) Fundamentos para regulação de semioquímicos inimigos naturais e agentes microbiológicos de controle de pragas. Brasília, Embrapa. p.73-101.). Georgis (1992)Georgis R (1992) Present and future prospects for entomopathogenic nematode products. Biocontrol Science and Technology, 2:83-99. and Jaramillo & Saavedra (2007)Jaramillo RM & Saavedra GM (2007) Ensayos sobre el efecto del nematodo entomopatógeno Heterorhabditis sp. en el control de Elasmopalpus lignosellus en el cultivo de espárrago. Arenagro Revista de la Asociación de Productores de terrenos de Chavimochic, 1:17-18. highlighted the potential of using EPN as biological control agents for E. lignosellus, verifying the pest control potential in peanut and asparagus crops.

Before being field-tested, the virulence of EPN against target insects must be evaluated, as nematode populations cause different mortality rates in different hosts. In addition, the optimal concentration of EPN that cause pest mortality also varies (Kaya & Hara, 1981Kaya HK & Hara AH (1981) Susceptibilidade de várias espécies de pupas lepidópteras ao nematódeo entomógeno Neoplectana carpocapsae. Journal of Nematology, 13:291-294.; Fuxa et al., 1988Fuxa JR, Richter AR & Agudelo-Silva F (1988) Efeito da idade do hospedeiro e da cepa nematoide na suscetibilidade de Spodoptera frugiperda a Steinernema feltiae. Journal of Nematology, 20:91-95.). Therefore, the objective of the present study was to select EPN with potential to control E. lignosellus larvae and, depending on the laboratory virulence data, adjust the concentration of the most virulent nematode to be applied under laboratory and greenhouse conditions.

MATERIALS AND METHODS

The experiments were performed at the Federal University of Uberlândia, Umuarama Campus (18°53’40’’S, 48°15’35’’W). Nematodes were multiplied in Tenebrio molitor L. (Coleoptera: Tenebrionidae) larvae raised following Potrich et al. (2007)Potrich TD, Lorini I, Voss M, Steffens MCS & Pavani DP (2007) Metodologia de criação de Tenebrio molitor em laboratório para obtenção de larvas. Passo Fundo, Embrapa Trigo. 1p. (Documentos, 82).. Dead T. molitor larvae were washed with water and placed in a dry chamber (petri dish with filter paper) for five days. After drying, they were removed and placed in White traps (1927White GF (1927) A method for obtaining infective nematode larvae from cultures. Science, 66:302-303. to collect infective juveniles (IJ), following Molina & López (2001)Molina JP & López NJC (2001) Producción in vivo de tres entomonematodos con dos sistemas de infección en dos hospedantes. Revista Colombiana de Entomología 27:73-78.. Infected larvae were maintained in a biochemical oxygen demand (B.O.D.) incubator at 26 ± 2 °C. IJ were used up to three days after emergence and stored at 16 ± 2 °C for up to five days.

Fifteen adult E. lignosellus couples were placed in cylindrical PVC cages (15 cm × 20 cm) lined with filter paper, where the adults were fed with a 10% honey aqueous solution. Every two days, the papers containing the postures were removed and stored in capped plastic Gerbox® plates. Daily, as the eggs hatched, the first instar larva were transferred to 100-mL plastic pots containing modified Chalfant (1975)Chalfant RBA (1975) Simplified technique for rearing the lesser cornstalk borer (Lepidoptera: Phycitidae). Journal of the Georgia Entomological Society, 10:33-37. artificial diet, without tetracycline and Vanderzant’s mixture, and added with 0.2 g of benzoic acid and 2 mL of corn oil. An approximately 2-cm layer of autoclaved vermiculite (120 °C, 1 atm, 20 min) was added over the larvae to make the breeding environment similar to the natural conditions used for the construction of larval shelters. After 15 days, the larvae were removed for use in the tests.

Virulence of entomopathogenic nematodes against larvae

Initially, the virulence of Heterorhabditis amazonensis MC01, H. amazonensis JPM3, H. amazonensis GL, Steinernema carpocapsae All, and Heterorhabditis amazonensis Nepet 11 against E. lignosellus larvae was analyzed under laboratory conditions. Ten second and third instar larvae were arranged in glass Petri dishes (9-cm diameter) lined with two sheets of filter paper containing an approximately 8-cm3 block of artificial diet. For each case, 1 mL of nematode suspension was applied at a concentration of 100 IJ pupa-1 per plate. A control treatment received only distilled water.

Five replications per treatment were performed in a completely randomized design. The plates were kept in a B.O.D. incubator at 25 ± 2 °C, 70% relative humidity (RH), and 24 h in the dark. Mortality assessments were performed after 24, 48 and 72 h.

Data with normal distribution and homoscedasticity were submitted to analysis of variance (ANOVA) with Tukey’s test comparison between the means obtained for each nematode (p < 0.05). Data without normal distribution were fitted to the Generalized Linear Model with binomial distribution (ANODEV), and Tukey’s test was used to compare the means (p < 0.05).

Concentration of Heterorhabditis amazonensis MC01 against larvae under laboratory conditions

To adjust the concentration of application of IJ, H. amazonensis MC01 was applied to E. lignosellus larvae at concentrations of 50, 100, 150, and 200 IJ larva-1 on Petri dishes containing 10 third and fourth instar larvae. Control plates received only distilled water. The volume of suspension/water per plate was 1 mL at the respective concentrations with five replications in a completely randomized design, totaling 25 plates.

The experiments were kept in a B.O.D. incubator at 25 ± 2 °C, 70% RH, and 24 h in the dark. Dead larvae were counted after 24, 48, 72 and 96 h. Data were subjected to ANOVA and subsequent regression analysis using the software Sigma Plot v.12.0, after meeting the assumptions of normality of residuals and homoscedasticity.

Concentration of Heterorhabditis amazonensis MC01 against larvae under greenhouse conditions

Untreated corn seeds of the BM 3061 hybrid were sown in 2-L plastic pots containing approximately 1.5 kg of sieved soil, classified as Dystrophic Dark Red Latosol (Embrapa, 2006Embrapa - Empresa Brasileira de Pesquisa Agropecuária (2006) Sistema brasileiro de classificação de solos. 2ª ed. Rio de Janeiro, Centro Nacional de Pesquisa de Solos. 306p.). Four seeds were sown in each pot, thinning to one plant per pot after emergence. The pots were fertilized with approximately 1.8 g of the 4-14-8 formulated per pot (i.e., 750 kg ha-1).

When the plant reached approximately 20 cm in height, six fourth instar larvae were released per pot, and then the suspensions containing four concentrations of H. amazonensis MC01 190, 210, 230, and 250 IJ larva-1 were applied on the soil surface using an automatic pipette. A treatment was maintained without the application of nematodes as a control. Each treatment was performed with five replications, totaling 25 pots distributed in a completely randomized design. In order to prevent the larvae from escaping, the pots were protected by a metal structure covered with an anti-aphid screen.

Assessment was performed after five days, verifying the percentage of larva mortality caused by the nematode. Means were compared using Tukey’s test (p < 0.05). In all tests, the dead larvae were kept in B.O.D. at 25 ± 2 °C in a dry chamber for four days for subsequent dissection, and then observed under a stereoscopic microscope to confirm nematode mortality.

RESULTS AND DISCUSSION

Virulence of entomopathogenic nematode isolates to larvae

After 24 h of application of the EPN isolates, none of the observed larvae were dead. At 48 and 72 h after application, statistical differences were found by ANOVA and ANODEV, respectively. After 48 h, all the tested nematodes caused mortality of the E. lignosellus larvae, differing from the control, in which low mortality from natural events was observed. In addition, no difference in virulence was observed between the isolates, all of which caused more than 60% mortality. After 72 h, the isolates that showed the highest virulence, with mortality > 90%, were S. carpocapsae All and H. amazonensis MC01, with no differences between them (Table 1).

Table 1
Elasmopalpus lignosellus larvae’ mean mortality after 48 and 72 h of application of entomopathogenic nematode isolates

Based on the obtained results, only H. amazonensis MC01 was selected for the subsequent tests, as it was isolated from the same region of the experiments and was thus more adapted to the local conditions than the other isolates. This isolate searches for the insect in the soil, with horizontal displacement of the soil (Campbell & Gaugler, 1997Campbell JF & Gaugler R (1997) Inter-specific variation in entomopathogenic nematode foraging strategy: dichotomy or variation along a continuum? Fundamental and Applied Nematology, 20:393-398.). Moreover, it has appendages on the cephalic region (Griffin et al., 2005Griffin C, Boemare N & Lewis EE (2005) Biology and behaviour. In: Grewal P, Ehlers RU & Shapiro-Ilan D (Eds.) Nematodes as Biocontrol Agents. Wallinford, CABI Publishing. p.47-64.) that contribute to the penetration into the insect’s body (Geden et al., 1985Geden CJ, Axtell RC & Brooks WM (1985) Susceptibility of the lesser mealworm, Alphitobius diaperinus (Coleoptera: Tenebrionidae) to the entomogenous nematodes Steinernema feltiae, S. glaseri (Steinernematidae) and Heterorhabditis heliothidis (Heterorhabditidae). Journal of Entomological Science, 20:331-339.; Andaló et al., 2012Andaló V, Santos V, Moreiria GF, Moreira CC, Freire M & Moino Junior A (2012) Movement of Heterorhabditis amazonensis and Steinernema arenarium in search of corn fall armyworm larvae in artificial conditions. Scientia Agricola, 69:226-230.).

Several studies have verified the action potential of steinermatids on lepidopteran larvae (Van Damme et al., 2015Van Damme VM, Beck BKEG, Berckmoes E, Moerkens R, Wittemans L, De Vis R, Nuyttens D, Casteels HF, Maes M, Tirry L & De Clercq P (2015) Efficacy of entomopathogenic nematodes against larvae of Tuta absoluta in the laboratory. Pest Management Science, 72:1702-1709.; Kamali et al., 2017Kamali S, Karimi J & Koppenhöfer AM (2017) New insight into the management of the tomato leaf miner, Tuta absoluta (Lepidoptera: Gelechiidae) with entomopathogenic nematodes. Journal of Economic Entomology, 111:112-119.). However, Steyn et al. (2019)Steyn LAI, Addison P & Malan AP (2019) Potential of South African entomopathogenic nematodes to control the leaf miner, Holocacista capensis (Lepidoptera: Heliozelidae). South African Journal of Enology and Viticulture, 40:01-09. highlighted the importance of performing studies that include Heterorhabditis in the isolation selection tests, as they observed Heterorhabditis spp. controlling Holocyst capensis Van Nieukerken & Geertsema (Lepidoptera: Heliozelidae). Kepenekci et al. (2013)Kepenekci İ, Tülek A, Alkan M & Hazır S (2013) Biological control potential of native entomopathogenic nematodes against the potato tuber moth, Phthorimaea operculella (Zeller) (Lepidoptera: Gelechiidae) in Turkey. Pakistan Journal of Zoology, 45:1415-1422. also observed H. bacteriophora causing high mortality (80%) in larvae of Phthorimaea operculella (Zeller) (Lepidoptera: Gelechiidae).

Concentration of Heterorhabditis amazonensis MC01 against larvae under laboratory conditions

Significant differences were found by ANOVA in all hours evaluated after application of H. amazonensis. The mortality of E. lignosellus after 24 and 48 h of application of the nematode was low, but after 72 h, a mortality of 48% was observed for 50 and 100 IJ larva-1, 60% for 150 IJ larva-1, and 70% for 200 IJ larva-1.

For 72 and 96 h, the relationship between larvae mortality and isolate concentrations was adjusted by a quadratic regression model with coefficient of determination (R2) of 91.32% and 90.31%, respectively. From the derivative of the parabola equation, maximum mortality was calculated at 190 IJ larva-1 for 72 h (66%) and at 182 IJ larva-1 for 96 h (78.7%) (Figure 1).

Figure 1
Mortality of Elasmopalpus lignosellus larvae at different Heterorhabditis amazonensis MC01 concentrations after 72 and 96 h of exposure.

The pathogenicity and virulence of H. amazonensis GL were assessed for E. lignosellus pupae in the laboratory, with CL50 = 6.49 IJ/cm2 after 48 h of nematode contact with pupae, and CL90 = 39.7 IJ/ cm2 after 48 h in the laboratory (Magnabosco et al., 2020Magnabosco MEB, Andaló V & Carvalho FJ (2020) Susceptibility of Elasmopalpus lignosellus pupae to entomopathogenic nematodes in maize. Revista Brasileira de Milho e Sorgo, 19:e1115.). This shows that both H. amazonensis populations are virulent to E. lignosellus with potential for pest control.

Few studies have been performed on EPN with E. lignosellus. Nevertheless, concentration tests were performed for other lepidopteran larvae. Helicoverpa armigera (Hübner) (Lepidoptera: Noctuidae) inoculated with 100 and 500 IJ of H. bacteriophora presented mortality between 12% and 30% after 72 h of exposure, reaching up to 50% after 96 h (Kary et al., 2012Kary NE, Dastjerdi HF, Golizadeh A & Mohammadi D (2012) A laboratory study of susceptibility of Helicoverpa armigera (Hübner) to three species of entomopathogenic nematodes. Munis Entomology and Zoology, 7:372-379.). However, S. frugiperda exposed to different Heterorhabditis isolates at a concentration of 100 IJ larvae-1 had mortality rates between 40% and 85%, indicating the variability between the infection processes of different isolates at different dosages and specific hosts (Andaló et al., 2010Andaló V, Santos V, Moreiria GF, Moreira CC & Moino Junior A (2010) Evaluation of entomopathogenic nematodes under laboratory and greenhouses conditions for the control of Spodoptera frugiperda. Ciência Rural, 40:1860-1866.). Observing the results for pupae of E. lignosellus, H. armigera, and S. frugiperda and the variations between the concentrations, we reinforce the importance of specific tests between entomopathogen and host.

A reduction in maximum mortality values was also observed in other studies and can be explained by a possible competition between nematodes interfering with infection rates (Selvan et al., 1993Selvan S, Campbell JF & Gaugler R (1993) Density-dependent effects on entomopathogenic nematodes (Heterorhabditidae and Steinernematidae) within an insect host. Journal of Invertebrate Pathology, 62:278-284.; Giometti et al., 2011Giometti FHC, Leite LG, Tavares FM, Schimt FS, Batista Filho A & Dell’Aqua R (2011) Virulência de nematóides entomopatogênicos (Nematoda: Rhabditida) a Sphenophorus levis (Coleoptera). Bragantia, 70:81-86.; Santos et al., 2011Santos V, Moino Junior A, Andalo V, Moreira CCM & Olinda RA (2011) Virulência de nematoides entomopatogênicos (Rhabditida: Steinernematidae e Heterorhabditidae) para o controle de Diabrotica speciosa germar (Coleoptera: Chrysomelidae). Ciência e Agrotecnologia, 35:1149-1156.; Rohde et al., 2012Rohde C, Moino Junior A, Carvalho FD & Silva MAT (2012) Selection of entomopathogenic nematodes for the control of the fruit fly Ceratitis capitata (Diptera: Tephritidae). Brazilian Journal of Agricultural Sciences, 7:797-802.). Thus, we infer that the increase in the concentration of nematodes does not always cause greater host mortality, as the nematode may tend to be more attracted to insects previously infected by the same organism. The scarce knowledge on the interaction between IJ and host makes it difficult to interpret the dynamics of infection caused by EPN (Lewis, 2002Lewis EE (2002) Behavioural ecology. In: Gaugler R (Ed.) Entomopathogenic Nematology. New York, CABI Publishing. p.205-223.).

Concentration of Heterorhabditis amazonensis MC01 against larvae under greenhouse conditions

Under the greenhouse conditions, no significant difference was observed among the concentrations tested (Tukey’s test at 5% probability). This shows that the suspension with the lowest concentration (190 IJ larva-1) offered the maximum control these pathogens could achieve, and that a higher concentration did not significantly increase control. Therefore, H. amazonensis MC01 was considered virulent to larvae of E. lignosellus under the conditions tested, and at all concentrations, the average larval mortality was greater than 70% (Figure 2).

Figure 2
Mean mortality of Elasmopalpus lignosellus larvae inoculated at different concentrations of H. amazonensis MC01 in a greenhouse.

Similar results were found by Leite et al. (2007)Leite LG, Tavares FM, Bussóla RA, Amorim DS, Ambrós CM & Harakava R (2007) Virulence of entomopathogenic nematodes (Nemata: Rhabditida) against larva of the fungus gnat Bradysia mabiusi (Lane, 1959) and persistence of Heterorhabditis indica Poinar et al. 1992 on organic substrates. Arquivos do Instituto Biológico, 74:337-342. for H. indica (IBCB-n05), which applied at 5.7 and 22.6 IJ cm-2 showed no statistical difference, reaching the efficiency of 75% and 85%, respectively, in the control of larvae of Bradysia mabiusi (Lane) (Diptera: Sciaridae). Different concentrations of Heterorhabditis sp. RSC01 also did not significantly affect the mortality of larvae of Diabrotica speciosa (Germar) (Coleoptera: Chrysomelidae) in corn (Santos et al., 2011Santos V, Moino Junior A, Andalo V, Moreira CCM & Olinda RA (2011) Virulência de nematoides entomopatogênicos (Rhabditida: Steinernematidae e Heterorhabditidae) para o controle de Diabrotica speciosa germar (Coleoptera: Chrysomelidae). Ciência e Agrotecnologia, 35:1149-1156.). Likewise, different concentrations of H. amazonensis RSC1 did not influence the efficiency against nymphs of Mahanarva spectabilis (Hemiptera: Cercopidae) in a greenhouse, and all concentrations tested caused a mortality of 57.14% (Batista et al., 2014Batista ES de P, Auad AM, Andalo V & Monteiro CM de O (2014) Virulence of entomopathogenic nematodes (Rhabditida: Steinernematidae, Heterorhabditidae) to spittlebug Mahanarva spectabilis (Hemiptera). Arquivos do Instituto Biológico, 81:145-149.).

Overall, the results show that the optimal concentration under conditions of maximum exposure of the larvae to nematodes is similar to that under greenhouse conditions. However, this does not exclude the need for field tests, in which other variables must be considered.

CONCLUSIONS

From the isolates tested on the E. lignosellus larvae, H. amazonensis MC01 and S. carpocapse All reducing the larva population by more than 90%.

The concentration of H. amazonensis MC01 that caused the highest mortality of larvae in the laboratory was 182 IJ larva-1. In the greenhouse, the nematode was also considered virulent to E. lignosellus since all concentrations tested caused larval mortality greater than 70%. In general, we found that the longer the exposure time, the greater the mortality of the larvae.

ACKNOWLEDGEMENTS, FINANCIAL SUPPORT, AND FULL DISCLOSURE

To the Federal University of Uberlândia and the Graduate Program in Agronomy for the financial support. The authors report that there is no conflict of interest.

  • 1
    This work is part of the dissertation defended by the first author, Maria Eduarda Berlatto Magnabosco, in the Graduate Program in Qualidade Ambiental at the Universidade Federal de Uberlândia.

REFERENCES

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  • Andaló V, Santos V, Moreiria GF, Moreira CC, Freire M & Moino Junior A (2012) Movement of Heterorhabditis amazonensis and Steinernema arenarium in search of corn fall armyworm larvae in artificial conditions. Scientia Agricola, 69:226-230.
  • Batista ES de P, Auad AM, Andalo V & Monteiro CM de O (2014) Virulence of entomopathogenic nematodes (Rhabditida: Steinernematidae, Heterorhabditidae) to spittlebug Mahanarva spectabilis (Hemiptera). Arquivos do Instituto Biológico, 81:145-149.
  • Cagnolo SR, Donari YM, & di Rienzo JA (2004) Existence of infective juveniles in the offspring of first and second generation adults of Steinernema rarum (OLI strain): evaluation of their virulence. Journal of Invertebrate Pathology 85:33-39.
  • Campbell JF & Gaugler R (1997) Inter-specific variation in entomopathogenic nematode foraging strategy: dichotomy or variation along a continuum? Fundamental and Applied Nematology, 20:393-398.
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  • Geden CJ, Axtell RC & Brooks WM (1985) Susceptibility of the lesser mealworm, Alphitobius diaperinus (Coleoptera: Tenebrionidae) to the entomogenous nematodes Steinernema feltiae, S. glaseri (Steinernematidae) and Heterorhabditis heliothidis (Heterorhabditidae). Journal of Entomological Science, 20:331-339.
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  • Leite LG, Tavares FM, Bussóla RA, Amorim DS, Ambrós CM & Harakava R (2007) Virulence of entomopathogenic nematodes (Nemata: Rhabditida) against larva of the fungus gnat Bradysia mabiusi (Lane, 1959) and persistence of Heterorhabditis indica Poinar et al. 1992 on organic substrates. Arquivos do Instituto Biológico, 74:337-342.
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Publication Dates

  • Publication in this collection
    08 July 2024
  • Date of issue
    2024

History

  • Received
    22 Jan 2022
  • Accepted
    24 Mar 2024
Universidade Federal de Viçosa Av. Peter Henry Rolfs, s/n, 36570-000 Viçosa, Minas Gerais Brasil, Tel./Fax: (55 31) 3612-2078 - Viçosa - MG - Brazil
E-mail: ceres@ufv.br