Effects of azadirachtin on mortality rate and reproductive system of the grasshopper Heteracris littoralis Ramb. (Orthoptera: Acrididae).
Male and female nymphs of Heteracris littoralis were topically treated with serial concentrations of azadirachtin. Effects on mortality, development, oogenesis and spermatogenesis were observed. Mortalitywas dose-dependent; fourth and fifth instars died about the time of ecdysis. Overaging took place at low concentrations. Ovaries in treated adult females showed complete shrinkage with abolished oocyte growth, and the number of deposited egg pods/female decreased from 4 to 9 in normal females, to 1 to 3 pods in treated insects. Deformation in sperm tubes was observed in treated males. Electronmicrographs revealed disintegration and destruction in follicular cells and mitochondria in females. In males the testicular epithelia and the spermatids completely disintegrated. Treatment with higher doses inhibited cyst formation around the spermatogonia.
azadirachtin, L[C.sub.50], fecundity, oocyte, sperm, ultrastructure
Increasing problems of pest resistance to pesticides enhanced interest in botanical insecticides during recent decades. Extracts from the neem tree Azadirachta indica, of which azadirachtin is the most important active principle, received the attention of many research workers. It was found to exhibit deterrent, antiovipositional, antifeedant, growth-disrupting (growth-regulating), fecundity and fitness-reducing properties on many insect species.
The disruption of insect development and behavior by azadirachtin was observed in Orthoptera (Schmuttereret al. 1993, Linton etal. 1997), Mallophaga (Habluetzel etal. 2006), Hemiptera (Nisbet etal. 1992), Isoptera (Grace &Yates 1992), Coleoptera (Steets 1976, Klocke & Barnby 1989), Lepidoptera (Nathan et al. 2006 a, b), and Diptera (Lucantoni et al. 2006).
In addition, azadirachtin is an effective sterilant. After uptake of the active material, females of some insect pest species were sterilized to various degrees, sometimes completely (Steets 1976, Schmutterer 1987), where juvenoids and ecdysteriods strongly affected fecundity and/or egg sterility if applied during sensitive growth phases of target insects (Karnavar 1987, Tanzubil & McCaffery 1990). On the histological level, azadirachtin was found to inhibit oogenesis (Chosh et al. 1999, Medina et al. 2004) and spermiogenesis (Linton et al. 1997, Abdel-Rahman et al. 2004).
The aim of the present work is to investigate some effects of azadirachtin on histological and ultrastructural levels of the gonads in H. littoralis. The economic importance and the pest status of this species have been documented by El-Shazly (1991).
Materials and Methods
Adults and nymphs of Heteracris littoralis Ramb. were collected from Abou Rawash district (Ciza Covernorate), Egypt. A laboratory stock was reared in electrically heated wooden cages (25 x 25 x 25 x25 cm at a constant temperature of 30[+ or -]1[degrees]C, with fluctuating relative humidity (50 to 70%). Insects were fed clover, Trifolium alexandrinum, from November to May and then fresh leaves of Sesbania sesban. Cages were supplied with suitable ovipositional pots for egg deposition which were kept moistened. Hatched hoppers were transferred to 20x25-cm cylindrical glass jars. After the fourth or fifth moult, hoppers were released in the large cages.
To test the effect of azadirachtin on mortality of 4th, 5th and 6th female nymphal instars, a series of concentrations was prepared (50 to 400 ppm). For each concentration, 20 to 30 insects were tested in five replicates of 5 to 6 grasshoppers each. At the beginning of the stadium, azadirachtinpreparations (5 [micro]l)were topically applied to the neck membrane of the tested instars. Control groups were treated with 5[micro]l acetone. The end point was determined 24 h after treatment by counting dead and moribund individuals in each jar. The average weight was determined for each group, to calculate toxicity/mg body weight. L[C.sub.50] values were determined according to Finney (1971) and mortality corrected according to Abbott's formula (Abbott 1925).
To study the effect of azadirachtin on life span and egg production of the adult females, groups of 20 newly emerged females were topically treated with different concentrations of azadirachtin (25 to 1000 ppm). Five [micro]l of azadirachtin preparation were applied to the neck membrane of the tested insects. The experiment was repeated three times. Insects were reared in groups of ten females and left to mate with normal males in 25x25 x 25-cm cages. Insects were offered suitable amounts of food and ovipositional pots, which were checked daily for egg deposition. Longevity was calculated for all groups.
To study the effect of azadirachtin on the morphology of the ovary and sperm tubes, 10 d-old females and newly emerged males were topically treated with azadirachtin (10 [micro]l of 25 ppm). Treated insects were dissected after 10 days and the ovaries, ovarioles and sperm tubes measured using a stage micrometer and an ocular piece. The measurements were taken three times with 5 replicates each of 5 insects each.
In insect groups used to study azadirachtin effects on the histology of the ovaries and testes, females were treated with 10 pl of 25 ppm, 10 days before their oviposition period (mid-preoviposition period), while males were treated after their imaginal molt with two doses: 25 and 200 ppm. Treated insects were examined 7 d after application. Parts of ovarioles, and sperm tubes of treated insects and control groups were fixed in Carnoy's Formula I for 6 h. Specimens were washed with absolute alcohol, then hydrated with a descending alcoholic series and preserved in Formal Saline solution (Abdel Rahman 1995). Specimens were dehydrated in ascending alcoholic series and cleared in xylene for a few seconds, infiltrated in three changes of paraffin wax (melting point 58[degrees]C) each lasting 20 min. Specimens were sectioned serially at 6p thick using a rotatory microtome (American Optical) and stained with Ehrlich haematoxylin and eosin.
For TEM observations, ovarioles and sperm tubes were fixed in 2.5% glutaraldehyde in phosphate buffer (pH 7.3) at 4[degrees]C for 24 h, then washed in three changes of the fresh buffer. Specimens were post-fixed in 1% osmium tetraoxide in the same buffer for 2 h at 4[degrees]C, then washed in the same buffer and dehydrated in alcoholic series up to absolute alcohol. They were then removed to absolute alcohol and acetone, followed by pure acetone for half an hour each. Infiltration took place in acetone and resin (Epon 812) 2:1 and 1:1 for 4 h each, then into pure resin overnight. Finally, the specimens were put in resin blocks for 3 days at 50[degrees]C. Semi-thin sections (I p thick) were prepared using a glass knife and were stained with toluedene blue for a few seconds. The specimens were examined under a normal light microscope and photographed. Ultra-thin sections (90 nm thick) were obtained using a diamond knife. Sections were put on a cupper grade mesh and stained with uranyl acetate and lead citrate for half an hour, then examined with a Joel JEM JE 1200EXII (Japan) transmission electron microscope and photographed.
Results and Discussion
Effect of azadirachtin on mortality rates and molting
Treated 4th, 5th and 6th instars of female H. littoralis displayed dose-dependent mortality rates, as demonstrated in Fig. 1 and Table 1. Females of the 4th instar were significantly more sensitive, as shown by the L[C.sub.50] values in Table 1. According to the values of the moments ([m.sub.1], [m.sub.2]), differences in the lethal doses between instars were significant at 95% confidence limits. Nymphs of the fourth and fifth instars died at about the time of ecdysis of the control individuals. At 50 ppm, 6th instar nymphs survived for a long period as over-aged individuals. The last instar in control groups lasted 9.8 [+ or -] 0.3 d, while over-aged nymphs survived for 15.16 [+ or -] 2.35 d (6 [+ or -] 1.5 d more than the control).
[FIGURE 1 OMITTED]
Azadirachtin inhibited molting when applied within the first two days after molt onto 6th instar nymphs. Nymphs were unable to undergo or terminate ecdysis. Treated nymphs remained in this condition, unable to shed their old cuticle successfully. Weak ecdysial movements that could last for several hours led to rupturing of old skin along the dorsal midline of the meso- and metathorax and over the pronotum and head capsule, but the shedding was not continued, leading finally to death. When insects were treated 3 to 5 days after the last molt, few adults were able to ecdyse, but shrinkage of wings was observed in emerging individuals.
These results agree with those of Sieber and Rembold (1983) on the molting and mortality of L. migratoria: a dose of 2 [micro]g/g body weight completely prevented molting and prolonged intermolt period, which ranged between 8 and 60 days, compared to 6 (4th instar) and 9 days (5th instar) in the control groups. At lower doses of azadirachtin (1.7 mg/g bodyweight) adults with curled wing tips and reduced longevity were produced. Other authors support these findings: Pener & Shalom (1987), Pener et al. (1989), Van der Host et al. (1989).
On the other hand treatment with higher doses (2.9 mg/g) resulted in death during the imaginal molt. Doses ranging between 6 and 7.3 mg/g body weight caused either death prior to the molt or greatly extended instar duration. Doses of 80 mg/g body weight resulted in death within 24 h [Mordue (Luntz) et al. 1985].
Also, nymphs of S. gregaria treated with azadirachtin survived beyond 40 days without molt and generally died during ecdysis (Rao & Subrahmanyam 1986, Nicol & Schmutterer 1991). Other grasshoppers treated with neem had abnormal nymph-adult molts as in Zonocerus variegatus (Olaifa et al. 1991).
It could be concluded that treatment of H. littoralis 4th, 5th and 6th instar nymphs with high concentration of azadirachtin resulted in high dose-dependent mortality rates during the period of ecdysis in comparison with control groups. At lower concentration, it caused prolongation of the stadium, leading finally to death. In some few cases malformed adults were able to emerge (Table 1).
Effects of azadirachtin on the fecundity and fertility of H. littoralis
Treated female suffered from decrease in number of egg pods/ female in a dose dependent manner (Table 2). The average number decreased from 6.47 [+ or -] 2.21 (control group) to 2.00 [+ or -] 0.82 (females treated with 25 ppm). At higher doses (100 ppm and above) no egg-pods were deposited.
Such was also the case observed in azadirachtin-treated L. migratoria adults (Rembold and Sieber, 1981) as well as in Oncopeltus fasciatus (Heteroptera: Lygaeidae) (Dom et al. 1987), Spodoptera exempta (Lepidoptera: Noctuidae) (Tanzubil and McCaffery, 1990), and in Sesamia calamistis (Lepidoptera: Noctuidae) and Eldana saccharina (Lepidoptera: Pyralidae) (Bruce et al. 2004).
Effects of azadirachtin on the female reproductive system
Effects of azadirachtin on the ovary of H. littoralis.--Female H. littoralis (10-d old adults) topically treated with azadirachtin (10 [micro]l of 25 ppm) showed shrinkage in the whole ovary, besides a partially abolished oocyte growth, as only a few eggs were developed (Fig. 2). The whole organ seemed like the developing ovary of a nymph (3.5[+ or -]0.3 cm in length, compared to the control 7.4[+ or -]0.2 cm), while the average length of ovarioles in treated insects was 1.5[+ or -]0.12 mm, compared to 8.0[+ or -]0.58 mm in the control females. Effects of azadirachtin on the histological components of the ovarioles.--A normal ovariole in female H. littoralis is surrounded by a peritoneal coat of connective tissue which contains a reticulum of muscle fibers. The walls are formed of a layer of compact cuboid epithelial cells, resting upon a basement membrane (the follicular cells) (Fig. 3) and containing a homogenous yolk material. The pronucleus is more or less located in a central position. The matrix contains large yolk spheres and clear spaces near the apices of the follicular cells. At the end of the maturation stage, the follicular epithelial cells provide the vitelline membrane and chorion around the egg. Thus in H. littoralis the follicular cells play an important role in incorporation of yolk granules into the oocytes during vitellogenesis.
[FIGURES 2-3 OMITTED]
Treatment of 10 d-old adultfemales with 25 ppm of azadirachtin affected the above histological components as follows: the oocytes were degenerate, with faint yolk deposition. The follicular cell layer was folded on itself and the cells partly destroyed, their compact shape lost as compared with control specimens. The yolk material was no longer homogenous and contained many vacuoles. The follicular epithelia were irregularly developed, showing clear separation of yolk. In a few cases the oocyte succeeded in reaching the egg stage, but large vacuoles appeared between the yolk spherioles, and the eggs failed to complete their development as compared with the normal compact yolk spherioles in the control groups.
Electron micrographs showed that normal follicle cells appeared with homogenous ooplasm (Fig. 4). Inside the cytoplasm, the mitochondria contained normal cristae, indicating a well-developed capability for follicle-cell protein synthesis and secretion throughout vitellogensis (Fig. 6). During vitellogenesis the nucleus and the nuclear membrane appeared normal and the cytoplasm was homogenous and rich in mitochondria (Fig. 8).
[FIGURES 4, 6 & 8 OMITTED]
Many changes were observed in the histological structure of treated female ovarioles as shown by electron micrograph. During vitellogenesis the follicle cells appeared degenerated, with the presence of many vacuoles (Fig. 5). The contents of mitochondria were totally disintegrated without any cristae inside (Fig. 7). The ooplasm was no longer homogenous; the nucleus appeared with many lysosome-like bodies, indicating the beginning of cell lysis (Fig. 9).
[FIGURES 5, 7 & 9 OMITTED]
Schmutterer et al. (1981, 1993) reported severe damage to the female ovarian follicles of Locusta, Nomadacris, and Schistocerca after treatmentwith azadirachtin. Also, Rembold (1987) reported delayed vitellogenin synthesis in azadirachtin-treated L. migratoria, causing severe damage to the oocytes. Shalom etal. (1988) showed inhibition ofoocytedevelopment andoocyteresorptioninfemale L. migratoria after treatment with azadirachtin The inhibition of ovarian follicle development was also reported by Chosh et al. (1999) on Gesonula punctifrons (Orthoptera: Acrididae) treated with azadirachtin.
The effect of azadirachtin on histological components of the reproductive system, in insects belonging to orders other than Orthoptera, reveals different degrees of damage. Schulz and Schluter, (1983) showed that neem caused dissolving of mitochondria inside the ooplasm in the ovarioles ofEpilachna varivestis (Coleoptera: Coccinellidae). Autophagic vacuoles were formed and the prefollicular epithelium was partly destroyed and folded on itself. Jagannadh and Nair (1997) reported that azadirachtin induced a considerable reduction in the ovariole size and a delay in previtellogenic differentiation of oocytes, in addition to apparent degeneration of ovarioles in larvae, pupae and adults of Spodoptera mauritia (Lepidoptera: Noctuidae). Medinaetal. (2004) reported that azadirachtin affected the ovarioles of Chrysoperla carnea (Neuroptera: Chrysopidae): growing follicles in treated females were significantly smaller than those of controls.
It seems that when azadirachtin is administered at an appropriate time, it can cause severe damage to the oocytes, probably as a result of interference with the vitellogenesis process. This may explain the blocking of the developmental process of ovarioles and consequently the shrinkage of the ovary (Fig. 2). Vitellogenesis is a rather complicated process, involving the deposition of yolk in the oocyte, resulting in a very rapid increase in size. Azadirachtin may inhibit vitellogenin synthesis or absorption which eventually leads to: inhibition of both oogenesis and ovarian ecdyosteroid synthesis (Rembold & Sieber 1981), inhibition of ovarian development (Karnavar 1987), delaying ofthe vitellogenin synthesis process (Rembold 1987) and interference with vitellogenin synthesis and its absorption bythe follicles (Schmutterer et al. 1981, 1993; Chosh et al. 1999).
The effects of azadirachtin application may resemble those of juvenile hormone and its analogues, in respect to ovarian development, time of application and vitellogenin synthesis. Several authors have reported the effects of juvenile hormone analogues/mimics on the histology of the reproductive system as well as oogenesis in different insect groups. Tobe and Pratt (1975) established a link between JH and ovarian maturation in S. gregaria, with a peak of JH synthesis atthe onset of the previtellogenicperiod. Previtellogenesis occurred on days 5 to G in adult females and vitellogenesis occurred on days 7 to 8. Application of the JH mimic was timed with respect to the gonadotrophic cycle of individual insects.
Feyereisen and Tobe (1981) showed that oogenesis and vitellogenesis are inhibited by other JH analogues such as precocene in many insects. Eid et al. (1988) showed that ovaries of the female S. gregaria treated with precocene did not exhibit the vitellogenic stage, while in the normal females vitellogenesis started earlier. Ahi (1988) used another JH mimic (aldrin) on Poehilocerus pictus and mentioned abnormal fragmentation of oocytes with degeneration of the follicular epithelial cells. Polivanova and Triseleva (1989) also observed inhibition of vitellogenesis and sterilization of L. migratoria when last instars were fed on treated food with precocenes. Application of precocene and meth oprene to Phormia regina (black blow fly) inhibited oocyte development and lowered the amount of vitellogenin, respectively (Yin et al. 1989). The follicular epithelium surrounding the vitellogenic oocytes of L. migratoria treated with the JH analogue, methoprene, was found to develop large spaces between the cells, with an eventual decrease in theirvolumes (Davey et al. 1993). Pinto et al. (2000) tested pyriproxyfen on Apis mellifera and reported the inhibition of vitellogenesis.
Effects of azadirachtin on the male reproductive system
Effects of azadirachtin on the sperm tubes of H. littoralis.--Treated sperm tubes showed a swelling in the zone of growth with a slight reduction in its length (Fig. 10b). A follicle in treated males measures 5.15 [+ or -] 0.11 mm in mean length while its mean width is 0.55 [+ or -] 0.13, these values were significantly larger than the control which measures 6.25 [+ or -] 0.21 mm in average length, its average width at the maturation zone being 0.3 [+ or -] 0.02.
[FIGURE 10 OMITTED]
Effects of azadirachtin on the histological components of the sperm tubes.--Histologically, sagittal and transverse sections in the apical part of a sperm tube of males treated with low doses of azadirachtin (25 ppm), showed swelling of the dividing cells; some cells were destroyed and cells in the central part were smaller in size as compared with the control group (Figs 11, 12). In the transformation zone there was clear cell damage, total lyses, and the tissue lost its consistency with the occurrence of many vacuoles. The testicular epithelia in the transformation zone were completely disintegrated; the spermatids were degenerated leaving vacuolated areas. The control group formed normal sperm (Figs 13, 14). In the maturation zone there was disintegration of the epithelial layer, while the matrix appears with many vacuoles and totally damaged cells. In the terminal zone there is degeneration of the sperm bundles and the peritoneal membrane has become finer, with the appearance of large vacuolated areas.
[FIGURES 11-14 OMITTED]
Electron micrographs of follicles from untreated males showed that the spermatocytes undergo their division and development normally (Fig. 15) then complete their differentiation and transformation till sperm is finally liberated (Fig. 16). In insects treated with 200 ppm azadirachtin, the cyst formation around the spermatogonia in the germarium was inhibited without any further development to spermatocytes and with the appearance of many vacuoles (Figs 17, 18). The electron micrographs also showed a clear separation of the basement membrane from the peritoneal membrane.
[FIGURES 15-18 OMITTED]
Schistocerca gregaria treated with azadirachtin suffered from arrested spermatogenic meiosis at Metaphase I (Linton et al. 1997). In Epilachna varivestis (Coleoptera: Coccinellidae) degeneration of the sperm bundles without sperm formation has been reported by Schulz and Schluter (1983). Disintegration of the germ cells and degeneration of the sperm bundles in the testes were also observed by Abdel-Rahman et al. (2004) after treatment of the male Pectinophora gossypiella (Lepidoptera: Gelechidae) with azadirachtin. Shimizu (1988) showed that azadirachtin caused degeneration of spermatocytes in males ofMamestra brassicae (Lepidoptera: Pieridae), suggesting a direct effect of azadirachtin on the testicular membrane, rendering the tissue incapable of developing spermatocytes.
A review of the literature concerning the effects of some other insect growth regulators on insect gonads showed that aldrin caused pycnosis of germ cells leading to incomplete spermiogenesis in Poehilocerus pictus (Ahi 1988).
However, it should be pointed outthat the factors which regulate spermatogenesis are not well understood (Dumser 1980). There is no strong evidence to indicate that hormones are generally involved (Engelmann 1970), but in some moths, the molting hormone could facilitate the process by increasing the permeability of the wall of the testis to some macromolecular factors (Wilde & Loof 1973).
It seems that at higher concentrations azadirachtin prevents the spermatogonia from cyst formation and therefore the spermatocytes fail to maketheirnormal divisions and complete spermiogenesis. On the other hand, at lower concentrations the process of spermatocyte formation proceeds till the appearance of the sperm bundles, but with aberrations and degenerations.
Accepted May 5, 2007
Abbott W.S. 1925. A method of computing the effectiveness ofan insecticide. Journal of Economic Entomology 18: 265-267.
Abdel-Rahman A.G., El-Sayed AX, Laila S.H. and Imam A.I. 2004. Histological alternations in male testis of Pectinophora gossypiella (S.) adults induced by treating larvae with neem formulations. lst Arab Conference Of Applied Biological Pest Control, Cairo, Egypt, 5-7. April 2004, p. 171.
Abdel Rahman K.M. 1995. Studies on the embryology and physiology of the grasshopper Chrotogonus lugubris Blanch. M. Sc. Thesis, Cairo University.
Ahi J. 1988. Histopathological effects of aldrin on the gonads of adult Poehilocerous pictus (Fabr.) Orthoptera: Acrididae. Journal of Environmental Biology 9: 173-182.
Bruce YA., Gounou S., Chabi-Olaye A., Smith H., Schulthess E 2004. The effectofneem (Azadirachta indicaA. Juss) oilon oviposition, development and reproductive potentials of Sesamia calamistis Hampson (Lepidoptera: Noctuidae) and Eldana saccharina Walker (Lepidoptera: Pyralidae). Agricultural and Forest Entomology 6: 223-232.
Davey K.G., Sevala VL., Gordon D.R.B. 1993. The action of juvenile hormone and anti gonadotropin on the follicle cells of Locusta migratoria. Invertebrate Reproduction and Development 24: 39-46.
Dorn A., Rademacher J.M., Sehn E. 1987. Effects of azadirachtin on reproductive organs and fertility in the large milkweed bug, Oncopeltus fzsciatus. Proc. 3d Int. Neem Conf, Nairobi, 1986, Eschborn: GTZ. pp. 273-288.
Dumser J.B. 1980. The regulation of spermatogenesis in insects. Annual Review of Entomology 25: 341-369.
Eid M.A.A., Salem M.S., Taha G.Z. 1988. Effects of precocene II on morphogenesis of the desert locust Schistocerca gregaria. Biochemical Systematics and Ecology 16: 515-520.
El-ShazlyM. M. 1991. Ecological studies on the grasshopper, Heteracris littoralis Rambur, together with some studies on its physiology and control. Ph. D. Thesis, Cairo Univ.
Engelmann E 1970. The Physiology of Insect Reproduction. Pergamon Press, Oxford.
Feyereisen R., Tobe S.S. 1981. A rapid partition assay for routine analyses of juvenile hormone released by insect corpora allata. Analytical Biochemistry, 111: 372-375.
Finney D.J. 1971. Probit Analysis. Cambridge University Press, Cambridge, United Kingdom 120 pp.
Ghosh D., Das P, Chel G. 1999. Effect of neem seed extract (azadirachtin) on growth and reproductive development of Gesonula punctifrons (Orthoptera). Proceedings Zoological Society, Calcutta. 52: 80-84.
Grace J.K., Yates J.R. 1992. Behavioural effects of a neem insecticide on Coptotermes formosanus (Isoptera: Rhinotermitidae). Tropical Pest Management 38: 176-180.
Habluetzel A., Carnevali E, Lucantoni L., Grana L., Attili A.R., Archilei E, Antonini M., Valbonesi A., Abbadessa V., Esposito E, van der Esch S. A. 2006. Impact of the botanical insecticide Neem Azal[R] on survival and reproduction of the biting louse Damalinia limbata on angora goats. Veterinary Parasitology 144: 328-337.
Jagannadh V, Nair V.S. K.1997. Effects of azadirachtin on ovarian development and fecundity in Spodoptera mauritia. Proceedings Indian National Science Academy Part B, Biological Sciences 63: 597-604.
Kamavar G.K. 1987. Influence of azadirachtin on insect nutrition and reproduction. Prodeedings Indian Academy of Sciences (Animal Sciences) 96: 341-347.
Klocke J.A., Barnby M. A. 1989. Plant allelochemicals as sources and models of insect control agents. In Phytochemical Ecology: Allelochemicals, Mycotoxins and Insect Pheromone and Allomones (Eds Chou C. H. and Walker G. R.). Institute of Botany, Academia Sinica Monograph Series No. 9. Taipei, Taiwan.
Linton Y.M., Nisbet A.J., Mordue (Luntz) A.J. 1997. The effects of azadirachtin on the testes of the desert locust, Schistocerca gregaria (Forskal). Journal of Insect Physiology 43: 1077-1084.
Lucantoni L., Giusti E, Cristofaro M., Pasqualini L., Esposito E, Lupetti P, Habluetzel A. 2006. Effects of a neem extract on blood feeding, oviposition and oocyte ultrastructure in Anopheles stephensi Liston (Diptera: Culicidae). Tissue and Cell 38: 361-371.
Medina P, Budia E, del. Estal P, Vinuela E. 2004. Influence of azadirachtin, a botanical insecticide, on Chrysoperla carnea reproduction: toxicity and ultrastructural approach. Journal of Economic Entomology 97: 43-50.
Mordue (Luntz) A.J., Cottee R K., Evans K.A.1985. Azadirachtin: its effects on gut motility, growth and moulting in Locusta. Physiological Entomology 10: 431-437.
Nathan S. S., Kalaivani K., Sehoon K., Murugan K. 2006a. The toxicity and behavioural effects of neem limonoids on Cnaphalocrocis medinalis (Guenee), the rice leaf folder. Chemosphere 62: 1381-1387.
Nathan S. S., Kalaivani K., Chung P G., Murugan K. 2006b. Effect of neem limonoids on lactate dehydrogenase (LDH) of the rice leaf folder, Cnaphalocrocis medinalis (Guenee) (Insecta: Lepidoptera: Pyralidae). Chemosphere 62: 1388-1393.
Nisbet A.J., Woodford J.A., Strang R.H.C. 1992. The effects of azadirachtin on feeding by Myzus persicae pp. 424-425. Proc. 81 Int. Symp. Insect-Plant Relationships (Eds Menken S. B. J., Visser J. H. and Harrewijn, P.).
Nicol C.M.Y, Schmutterer H. 1991. Contact effects of seed oil from the neem tree, Azadirachta indica (A. Juss.), on nymphs of the gregarious phase of the desert locust, Schistocerca gregaria (Forek.). Journal of Applied Entomology 111: 197-205.
Olaifa J.L, Adedokun T.A., Adenuga A.O. 1991. Antifeedant and growth-regulating effects of neem products on the variegated grasshopper Zonocerus variegatus L. (Orthoptera: Pyrgomorphidae). Revue de Zoologie Africaine 105: 157-162.
Pener M.P., Shalom U. 1987. Endocrine manipulations, juvenile hormone and ontogenesis ofmale sexual behaviour in locusts. Insect Biochemistry 17:1109-1113.
Pener M.P., van den Broek A.T.M., van Marrewijk W.J.A., van Doorn J.M., van der Horst D.J., Beenakkers A.M.T. 1989. Developmentof imaginal competence to adipokinetic hormone in Locusta: lipid and carbohydrase levels, and glycogen phosphorylase activityin azadirachtin-induced over-aged nymphs. Comparative Biochemistry and Physiology. B, Comparative Biochemistry 94: 293-298.
Pinto L.Z., Bitondi M.M.G., Simoes Z.L.P. 2000. Inhibition of vitellogenin synthesis in Apis mellifera workers by a juvenile hormone analogue, pyriproxyfen. Journal of Insect Physiology 46: 153-160.
Polivanova E.N., TriselevaT.A. 1989. Suppression of development of Locustrz migratoria L. during nymphal feeding on plants containing prococenes, and prospects for using these plants in biological control. Doklady Biological Sciences 306: 289-291.
Rao P.J., Subrahmanyam B. 1986. Azadirachtin induced changes in development, food utilization and haemolymph constituents of Schistocerca gregaria Forsk. Zeitschrift fur Angewandte Entomolgie Memorias Instituto Oswald Cruz 102: 217-224.
Rembold H. 1987. The azadirachtin-potent insect growth inhibitors. Memorias Instituto Oswald Cruz. 82: 61-66.
Rembold H., Sieber K.P. 1981. Inhibition of oogenesis and ovarian ecdysteroid synthesis by azadirachtin in Locusta migratoria migratoroides (R. & E). Zeitschrift fur Naturforschung, C36: 466-469.
Schmutterer H.1987. Fecundity-reducing and sterilizing effects of neem seed kernel extracts in the Colorado potato beetle, Leptinotarsa decemlineata. Proc. 3d Int. Neem Conf, Nairobi, 1986, Eschborn: GTZ. pp. 289-296.
Schmutterer H., Asher K.R.S., Rembold H. 1981. Natural pesticides from the neem tree (Azadirachta indica). lst Int. Neem Conf. Rottach-Egern. 297 pp.
Schmutterer H., Baumgart M., Freisewinkel D., Langenwald J., Nicol C.M.Y. 1993. The effects of neem oil and other neem products on nymphs and resulting adults ofSchistocerca gregaria, Nomadacris septemfasciata, Locusta migratoria migratorioides, and Zonocercus variegatus. Journal of Applied Entomology 116: 178-186.
Schulz W. D., Schhiter LL 1983. Structural damage caused by neem in Epilichna varivestis: a summary of histological and ultrastructural data. II Tissues affected in adults, pp. 237-252. Proc. 2nd Int. Neem Conf., (Rauischolzhausen 1983).
Shalom LL, Applebaum S.W., Pener M P. 1988. Vitellogenesis and oocyte development in azadirachtin-induced fifth-instar overage nymphs of Locusta migratoria (L.). Archives Insect Biochemistry Physiology 9: 313-322.
Shimizu T. 1988. Suppressive effects of azadirachtin on spermiogenesis of the diapausing cabbage army worm, Mamestra brassicae, in vitro. Entomologia Experimentalis et Applicata 46: 197-199.
Sieber K.P., Rembold H. 1983. The effects of azadirachtin on the endocrine control of moulting in Locusta migratoria. Journal of Insect Physiology 29: 523-527.
Steets R. 1976. Zur Wirkung eines gereinigten Extraktes aus Friichten von Azadirachta indica A. Juss aufLeptinotarsa decemlineata Say (Coleoptera: Chrysomelidae). Zeitschrift fur Angewandte Entomolgie 82: 169-176.
Tanzubil P B., McCafferyA.R.1990. Effects ofazadirachtin on reproduction in the African armyworm (Spodoptera exempta). Entomologia Experimentalis et Applicata 57: 115-121.
Tobe S.S., Pratt G.E. 1975. Corpus allatum activity in vitro during ovarian maturation in the desert locust, Schistocerca gregaria. Journal of Experimental Biology 62: 611-627.
Van der Horst D.J., Van Doorm J.M., Pener M.P, Van den BroekA.T.M., Van Marrewijk W.J.A., Beenakkers A.M.T. 1989. Development of imaginal competenceto adipokinetic hormone in Locusta: lipophorin conversions in prococene-induced adultiforms and azadirachtin-induced over-aged nymphs. Comp. Comparative Biochemistry Physiology 92: 133-136.
Wilde J. De, Loof A. De 1973. Reproduction endocrine control. In: Rockstein M. (Ed.) The Physiology of Insecta. Vol. 1 pp. 97-157.
Yin C.M., Zou B.X., Stoffolano J.G. Jr. 1989. Precocene II treatment inhibits terminal oocyte development but not vitellogenin synthesis and release in the black blowfly, Phormia regina Meigen. Journal ofInsect Physiology 35: 465-474.
N.A. GHAZAWI, E.D. EL-SHRANOUBI, M.M. EL-SHAZLY, K.M. ABDEL RAHMAN Entomology Department, Faculty of Science, Cairo University, Egypt. Email: firstname.lastname@example.org
Table 1. Effect of different concentrations of azadirachtin on the mortality rate of fourth, fifth and sixth female instar nymphs of H. littoralis. Percent dead Concentration (PPm) Fourth instar Fifth instar Sixth instar 400 86.66 80.00 73.33 200 84.61 60.00 66.67 100 50.00 50.00 46.67 75 30.00 37.50 23.07 50 20.00 20.00 14.28 Control 0.00 0.00 0.00 L[C.sub.50] (PPM) * 101.50 (^) ** 126.12 (B) 148.22 (c) Toxicity in mg/g body 7.51 (^) 15.76 (B) 28.00 (c) weight Moments ([m.sub.l]- 6.05 - 9.31 10.33 - 17.09 20.21 - 33.21 [m.sub.2]) at 95% confidence SE Slope 0.14 0.16 0.12 * L[C.sub.50] was estimated according to Abbott (1925) and Finney (1971). ** L[C.sub.50] values followed by different letters are significantly different from each other based on 95% confidence limits. Table 2. Effect of different doses of azadirachtin on the longevity and egg production of H. littoralis (mean [+ or -] SD). Longevity (days) Dose Ppm Pre-ovip. Period Ovip. Period Control 20.50 [+ or -] 3.14 42.60 [+ or -] 4.61 (a) (15-25) (36-61) 25 22.50 [+ or -] 2.96 8.70 [+ or -] 6.40 (b) (17-28) (1-21) 50 22.60 [+ or -] 4.58 7.60 [+ or -] 6.40 (b) (17-27) (1-18) 75 23.70 [+ or -] 4.06 6.80 [+ or -] 5.40 (b) (18-28) (1-15) 100 30.30 [+ or -] 2.60 (x) - (24-36) 200 25.20 [+ or -] 1.20 (x) - (20-27) 400 22.50 [+ or -] 1.10 (x) - (18-24) 1000 21.30 [+ or -] 3.30 (x) - (15-25) Longevity (days) Dose Ppm Post-ovip. period Total Control 6.30 [+ or -] 2.11 (a) 70.21 [+ or -] 3.11 (a) (3 - 11) (62-90) 25 2.70 [+ or -] 1.10 (b) 36.10 [+ or -] 5.60 (b) (1-4) (18-53) 50 2.20 [+ or -] 1.10 (b) 33.20 [+ or -] 6.40 (b) (1-3) (18-48) 75 2.40 [+ or -] 1.30 (b) 33.60 [+ or -] 5.90 (b) (1-5) (19-48) 100 - 30.30 [+ or -] 2.60 (x) (24-36) 200 - 25.20 [+ or -] 1.20 (x) (20-27) 400 - 22.50 [+ or -] 1.10 (x) (18-24) 1000 - 21.30 [+ or -] 3.30 (x) (15-25) Dose Ppm No. egg-pods/female No. eggs/pod Control 6.47 [+ or -] 2.21 (a) 31 [+ or -] 6.0 (a) (4-9) (26-45) 25 2.00 [+ or -] 0.82 (b) 29 [+ or -] 4.0 (b) (1-3) (21 -33) 50 1.85 [+ or -] 0.69 (b) 27 [+ or -] 3.6 (b) (1-3) (24-31) 75 1.64 [+ or -] 0.67 (b) 19 [+ or -] 2.4 (c) (1-2) (17-24) 100 - - 200 - - 400 - - 1000 - - Values followed by different superscripts (a, b, c) in the same column are significantly different (P < 0.05). (x) individuals died without laying eggs. ovip., ovipostion.
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|Author:||Ghazawi, N.A.; El-Shranoubi, E.D.; El-Shazly, M.M.; Rahman, K.M. Abdel|
|Publication:||Journal of Orthoptera Research|
|Date:||Jan 1, 2007|
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