A comparative bioefficacy of seed and root extracts of a medicinal plant, Withania somnifera when administered to prepupae of lepidopteran insects, Spodoptera litura (Lepidoptera: Noctuidae) and Pericallia ricini (Lepidoptera: Arctiidae)

The lepidopterans, Spodoptera litura and Pericallia ricini, are polyphagous pests of agricultural importance. The unscrupulous and non-judicious use of chemical pesticides for controlling the insect pests has resulted into severe environmental hazards, threatening non-target organisms and human health. Administration of seed and root extracts of a medicinal plant, Ashwagandha (Withania somnifera) to prepupae of two economically important insect pests viz. S. litura and P. ricini resulted into disruption of molting and metamorphosis leading to a number of developmental aberrations such as prolongation of the life span of prepupae, postponement of pupal-adult ecdysis, ecdysial failure, reduced pupation and adult emergence, formation of larval-pupal and pupal-adult intermediates, abnormal pupae, and adultoids. Treatment with seed extracts of W. somnifera was more effective as it alone caused mortality in both the lepidopteran insects viz. S. litura and P. ricini, whereas no such effect was observed when treated with root extracts. P. ricini was more susceptible to W. somnifera as it resulted into formation of larval-pupal-adult chimeras in addition to effects described earlier, whereas this effect was not observed in the case of S. litura. These results are similar to these produced by the administration of JHAs and hence mimic their action by the way of interfering with the neuroendocrine system.

Withania somnifera (Family: Solanaceae), also known as Ashwagandha or Indian ginseng, is an important medicinal plant used extensively in Ayurveda, the classical Indian system of the medicine (Bhattacharya, Bhattacharya, Sairam, & Ghosal, 2000). This medicinal plant possesses a spectrum of diverse phytochemicals such as alkaloids (withanine, withasomnine, somniferine), steroidal lactones (withaferins, withanolides), and steroids (stigmasterol, sitoinosides) that are responsible for a broad range of biological implications (Dar, Hamid, & Ahmad, 2015). It is used as remedy for several disease due to its potential therapeutic effects such anti-inflammatory, antioxidant, anti-aging, anticancer, anti-anxiety, anti-depressant, anti-ulcer, antihypertensive, antimicrobial, cardioprotectant, immunomodulator, and hypoglycemic agent (Alam et al., 2012). Whereas the medicinal properties of Ashwagandha are well documented, its insect growth regulatory effects have not been described in details except in a few instances involving only last instar larvae of certain lepidopteran pests (Gaur & Kumar, 2017a, 2017b. In the present communication, a comparative efficacy of seed and root extracts of Ashwagandha, W. somnifera, has been described as a result of administration of these to prepupae of two economically important lepidopteran pests viz. S. litura and P. ricini.

Insect rearing
Wild eggs of S. litura and P. ricini were collected from castor plant (Ricinus communis) in the Department of Zoology, University of Allahabad, Allahabad (25°27′ N 81°44′ E), UP, India and kept in the BOD incubator at 26 ± 2°C, 70 ± 5% relative humidity. After post hatching, neonate larvae were kept in sterilized glass troughs and provided soft, fresh, sterilized castor leaves for feeding. In order to maintain sanitation, the developing larvae were transferred daily to clean sterilized glass troughs and supplied with fresh sterilized leaves for feeding. When developing larvae reached the penultimate larval instar, they were transferred to glass troughs containing 3-5″ of sterilized sawdust. The last instar larvae of S. litura pupated in the sawdust, whereas the last instar larvae of P. ricini pupated by forming cocoons attached to the walls of the glass troughs. The pupal duration lasted for 7-9 days in case of S. litura and 9-11 days in P. ricini, and thereafter, adult moths emerged. The adult moths were kept in ventilated cages (30 × 30 × 30 cm) and given 10% honey solution for feeding and fresh castor leaves for oviposition.

Plant material and extraction
The dried seeds of W. somnifera were purchased online from Srivilliputtur, Tamil Nadu (India). The seeds were washed thoroughly with distilled water and dried at room temperature away from sunlight for a week and grinded with the help of grinder to obtain a fine powder, whereas the dried root powder of W. somnifera was purchased online from Srijain Ayurvedic Pharmacy, Kattedan, Hyderabad (India).
The acetone extract of seed and root of W. somnifera was prepared according to the method of Kumar (2017a, 2017b). 125 g of seed and root powder were separately weighed and dissolved in 500 ml of acetone and heated at 50°C for 2 days using Soxhlet apparatus and filtered through Whatman no. 1 filter paper. In order to ensure complete evaporation of acetone from the filterates, the filerates were condensed by using rotatory evaporator under reduced pressure of 22-26 mmHg at 45°C resulting into formation of a dark brown, sticky, thick paste of crude extract of seeds and roots of W. somnifera. The desired doses were obtained by dissolving 1 mg of crude extract into 1 ml pure acetone and kept at 4°C.

Experimental procedure
Twenty prepupae each of S. litura and P. ricini were administered topically with 5 μg, 10 μg, 15 μg, and 20 μg doses of seed and root extracts of W. somnifera on the dorsum of the posterior abdomen with the help of a microapplicator according to method of Singh and Kumar (2015a). Controls were treated with similar doses of pure acetone only. After treatment, both the treated and control prepupae were transferred to sterilized glass troughs containing saw dust for pupation. All the experiments were replicated thrice. Observations were recorded 3 h post treatment till the emergence of adultoids/adults. All the dead and malformed/deformed specimens were fixed in Bouin's fluid and preserved in 70% ethyl alcohol for morphological studies and photography.

Statistical analysis
All the data regarding duration of prepupae and pupal-adult ecdysis were subjected to one-way ANOVA to find out significant difference between mean prepupal and pupal-adult duration of the treated and control groups. Correlation coefficient was also calculated to determine the correlation between the doses administered and various morphological deformities observed. All the calculations were done using Graph Pad Prism 2007, 5.01 software (San Diego, California).

Results
Topical administration of seed and root extracts of W. somnifera to prepupae of S. litura and P. ricini resulted into disruption of growth, molting, and metamorphosis. The developmental abnormalities as a consequence of treatment of both the seed and root extracts of W. somnifera in S. litura and P. ricini comprised delay in prepupal and pupal-adult ecdysis, ecdysial stasis, formation of larval-pupal and pupal-adult intermediates, reduction in pupation and adult emergence, and formation of abnormal pupae and adultoids.

Mortality
Administration of seed extracts of W. somnifera to prepupae of S. litura and P. ricini resulted into mortality in a dose-dependent manner showing a positive correlation both in S. litura (r = 0.90) ( Table 1) and P. ricini (r = 0.98) (Table 3). However, no mortality occurred when prepupae of S. litura and P. ricini were treated with root extracts of W. somnifera (Tables 2 and 4).

Prepupal duration
The prepupal duration was prolonged significantly in a dose-dependent manner as a consequence of treatment of prepupae of both the insects viz. S. litura and P. ricini with the seed and root extracts of W. somnifera (Tables 1, 2, 3, and 4).
Therefore, treatment with seed extracts was more effective in inducing prolongation of prepupal duration in S. litura as compared to similar result induced by treatment with root extracts in P. ricini.

Pupal-adult ecdysis
Administration of seed and root extracts of W. somnifera to prepupae of S. litura and P. ricini resulted into significantly increased pupal-adult ecdysis duration as compared to controls, showing a positive correlation between the doses administered and prolongation of pupal-adult ecdysis at all the doses of seed and root extracts of W. somnifera (Tables 1, 2, 3, and 4). There was a maximum prolongation of 0.88 days (F = 4.73; df = 4, 115; p ≤ 0.05) (r = 0.80) ( Table 1) in pupal-adult ecdysis at 20 μg when S. litura prepupae were treated with W. somnifera seed extracts as compared to only 0.43 days (F = 5.40; df = 4, 184; p ≤ 0.001) (r = 0.89) (Table 2) at the same dose when treated with root extracts.
Therefore, seed extracts of W. somnifera were much more effective in causing postponement of pupal-adult ecdysis in both S. litura and P. ricini as compared to root extracts of W. somnifera.

Ecdysial failure
Ecdysial failure was observed as a result of treatment of prepupae of both S. litura and P. ricini with seed and root extracts of W. somnifera (Tables 1, 2, 3, and 4).
Depending upon the degree of abnormality, the ecdysial stasis caused by the seed and root extracts of W. somnifera in polyphagous pest, S. litura could be broadly classified into the following types: 1. Pupa with larval exuviae attached to whole ventral surface of abdomen, dorsal surface of posterior abdomen including posterior extremity of the body (Plate 1b). In some cases, larval exuviae remained attached to entire ventral surface of the pupa, whereas it was found adhered to only posterior region of the dorsal abdomen (Plate 1c) or larval exuviae attached to ventral surface of the abdomen of pupae (Plate 1d) 2. Pupa deformed and twisted having larval exuviae attached to ventral surface of head, thorax, and abdomen and posterior region of dorsal abdomen (Plate 1e). 3. Pupa with larval head capsule remained attached to ventral surface of head region; deformed thoracic legs and proboscis; reduced pupal cremaster (Plate 1f).
Depending upon the extent of abnormality, the ecdysial failure caused by the seed and root extracts of W. somnifera in hairy caterpillar, P. ricini could be divided into the following types: 1. Prepupa showing complete ecdysial failure, unable to cast off larval exuviae (Plate 2b). 2. Pupa with larval exuviae attached to all over the body surface except at the dorsal surface of thorax (Plate 2c). 3. Pupa with white and untanned antennae; larval exuviae found attached to the ventral and dorsal surfaces of the abdomen (Plate 2d). 4. Abnormal white untanned pupa with larval exuviae attached to entire ventral surface and dorsal region of posterior abdomen (Plate 2e). 5. Abnormal pupa showing deformity in the adjoining area between thorax and abdomen and larval exuviae attached to ventral surface of the body and dorsal surface of posterior abdomen (Plate 2f). In some pupae, the anterior part of the body including head and thorax was extremely malformed and twisted with larval exuviae attached to entire ventral surface of the body (Plate 2 g).

Larval-pupal intermediates
Topical administration of seed and root extracts of W. somnifera to prepupal instar of S. litura and P. ricini resulted into formation of larval-pupal intermediates in all the treated groups (Tables 1, 2, 3, and 4). The larval-pupal intermediates produced by the administration of seed and root extracts of W. somnifera to S. litura could be broadly classified into following types: The larval-pupal intermediates produced by the treatment of seed and root extracts of W. somnifera to P. ricini could be classified into following types:

Pupation
Administration of seed extracts of W. somnifera to prepupae of P. ricini resulted into reduction in percentage pupation. The percentage pupation was reduced from 100% in controls to 72%, 68%, 57%, and 52% at 5 μg, 10 μg, 15 μg, and 20 μg doses respectively showing negative correlation between the doses administered and the percentage pupation in a dose dependent manner (r = − 0.94) ( Table 3). The percentage pupation was also reduced with treatment of seed and root extracts of W. somnifera to prepupae of S. litura and root extracts of W. somnifera treatment to P. ricini. There was a negative correlation between the doses administrated and the percentage pupation (Tables 1, 2, 3, and 4).

Abnormal pupae
Administration of seed and root extracts of W. somnifera to prepupae of S. litura resulted into formation of abnormal pupae. Abnormal pupae consisted of reduced wings and ventral surface of anterior abdomen white and unsclerotized (Plate 1 l). In some pupae, the right antenna was free and not glued to the body (Plate 1 m) or highly deformed pupa with extremely reduced fore wing, white, unsclerotized right hind wing, and free proboscis not glued to the body (Plate 1n).
Administration of seed and root extracts of W. somnifera to prepupae of P. ricini also resulted into formation of abnormal pupae.
Depending upon the degree of abnormalities, these have been classified into following types: 1. Abnormal pupa with partially tanned, swollen, bulged left wing; both the wings reduced; white antennae; left prothoracic leg, right mesothoracic leg, and anterior part of ventral abdomen untanned; intersegmental spaces between abdominal sclerites unusual in being unsclerotized and extended (Plate 2 s). 2. Abnormal pupa showing partially white, untanned right mesothoracic leg, distal end of metathoracic legs, and anterior part of ventral abdomen (Plate 2 t) 3. Abnormal pupa with reduced, swollen bulged left fore wing (Plate 2u). 4. Abnormal pupa with highly deformed body parts like eyes, proboscis, crumpled and reduced wings; undeveloped thoracic legs; white, untanned, and deformed abdomen (Plate 2v). 5. Abnormal pupa with reduced, less tanned left wing; white and untanned proximal and distal part of right antenna (Plate 2w).

Pupal-adult intermediates
Topical administration of seed and root extracts of W. somnifera to prepupae of S. litura resulted into formation of pupal-adult intermediates. Administration of seed and root extracts of W. somnifera to prepupae of P. ricini also resulted into formation of pupal-adult intermediates. These pupal-adult intermediates could be broadly classified into following types:

Adult emergence
Administration of seed extracts to prepupae of S. litura and P. ricini resulted into suppression of adult emergence in a dose dependent manner. There was a negative correlation between the doses administered and percentage of adult emergence both in S. litura (r = − 0.84) ( Table 1) and P. ricini (r = − 0.85) (Table 3). Adult emergence was also reduced by administration of root extracts of W. somnifera to prepupae of S. litura and P. ricini. There was a negative correlation between the doses applied and incidence of adult emergence both in case of S. litura (r = 0.74) ( Table 2) and P. ricini (r = − 0.75) ( Table 4).

Larval-pupal-adult intermediates
Topical administration of seed and root extracts of W. somnifera to prepupae of P. ricini resulted into formation of larval-pupal-adult intermediates, whereas these were not produced in case of S. litura (Tables 3 and 4).
Depending upon the larval/pupal/adult characters, these could be broadly divided into the following types:

Adultoids
Topical administration of seed and root extracts of W. somnifera to prepupae of S. litura resulted into formation of adultoids. Depending upon degree of abnormalities, these have been classified into the following types-1. Adultoids with coiled and bifurcated proboscis; crumpled wings; parts of middle and posterior abdomen on dorsal surface devoid of scales (Plate 1 t, u). 2. Adultoid with less scales on crumpled wings, dorsal thorax, and abdomen; proboscis bifurcated; right prothoracic leg reduced as compared to left prothoracic leg (Plate 1v, w). 3. Adultoid pupal exuviae not shed off, covering the head and thorax; abdomen covered with usual scales but genitalia not developed (Plate 1x). 4. Adultoid with pupal exuviae attached to ventral surface of head and thorax; a few scales present on the dorsal surface of anterior and middle abdomen (Plate 1y). 5. Adultoid with crumpled wings and deformed body unable to eclose from pupal exuviae (Plate 1z). In some cases, pupal exuviae remained attached to abdomen (Plate 1aa) or right wing (Plate 1bb). In some cases, adultoids unable to eclose from the pupal cuticle and the larval cuticle was also found attached to the posterior extremity of the body (Plate 1 cc).
Treatment of prepupae of P. ricini with seed and root extracts of W. somnifera also resulted into formation of adultoids. Adultoid with white, untanned, bifurcated proboscis, and right wing unable to eclose from pupal exuviae was produced (Plate 2hh). In some cases, adultoid with coiled, bifurcated proboscis, and crumpled wings (Plate 2ii) or adultoid devoid of scales in the region of head and thorax and a few scars of scales found on the anterior and middle abdomen also developed (2jj). In some adultoids, the right wing (Plate 2kk) or left wing were reduced (Plate 2ll).

Discussion
Topical administration of seed extracts of W. somnifera to prepupae of S. litura and P. ricini was more severe as it alone caused toxicity in a dose-dependent manner as compared to root extracts where no toxicity was observed. This is comparable with the similar findings in P. ricini where treatment with seed extracts produced toxic effects but not with the root extracts of W. somnifera (Gaur & Kumar, 2017b). These toxicological effects may be due to the presence of certain bioactive compounds such as withanolide-WS-2 (aliphatic ester), withanolide-WS-1 (aliphatic ketone) in the seeds of W. somnifera (Dar et al., 2015). Such kind of toxic effect has also been observed as a result of treatment of developmental stages of other lepidopterans with extracts of W. somnifera, for instance, treatment of sixth instar larvae of S. litura with leaves extracts (Gaur & Kumar, 2010) and root extracts (Gaur & Kumar, 2017a).
The prepupal and pupal-adult ecdysis duration were significantly prolonged as a consequence of administration of seed and root extracts of W. somnifera to prepupae of both the lepidopterans viz. S. litura and P. ricini. The treatment with seed extracts has not only been found to be more effective in the prolongation of pupal-adult ecdysis in both the insects viz. S. litura and P. ricini but also resulting into the prolongation of prepupal period in S. litura, whereas the administration of root extracts only caused the prolongation of prepupal period in P. ricini. The crude volatile oil from the leaves of Piper betle has also been reported to cause prolongation of larval and pupal durations in the lepidopteran insect, S. litura (Srinivasan et al., 2016). In several cases, the plant extracts or their active bio ingredients have been observed to prolong larval and pupal duration when administered to different larval instars of lepidopteran insects. This has been observed as a result of administration of azadirachtin, salannin, deacetylgedunin, gedunin, 17-hydroxyazadiradion, and deacetylnimbin (limonoids) from Azadirachta indica to first to fifth instar larvae of Cnaphalocrocis medinalis (Lepidoptera: Crambidae) (Nathan, Kalaivani, Sehoon, & Murugan, 2006); leaves, root, fruit extracts of Pedalium murex to fourth instar larvae of S. litura (Sahayaraj & Sathyamoorthi, 2010); ononitol monohydrate isolated from leaves extracts of Cassia tora to third instar larvae of Helicoverpa armigera (Lepidoptera: Noctuidae), and S. litura . Such type of prolongation of developmental period was similar to that produced by the administration of juvenile hormone analogue (JHA), pyriproxyfen, to different larval instars of lepidopteran insects viz. fifth instar larvae of Choristoneura rosaceana (Lepidoptera: Tortricidae) (Sial & Brunner, 2010), second instar larvae of S. littoralis (Nasr, Badawy, & Rabea, 2010), and third instar larvae of Plutella xylostella (Lepidoptera: Plutellidae) (Alizadeh et al., 2012). In addition to that, administration of botanical extracts/natural products causing prolongation of developmental stages in other insects have also been described such as seed extracts of A. indica and leaves extracts of Citrullus colocynthis in Schistocerca gregaria (Orthoptera: Acrididae) (Nassar, Ghazawy, Torkey, & Rawy, 2018); rotenone from the roots of Lanochocrapus species or Derris species and limonine from citrus fruit peels in the vector of Bancroftian filariasis, Culex (Cx.) pipiens pallens (Bakr, Nassar, El-Barky, Abdeldayem, & Kotb, 2018). This kind of prolongation of prepupal and pupal duration is obviously due to inhibition/interference with the molting process, caused by an increase in the juvenile hormone (JH) titer in the insect body (Hangartner & Masner, 1973;Lapcharoen et al., 2005). There are two JH sensitive periods found in the last instar larvae of holometabolous insects. During these periods, the presence of JH is not required so that the cells of a developmental stage become committed to a new developmental fate (Nijhout, 1998). If the JH is present during these sensitive periods, the current developmental state or status quo will be maintained (Nijhout, 1998) and the switch to next developmental stage will not take place (Riddiford, Hiruma, Zhou, & Nelson, 2003). This clearly demonstrates that the plant extracts from the medicinal plant, Ashwagandha, W. somnifera mimic the action of JH producing similar effects as with the exogenous administration of JHAs as the presence of JHAs during sensitive/critical period may lead to inhibition of ecdysone production or alteration of ecdysteroid titer in the insect body (Alizadeh et al., 2012;Ghasemi, Sendi, & Ghadamyari, 2010;Suzuki, Sakurai, & Iwami, 2010).
Another prominent and conspicuous effect of administration of seed and root extracts of W. somnifera to prepupae of S. litura and P. ricini is the inhibition of ecdysis/molting eventually leading to death of the treated insects. The insects suffering from ecdysial stasis were unable to cast off old larval cuticle that was found all over the body resulting into complete ecdysial stasis or remained attached to different parts of the pupal body showing partial ecdysial stasis. These effects have also been observed as a result of administration of IGRs (lufenuron and diflubenzuron) to fifth instar larvae of H. armigera (Butter, Singh, & Dhawan, 2003;Unsal, Ozparlak, & Aktumsek, 2004) and JHAs (diofenolan and pyriproxyfen) to last instar larvae of Papilio demoleus (Lepidoptera: Papilionidae) and S. litura (Singh & Kumar, 2011a, 2011b, 2015a. In the last larval stadium of holometabolous insects, the JH titer is high during the initial phase of final stadium but subsequently it declines to undetectable levels. In the absence of JH, the prothoracicotropic hormone (PTTH) is released from the neurosecretory cells and that induces the synthesis of ecdysteroids from prothoracic glands to initiate metamorphosis (Bollenbacher, Smith, Goodman, & Gilbert, 1981;Gilbert, Iatrou, & Gill, 2005;Rountree & Bollenbacher, 1986). The ecdysial failure induced by W. somnifera extracts in both the insects viz. S. litura and P. ricini is similar to that induced by JHAs/IGRs and obviously due to hormonal imbalance as the exogenous administration of JHA, hydroprene, to rice weevil, Sitophilus oryzae (Coleoptera: Curculionidae) results into ecdysial failure because of the interference with the release of brain hormones (PTTH) (Gupta & Mkhize, 1983). It has been suggested that the administration of phytochemicals like azadirachtin from A. indica and goniothalamin from leaves of Goniothalamus species caused molting inhibition due to interference with the endocrine system by disrupting the synthesis and release of ecdysteroids or due to modification and suppression of the ecdysteroids titer (Nathan, Choi, Paik, & Kalaivani, 2008;Sieber & Rembold, 1983). The phytochemicals such as azadirachtin and podophyllotoxin can interfere with the neuroendocrine system by blocking directly the release of morphogenetic peptides (PTTH) (Mordue (Luntz & Nisbet, 2000;Garcia & Azambuja, 2004). Therefore, plant extracts from W. somnifera are similar in action to IGRs as both act by interfering with the neuroendocrine control.
The formation of larval-pupal and pupal-adult intermediates as a consequence of treatment with seed and root extracts of W. somnifera to prepupae of S. litura and P. ricini is similar to those produced as a result of treatment of noctuid larvae with other plant extracts or their active bio ingredients such as leaves, root, fruit extracts of P. murex in S. litura (Sahayaraj & Sathyamoorthi, 2010); seed extracts of Ceasalpinea bonduc in S. litura (Baskar, Maheswaran, & Ignacimuthu, 2012); triterpenoid friedelin isolated from leaves of Azima tetracantha in H. armigera and S. litura (Baskar, Duraipandiyan, & Ignacimuthu, 2014); and pogostone, an active ingredient of patchouli oil isolated from leaves of Pogostemon cablin in Spodoptera exigua (Huang et al., 2014). Surprisingly, administration of JHAs has also been observed to produce such intermediates in several lepidopteran insects, as observed in the present study or treatment with different IGRs. For instance, ethyl 11-chloro-3,7,11-trimethyldodec-2-trans-enoate application caused the development of larval-pupal and pupal-adult intermediates in Tortrix viridana (Lepidoptera: Tortricidae) (Novak & Sehnal, 1973); methoprene caused formation of pupal-adult intermediates in S. littoralis (Kocak & Kilincer, 1997); pyriproxyfen and diofenolan caused production of larval-pupal intermediates in S. litura (Singh & Kumar, 2015a). The formation of intermediates/chimeras having larval, pupal, and adult characteristics as a result of administration of seed and root extracts of W. somnifera to P. ricini have also been observed with IGR (Gaur & Kumar, 2017b) and JHAs like diofenolan and pyriproxyfen (Singh & Kumar, 2011a, 2011b. It has been suggested that the phytochemicals/secondary metabolites of plants act as JH mimics (Bede & Tobe, 2000) and are responsible for interference with the normal hormonal coordination of the metabolic processes of the developing stages (Sakthivadivel & Thilagavathy, 2003). Moreover, it has been found that the administration of fruit extracts of Melia azedarach significantly increased JH titer in the hemolymph as compared to that of controls in treated larvae of S. littoralis and this high JH titer is responsible for insufficient development of pupal characters leading to the formation of larval-pupal intermediates (Schmidt, Rembold, Ahmed, & Breuer, 1998). Infact, appropriate titres of JH and ecdysone during larval-pupal ecdysis in the insect determine the commitment of metamorphosis of larva into pupa (Doane, 1973;Nijhout, 1998). Infact, the presence or absence of JH during metamorphosis determines the course of development. The presence of JH during at an inappropriate time during the molting process prevents cellular differentiation and in the absence of JH, morphogenesis and maturation occurs and the development proceeds towards the adult stage (Bowers, 1971). Therefore, any exogenous application of JH/JHAs/IGRs or plant extracts that mimic the JH action prevents the maturation and leads to the formation of nonviable intermediates. The larval-pupal intermediates thus formed remain as such or in a state of status quo when JH titer remains high (Metwally & Sehnal, 1973).
Administration of seed and root extracts of W. somnifera also resulted into a significant reduction in pupation and adult emergence in both the insects viz. S. litura and P. ricini. The effect was observed in a dose-dependent manner in case of treatment with seed extracts of W. somnifera. These effects are similar to those observed by the treatment of larvae of Spodoptera spp. with various plant extracts such as Commiphora molmol (Family: Burseraceae), Pedalium murex (Family: Pedaliaceae), Condalia microphylla (Family: Rhamnaceae), and Calceolaria talcana (Family: Calceolariaceae) Munoz, Lamilla, Marin, Alarcon, & Cespedes, 2013;Sahayaraj & Sathyamoorthi, 2010;Shonouda, Farrag, & Salama, 2000). Moreover, it is interesting to note that such effects have also been observed as a result of treatment of lepidopteran larvae with JHAs, pyriproxyfen and diofenolan (Oouchi, 2005;Singh & Kumar, 2015a). This clearly demonstrates that the plant extracts mimic the action of JH in this respect and pupation is inhibited/suppressed due to high JH titer (Eto, 1990;Kotaki, Nakakita, & Kuwahara, 1993), whereas during the normal course of development JH is virtually absent in the pupae (Tunaz & Uygun, 2004). Similarly, JHA, diofenolan, has also been reported to reduce pupation and completely blocking adult emergence and this inhibitory effect on adult emergence is possibly due to suppression/interference with the release of eclosion hormone (Ghoneim, Bream, Tanani, & Nassar, 2007). Thus the effect produced by seed and root extracts of W. somnifera is comparable with a phytochemical, azadirachtin, which has been reported to block the synthesis/release of eclosion hormone (Rembold, Sharma, Czoppelt, & Schmutterer, 1982).
In present study, some of the adultoids were unable to eclose properly from pupal exuviae or pupal exuviae remained attached to different parts of the body. This kind of detrimental effect on adult eclosion has also been observed as a consequence of treatment with plant extracts or their active ingredients (Lapcharoen et al., 2005;Nenaah, 2011;Soonwera & Phasomkusolsil, 2016;Sreelatha, Hymavathi, Rao, Devanand, & Rani, 2010). The plant extracts mimic the action of JHAs as exogenous administration of JHAs exert inhibitory effect on the neuropeptide, eclosion hormone, produced by the ventral tritocerebral neurosecretory cell which leads to inhibition of adult eclosion (Singh & Kumar, 2015a, 2015b.

Conclusion
Seed and root extracts from the medicinal herb, W. somnifera caused disruption of molting and metamorphosis and this may be due to interference with the neuroendocrine mechanism in the polyphagous pests, S. litura and P. ricini. These results show that extracts of W. somnifera mimic the action of JH/JHAs and that can be judicially employed for the control of polyphagous insects under field conditions along with other bio-rational approaches of insect pest management.