Basic requirements

Spatial and temporal control of heterologous gene expression is an area of considerable and growing interest with relevance to basic and applied biological and medical research, including gene therapy and functional genomics. However, these heterologous regulatory systems should interfere minimally with the complex endogenous regulatory networks. Ideally, heterologous modification of gene expression in host cells should give rapid, robust, precise and reversible induction (or suppression) of the target gene(s). The necessary criteria are thus (Saez et al., 1997; Bohl and Heard, 1998; DeMayo and Tsai, 2001; Fussenegger, 2001; Graham, 2002):

Ecdysteroid receptors in arthropods

Ecdysteroid receptors are members of the nuclear receptor superfamily (Laudet, 1997), which are characterised by a domain structure. The N-terminal A/B-domain is highly variable and is associated with transcriptional activation. The C-domain is highly conserved and is involved in binding the receptor complex to specific response elements in the DNA. The D-domain is variable and represents a hinge region between the DNA-binding domain and the ligand-binding domain (E-domain). The E-domain is not only responsible for ligand binding, but also has been implicated in receptor dimerisation and interactions with other transcriptional activators. There may also be a C-terminal F-domain, which, if present, is highly variable between even closely related nuclear receptors (Kumar and Thompson, 1999). Nuclear receptors regulate gene expression as dimers, either as homodimers or as heterodimers with another member of the nuclear receptor superfamily. One of the most promiscuous heterodimeric partners for vertebrate nuclear receptors is RXR, of which the equivalent in insects is Ultraspiracle (USP; Oro et al., 1990). In the case of ecdysteroid receptors, only the EcR:USP (or EcR:RXR) (Yao et al., 1993) complex is able to bind the ecdysteroid ligand with high affinity and the presence of ecdysteroid promotes complex formation. The ecdysteroid binds to the EcR protein. No definitive ligand for USP has been identified, but it has been suggested that juvenile hormones (or methyl farnesoate in Crustacea) may bind to this receptor component and modify the transactivation capacity of the complex (Jones and Jones, 2000).

The most extensively studied ecdysteroid receptor system in arthropods is that of Drosophila melanogaster, where three isoforms (A, B1 and B2) of EcR occur (Koelle et al., 1991; Talbot et al., 1993). These isoforms arise through alternative promoter usage and differential splicing, resulting in different A/B-domains, but they all possess common DNA- and ligand-binding domains. The EcR isoforms show tissue- and stage-specificity. Although there is only one form of USP in D. melanogaster, two or more isoforms have been found in other arthropods. USP isoforms also show tissue- and stage-specificity (Kapitskaya et al., 1996).

EcR and USP gene homologues have now been characterised from a variety of arthropod species: Aedes aegypti (Cho et al., 1995; Kapitskaya et al., 1996), Amblyomma americana (Palmer et al., 1999), Bombyx mori (Swevers et al., 1996), Ceratitis capitata (Verras et al., 1999), Chironomus tentans (Imhof et al., 1993; Vögtli et al., 1999), Choristoneura fumiferana (Kothapalli et al., 1995; Perera et al., 1999), Heliothis virescens (Martinez et al., 1999c), Locusta migratoria (Saleh et al., 1998; Hayward et al., 1999), Lucilia cuprina (Hannan and Hill, 1997; 2001), Manduca sexta (Fujiwara et al., 1995; Jindra et al., 1997), Ostrinia nubilalis (Albertsen et al., 2000), Sarcophaga crassipalpis (Rinehart et al., 2001), Tenebrio molitor (Mouillet et al., 1997; Nicolai et al., 2000), Uca pugilator (Durica et al., 2002).

The biochemical characterisation of ecdysteroid receptor complexes lags well behind that of vertebrate steroid hormone receptors and has been in a period of quiescence for the past decade, as emphasis has been placed on the characterisation and expression of the genes. The generally accepted ligand for ecdysteroid receptors in arthropods is 20E, but this does not preclude the other ecdysteroids being significant at particular stages of development or in certain tissues (Wang et al., 2000). In fact, ecdysteroid receptor complexes recognise a wide range of ecdysteroid structural analogues and sophisticated structure-activity and molecular modelling studies are now beginning to be performed (Dinan et al., 1999a; Wurtz et al., 2000; Ravi et al., 2001; Kumar et al., 2002). Owing to the importance of ecdysteroid receptors in the regulation of arthropod development, they are seen as an appropriate target for the development of new pest control agents. In the context of this review, the identification of bisacylhydrazines as non-steroidal ecdysteroid agonists (Wing, 1988; Dhadialla et al., 1998) is particularly worth mentioning as, in addition to several of these molecules being commercialised as insecticides, other analogues appear appropriate as gene switching elicitors. Antagonists for ecdysteroid receptors are also being identified (Dinan et al., 1999b).

Ecdysteroid-responsive expression systems

Ecdysteroid systems vs. other systems

Fussenegger (2001) provides a comprehensive description of the heterologous molecular switching systems currently under consideration. Each has its own advantages, but none fulfils all the desirable criteria perfectly. From the time of early studies, transgenic ecdysteroid-inducible gene expression systems in mammalian cells have appeared to possess lower basal activity and higher inducibility than tetracycline-based systems (No et al., 1996). Senner et al. (2001) compared 3 inducer systems (tetracycline, dimerizer and ecdysteroid) in one system (rat C6 glioma cells) under identical conditions. Each system required transient transfection with two plasmids (a regulator plasmid and a reporter plasmid) and treatment with an elicitor (inducers for the ecdysteroid and dimerizer systems and a repressor for the tetracycline system). The ecdysteroid system provided the highest induced activity, but the authors conclude that each of the systems may be beneficial, depending on what the experimental goals are. Van Craenenbroeck et al. (2001) compared the tetracycline and ecdysteroid systems to regulate the expression of neurotransmitter receptors in mouse fibrosarcoma L929sA and HEK293 cells. The tetracycline system resulted in higher levels of the neurotransmitter receptors being expressed, but the ecdysteroid system gave more tightly regulated expression. Moreover, this study underlined the importance of the genetic background of the cells being used.

Morgan et al. (1999) compare several exogenously regulatable promoter systems for their suitability for the study of the functions of genes implicated in aging.

Ecdysteroid specificity

Gene expression systems in mammalian and plants cells possess markedly different ecdysteroid specificities to ecdysteroid receptors in insect systems. Both the affinity and specificity seem to be affected. Thus, the generally accepted endogenous hormone in insects, 20E, is inactive in transgenic systems. Two phytoecdysteroids, murA and ponA, are normally used to activate the transgenic systems, but even these are required at least 100-fold higher concentrations than in insect systems; e.g. EC₅₀ values for murA and ponA in the Drosophila melanogaster B_II bioassay are 2.2 × 10⁻⁸M and 3.1 × 10⁻¹⁰M, respectively (Dinan et al., 1999a), while concentrations of 1 – 10 µM are required to induce transgenic expression. The basis of this altered affinity/specificity is not clear and it could derive from: (i) altered metabolism, (ii) use of RXR, rather than USP, (iii) altered transportation into cells, (iv) fusion of the EcR ligand-binding domain to the GR DNA-binding domain and/or VP16 to form VgEcR, (v) the different properties of mammalian transcription factors, enhancers, repressors etc.

A limited investigation of the ecdysteroid specificity of VgEcR/RXR in CV-1 cells has been performed (Saez et al., 2000). MurA, ponA and 14-deoxymuristerone A were almost equivalently active (EC₅₀ = ca. 5 × 10⁻⁷M), with ponasterone C being moderately active (EC₅₀ = 2 × 10⁻⁵M), polB being weakly active and 20E, inokosterone, makisterone A, E, 2-deoxyecdysone, 20E 22-acetate and 2-deoxy-20-hydroxyecdysone being inactive or only very weakly active at 10⁻⁴M. This study also showed that the presence of a natural (9-cis-retinoic acid) or synthetic (LG268 or LG1069) RXR ligands, while inactive in itself, potentiated the activity of ponA by 3- to 5-fold.

Availability of ligands

Registration problems

Development of ecdysteroid systems for human therapeutic use may be hampered by the steroidal nature of ecdysteroids and the insecticidal origin of BAHs, which may prejudice their use as elicitors, this being in spite of the fact that both ecdysteroids and BAHs have low mammalian toxicities and ecdysteroids are a normal (but small) component of the human diet. For plant systems, ecdysteroids per se cannot be considered because of penetration problems and BAHs may not be acceptable because of the enhanced risk of development of resistance to insecticidal analogues. However, use might be restricted to specified crops under conditions where exposure to sensitive insect species is minimal.

Biochemical problems

Although the systems developed to date are effective for use in in vitro expression systems, the requirements for an effective in vivo system are much more stringent. In this context, one can identify the following aspects of ecdysteroid-regulatable systems which would need to be improved in order to generate a medically viable system:

Prospects

There is little doubt that ecdysteroid-regulated transgenic systems have considerable potential for in vitro work. The applied potential is somewhat more questionable at present, owing to the following current limitations: i) genetic complexity, ii) altered affinity and selectivity of VgEcR for ligands and iii) potential problems in the registration of ecdysteroids and BAHs for human therapeutic uses or with plant transgenic systems. However, significant progress is being made in designing chimaeric receptors which would allow only one trans-acting factor to be transfected. It is only a matter of time until the reasons for the altered affinity and selectivity of ecdysteroid receptors in mammalian and plant cells are elucidated and more efficient systems are developed either by identifying more effective ligands or site-directed mutagenesis of EcR to enhance affinity for currently used ligands. Although ecdysteroids and BAHs are nontoxic to humans, general public resistance to steroids and insecticides may hamper their registration.

Ecdysteroids are rapidly eliminated

In the case of humans, two different studies have been performed. Simon and Koolman (1989) analysed the pharmacokinetics of E and 20E (given orally, 0.2 mg/kg b.w.) to a male volunteer, by monitoring with a radioimmunoassay the subsequent plasma and urine titres. This gave an effective half-time (EHT) of elimination of 4 hours for E and 9 hours for 20E. In lambs, EHT for 20E was shown to depend strongly on the mode of administration, with values of 0.4, 0.2 and 2 hours after oral, intravenous and intramuscular administration, respectively (Simon and Koolman, 1989). The method used did not allow the detection of metabolites, if present. The half-life seems shorter in smaller mammals, with reported values of 8.15 min for 20E in mice (Dzukharova et al., 1987). More recently, Albanese et al. (2000) found a plasma half-life of 48 min for ponA in mice after intra-peritoneal injection of 750 µg of this compound.

Both urinary and faecal routes seem to be used for the elimination of the administered molecules. In mice, the faecal route was found to be the major one by Hikino et al. (1972a&b) and Lafont et al. (1988), although Dzukharova et al. (1987) found that faecal and urinary routes were equally important. Such a question can be easily assessed only by the use of radiolabelled molecules, but no data are available for humans. Kinetic studies in mice showed that ecdysteroids were taken up by the liver and then excreted into the gut via the bile (Hikino et al.,1972a&b; Lafont et al., 1988).

Metabolic conversions

Another question concerns whether ecdysteroids undergo metabolic conversions in mammals. The presently available data are not fully consistent. In mice, Girault et al. (1988) analysed the faecal metabolites of injected E and isolated unchanged E, a major metabolite identified by MS and proton NMR as 14-deoxyecdysone together with molecules with a fully reduced B-ring and, additionally, epimerized in position 3 (Figure 6A). Such a metabolism is reminiscent of the hepatic reduction of the 4-en-3-one on ring-A of vertebrate steroid hormones, whereas dehydroxylation resembles that of bile acids and could result from the actions of anaerobic intestinal bacteria.

More recent studies were performed on ingested 20E in rats (Ramazanov et al., 1996) and humans (Tsitsimpikou et al., 2001). In these cases only urine was analyzed. Ramazanov et al. administered 20E to 40 rats (50 mg/kg) directly in stomach with a special probe, and they collected urine (3.5 L) over the following 10 days. After several chromatographic steps, they isolated unchanged 20E and three new metabolites, which were analyzed by IR and mass spectrometry. The IR spectra showed the disappearance of the signal at 650 cm ⁻¹ (7-en-6-one) and the structures were deduced from MS data (Figure 6B).

Tsitsimpikou et al. (2001) analysed the urine of a volunteer having ingested 20 mg of “Ecdysten™” (a commercial preparation containing 20E – see section 6); they collected urine over 5 days and analysed ecdysteroids by GC-MS after derivatization. They found, together with 20E, two less hydroxylated metabolites, which they tentatively identified as 2d20E and 2dE by comparison with available reference molecules.

Mass spectrometry does not provide sufficient information, and only NMR can allow an unambiguous determination of structures. Anyway, it seems reasonable to assume that modification of the B-ring and dehydroxylation are general features of ecdysteroid metabolism in mammals.

Conclusions/prospects

There is rapid catabolism/elimination of ecdysteroids, which means that large amounts would have to be used in order to maintain circulating levels above the concentration required for gene switches systems to be activated. Alternatively, slow-delivery systems like subcutaneous implants represent another way to maintain sustained ecdysteroid levels for several days (Albanese et al., 2000). Another remaining question concerns the metabolism in peripheral tissues. As we have seen with mice, the observed conversions are most probably performed by hepatocytes and intestinal bacteria. It would be of interest to determine whether other mammalian tissues are able to metabolise ecdysteroids, and the nature of the reactions they can perform.

Whether side-chain cleavage between C-20 and C-22 (and possibly also between C-17 and C-20) can take place is a very important question which remains to be investigated by using ecdysteroids labelled on the steroid nucleus, as labelling on the side-chain would be lost if such a reaction would occur. This question seems particularly important for several reasons: (1) cleavage between C-20 and C-22 would result in the formation of 21C steroids that would share some resemblance with vertebrate neurosteroids (Lafont and Sláma, 1995), and (2) in some pharmacological studies rubrosterone (2β,3β,14α-trihydroxy-5β-androst-7-ene-6,17-dione) was as active as 20E (Otaka et al., 1968).

Ecdysteroids and growth (Table 2)

The anabolic effects of several phytoecdysteroids (20E, cyasterone, turkesterone, viticosterone E – see structures on Ecdybase) on mice or rats were reported long ago (see e.g. Okui et al., 1968; Syrov and Kurmukov, 1975a&b; 1976a–c, Syrov et al., 1978, 1981a; Stopka et al., 1999). Growth-promoting effects have also been more recently reported for pigs (Kratky et al., 1997) and Japanese quails (Koudela et al., 1995; Sláma et al., 1996). In many instances however, these effects are not spectacular when considering the growth (weight) curves as they are observed during certain phases of growth or for one sex only and, in many cases, adequate statistical analyses are lacking. Nevertheless, even small effects (i.e. <5 % increase) on growth could be of economical interest for nutritionists, but their firm establishment requires the use of large numbers of animals, which is hardly feasible with large mammals. The addition of E to sheep food increases body growth rate and also wool growth (Purser and Baker, 1994). Surprisingly, these effects were obtained with minute amounts of ecdysone (0.02 µg/kg per day!), and were more evident when animals were fed on a poor quality diet, which indicates that E improves food utilization. In this case, it has been suggested that the effect results from the toxicity of E towards rumen protozoa, but this has not been fully established. In fact, through a stimulation of protein synthesis (and/or a reduction of protein catabolism), ecdysteroids would increase the lean body mass. In pigs, doses of 0.2–0.4 mg/kg/day resulted in better nitrogen retention and a body weight increase of 112–116% relative to controls, while food consumption was lowered by 11–17% (Kratky et al., 1997). Other experiments used diets supplemented with ecdysteroid-containing plants (e.g. Rhaponticum carthamoides) and reported similar growth-promoting effects on pigs over a 30-day period (Selepcova et al., 1993b). In quails, 20E in the diet promoted increased growth (115% of controls), but this was associated with a decreased index of food conversion (Sláma et al., 1996). From these data, it appears difficult to draw general conclusions.

Ecdysteroids and physical performance

20E is claimed to have tonic properties (Abubakirov et al., 1988). Indeed it stimulates muscle growth, provided that protein supply is adequate. Such anabolic effects result in increased physical performance without training (Chermnykh et al., 1988). This was for instance demonstrated using the forced swimming test with rats: animals given ecdysteroids for one week were able to swim for significantly longer times (Azizov and Seifulla, 1998). These effects are similar to those of anabolic steroids. 20E is also able to increase muscle ATP content in vitamin D-deprived rats (Kholodova et al., 1997).

Ecdysteroids: effects on cellular proliferation and differentiation

Wound-healing effects of ecdysteroids have been described (Syrov and Khushbatkova, 1996; Darmograi et al., 1998). 20E (applied at 0.1% w/w in liposomes) shortens the duration of skin repair after superficial wounding and 20E (2 × 10⁻⁴M) stimulates keratinocyte differentiation in vitro (Detmar et al., 1994), an effect measured by the increase of the activity of transglutaminase (an enzyme involved in protein connection through isopeptidic bond formation). Accordingly, ecdysteroids show psoriasis-inhibiting effects (Inaoka et al. 1997). These results have led to many patents concerning the use of ecdysteroids in cosmetics (Lin and Lin, 1989; Meybeck and Bonté, 1990, 1993; Meybeck et al., 1994; Tsuji et al., 1995a&b; Darmograi et al. 1998; Meybeck 1999a&b). In this context, the incorporation of 20E or its acyl ester (2,3,22-tripalmitate) into liposomes has been tested as a slow-release form (Politova et al., 2001).

20E administered orally to rats (5 mg/kg) accelerates the healing process after an experimental bone fracture (Syrov et al., 1986a), and the same molecule (10–100 ng/ml) can stimulate the in vitro proliferation of rat osteosarcoma UMR106 cells (osteoblasts) by 41% (Gao and Wang, 2000). Similarly, 20E stimulates proliferation of human umbilical vein endothelial cells (Lin et al., 1997; Wu et al., 1998b), and several phytoecdysteroids can stimulate erythropoiesis in rats (Syrov et al., 1997b).

The effects of ecdysteroids on tumorous cell proliferation are somewhat conflicting: Lagova and Valueva (1981) reported that 20E (0.1–300 mg/kg, subcutaneous injections for 5 days) was mainly ineffective on tumour growth in mice, but it stimulated the growth of mammary gland carcinomas in mice and rats. El-Mofti (1987, 1994) reported that E was able to induce neoplastic lesions in toads and mice; other authors reported inhibitory effects on tumor cell proliferation (Hirono et al., 1969; Burdette, 1974; Shibatani et al., 1996). More recently, Konovalova et al. (2002) showed that injected 20E had a synergistic effect with low doses of an antitumour drug (cis-platin). Most probably, the results may differ according with the cell types, the nature and concentration of ecdysteroids used, and this clearly requires more extensive studies. In addition, genoprotective effects of ecdysteroids have been reported (Gubskii et al., 1993; Levitskii et al., 1993a&b, 1996; Chabanny et al., 1994); ecdysteroids can prevent chromatin damages induced by various chemicals.

Ecdysteroids and protein synthesis

Stimulatory effects of ecdysone on protein synthesis were reported as early as 1963 (Burdette and Coda, 1963), and the discovery of phytoecdysteroids made these molecules available in large amounts for pharmacological assays. It was rapidly shown that ecdysteroids were able to stimulate protein synthesis in mouse liver (Okui et al., 1968; Otaka et al., 1968, 1969a&b). In fact, it was shown that 20E stimulates the incorporation of [¹⁴C]leucine in a cell-free translation system (rat liver polysomes), i.e. it increases the efficiency of the translational machinery (Syrov et al., 1978). Such conclusions have been confirmed and extended to other tissues, especially heart and muscles (Syrov et al., 1975a; Aizikov et al., 1978; Khimiko et al., 2000). Recent structure-activity studies (Syrov et al., 2001) as measured by a stimulation of [¹⁴C] aminoacid incorporation into proteins showed that among the compounds tested turkesterone was the most active, followed by cyasterone and 20E.

Ecdysteroids and glucose metabolism

It was shown early on (Table 3) that 20E given per os to rats reduces hyperglycaemia induced either by glucagon or by alloxan treatment (Matsuda et al., 1970; Uchiyama and Ogawa, 1970; Yoshida et al., 1971, Uchiyama and Yoshida, 1974). In fact, 20E stimulates the incorporation of glucose into glycogen and protein in mouse liver (Yoshida et al., 1971) and more generally it enhances glucose utilization by tissues (Syrov et al., 1997a). The mechanism involved seems to be an increase of tissue sensitivity to insulin (Kosovsky et al., 1989) and preparations containing phytoecdysteroids have been proposed as oral antidiabetics (Takahashi and Nishimoto, 1992; Yang et al., 2001). Depending on the extent of hyperglycaemia, phytoecdysteroid effects may be more or less pronounced that those of manilil, a widely used pharmacological molecule (Kutepova et al., 2001).

Ecdysteroids and lipid metabolism

Ecdysteroids display hypocholesterolaemic effects (Lupien et al., 1969; Mironova et al., 1982; Syrov et al., 1983), through a reduction of cholesterol biosynthesis and an increase of its catabolism (Uchiyama and Yoshida, 1974). 20E (5 mg/kg per os) stimulates the conversion of cholesterol into bile acids in rats (Syrov et al., 1986b), and such an effect is reminiscent of some oxysterols (Schroepfer, 2000). In connection with these effects, ecdysteroids may also have antiatherosclerotic actions (Matsuda et al., 1974; Syrov et al., 1983). Intraperitoneally injected 20E (0.5 mg/kg in rats) also enhances [¹⁴C]acetate incorporation into liver triglycerides and reduces triglyceride lipase activity (Catalán et al., 1985).

Ecdysteroids: a “universal medicine“?

An impressive number of papers dealing with ecdysteroid effects are available in the literature. They concern almost every physiological function, and we will give below a brief insight of the published data. It must be noted, however, that in many instances that, in addition to the difficulties caused by language barriers, the experiments are not always described with all the desirable details.

Ecdysteroids improve nervous function: in early studies, it was shown that 20E induced glutamic decarboxylase (an enzyme involved in GABA biosynthesis) in rat brain (Chaudhary et al., 1969), and that E was able to induce acetylcholinesterase in rat brain too (Catalán et al., 1984). More recently, ecdysteroids were shown to represent neuron-protective agents; they reduce glutamate-induced cell death in cortex neurons of rat foetuses and they are proposed as a therapy against mental and behavioural disorders (Aikake et al., 1996). In addition, they may protect against amnesia induced by diazepam or alcohol (Xu et al., 1999). Similar neuroprotective effects have been described for progesterone and oestradiol mixtures in animal models of neurodegeneration (Vongher and Frye, 1999).

Ecdysteroids stimulate hepatic functions: 20E accelerates recovery after hepatitis induced by heliotrine treatment (Syrov et al., 1981b). 20E and other ecdysteroids (turkesterone, cyasterone) administered (10 mg/kg) to rats with hepatitis induced by subcutaneous injection of carbon tetrachloride prevent its hepatotoxic action (Syrov et al., 1992). Moreover, a pretreatment with 20E (5 mg/kg) for one week will reduce the effects of a subsequent heliotrine treatment (Badal'yants et al., 1996).

Ecdysteroids improve heart and lung function: 20E has been recommended for the prevention of myocardial ischaemia, arrhythmia and is described as enhancing VEGF expression (Wu, 2001). An antiarrhythmic effect of 20E was also reported by Kurmukov and Yermishina (1991) and Yang et al. (1996), and an extract of Leuzea carthamoides containing high amounts of 20E also showed a similar effect (Maimeskulova and Malslov, 2000). In rabbits experimentally rendered atherosclerotic (by a high cholesterol diet), 20E (10 mg/kg/day per os) given for 28 days was able to increase Na⁺/K⁺ ATPase in myocardium (Khushbaktova et al., 1987). Intravenous injection of 20E showed also a therapeutic effect after lung contusion (Wu et al., 1997, 1998a).

Ecdysteroids improve renal function: when rats are given a nephrotoxic mixture (uranyl acetate + glycerol), 20E (5 mg/kg) seems thereafter able to restore a normal glomerular filtration rate and to suppress albuminuria (Saatov et al., 1999; Syrov and Khushbaktova, 2001).

Ecdysteroids and the immune system: various immunomodulatory effects of ecdysteroids have been described. Single intraperitoneal injections of various ecdysteroids (20E, 2dE, 2d20E, polB, turkesterone, 1–5 mg/kg) increase the concentration of antibody-forming cells in the spleen of mice immunised with sheep red blood cells (Sakhibov et al., 1989). Low (7.5×10⁻¹²–7.5×10⁻⁸ M) concentrations of 20E induce the activation (E-rosette formation test) of human lymphocytes (Trenin et al., 1996; Trenin and Volodin, 1999). Low to moderate (10⁻¹²–10⁻⁵ M) concentrations of 20E or other ecdysteroids stimulate, whereas higher (10⁻⁴M) concentrations eventually inhibit, DNA synthesis in concanavalin A – activated lymphocytes (Kuzmitsky et al., 1990; Fomovska et al., 1992; Chiang et al., 1992).

20E (10–20 mg/kg/day per os) has antiinflammatory properties similar to cortisone acetate in rats and mice (Kurmukov and Syrov, 1988; Fomovska et al., 1992) and turkesterone improves lung defence mechanisms in diabetic rats (Najmutdinova and Saatov, 1999). 20E was shown to inhibit in a dose-dependent fashion (10⁻⁹–10⁻⁴ M) histamine release from rat peritoneal mast cells induced by anti-IgE or concanavailin A (Takei et al., 1991). Taniguchi et al. (1997), however, could not observe any antiinflammatory effect of 20E given orally to rats (5 mg/kg/day for 7 days).

Ecdysteroids have antioxidant properties: 20E has antioxidative and anti-free radical properties (Osynska et al., 1992) and it can thus reduce lipid peroxidation (Kuzmenko et al., 1997, 2001). Several models were used in these studies, as the chemiluminescence of blood serum induced by H₂O₂ using rats receiving a vitamin D-deficient diet eventually supplemented with 0.1 mg 20E/kg per day, or the uptake of oxygen by methyl linoleate micelles in the presence or absence of 20E.

Are ecdysteroids toxic to microorganisms?: there are a few reports about antimicrobial activity of ecdysteroids. However, Ahmad et al. (1996) reported antifungal and antibacterial activity of 20E at rather high concentrations (between 100 and 400 µg/ml, i.e. 2–8 × 10⁻⁴ M). An antimicrobial activity of 20E and its acetates was also observed by Volodin et al. (1999). Toxic effects on protozoa have also been reported; rabbits receiving 20E per os (5 mg/g/day for 3 months) showed a reduced infection with Lamblia duodenalis (Syrov et al., 1990), and the improvement of ruminant productivity by ecdysone was also interpreted by its toxicity towards rumen protozoa (Purser and Baker, 1994).

Ecdysteroids are not toxic to vertebrates: ecdysteroids have a very low toxicity (LD50 > 6g/kg), they are not hypertensive and, in spite of their anabolic action, they would have neither androgenic nor oestrogenic (or antioestrogenic) effects; they induce no virilisation and they do not induce significant changes in castrated animals (e.g. Prabhu and Nayar, 1974). All together this suggests that ecdysteroids are attractive compounds for a wide array of uses, which have been proposed, and of course it would be of particular interest to understand more precisely their mode(s) of action in mammals.

Do ecdysteroids have genomic effects on vertebrates?

In insects, ecdysteroids have well-known genomic effects which involve nuclear receptors (see Section 2). When considering the molecules in 3-dimensions, it is clear that they show striking differences to vertebrate sex or adrenal steroids, and their full cholesterol side-chain most probably prevents any binding to the receptors of these vertebrate hormones. Recently, however, it has been found that some previously “orphan” nuclear receptors (e.g. LXR, PXR) bind endogenously produced oxysterols (Janowski et al., 1999 ; Schroepffer, 2000) or have a broad specificity and may bind a wide array of xenobiotics including several steroids (Jones et al., 2000). Given this broad ligand specificity, these proteins might rather function as “endocrine sensors” rather than “true receptors” (Evans, 2002). So, until ecdysteroids are directly tested for binding to such receptors, it remains conceivable that they may have transcriptional effects through binding to some nuclear receptor(s); indeed early studies showed a rapid in vivo stimulation by 20E of the incorporation of [¹⁴C]orotic acid into RNA in mouse liver (Uchiyama and Otaka, 1974).

Ecdysteroids: membrane effects?

Membrane effects of steroids are nowadays well documented and they may proceed through three different pathways (Figure 7). According to Brann et al. (1995), these effects may either involve: (1) the dissolution of ecdysteroids in the membrane bilayer and a change in the environment of some membrane proteins (and hence of their activity), (2) their interaction with a specific membrane receptor, which will activate some transduction mechanism, or (3) their binding to a modulatory site of the receptor for another molecule. These different effects are not mutually exclusive. Very recently, a membrane progestin receptor involved in fish oocyte meiotic reinitiation was cloned and its physiological relevance was fully established (Zhu et al., 2003).

Some recent data

Recently, Constantino et al. (2001) fortuitously made a crucial observation. Using the Invitrogen^® ecdysteroid-inducible expression system to analyse the transduction mechanisms of interleukin-3 (IL-3) in a pro-B lymphocyte cell line, they found in control experiments that murA and ponA were able to potentiate the IL-3-dependent activation of PI 3-kinase/Akt pathway in non-transformed cells.

Given the central role of the Akt/PKB pathway in mammalian cell metabolism (e.g. Brazil and Hemmings, 2001; Whiteman et al., 2002), such results provide an interesting basis for explaining in a single way many effects of ecdysteroids on mammals, as concerns their hypoglycaemic, antiapoptotic and anabolic actions (Figure 8). The available data do not allow to decide whether edysteroids act on the IL-3 receptor itself or on a downstream step.