Multicomponent alarm pheromones in the mandibular glands of major workers of the African weaver ant, Oecophylla longinoda

ABSTRACT. The complex system of alarm communication in Oecophylla longinoda is described. The mandibular gland secretion of major workers releases in other major workers a complex pattern of behaviour, which includes components of alerting, attraction and biting. The main constituents of the secretion are hexanal and 1-hexanol, which release alerting and attraction respectively. Of the thirty or so trace components, at least two, 2-butyl-2-octenal and 3-undecanone, act as markers for attack. In combination, these components produce a sequential message in space and time, dependent on their relative proportions, volatilities and threshold concentrations for behavioural reponses.     

Volatile components from the mandibular glands of the turtle ants, Cephalotes alfaroi and Cephalotes cristatus

GC–MS analysis of whole head extracts from the turtle ants, Cephalotes alfaroi and Cephalotes cristatus, showed that 4-heptanone and 4-heptanol were the major volatile components in the mandibular glands. 4-Heptanone and 4-heptanol have rarely been identified in mandibular gland secretions from other ant genera. Thus, these compounds may be chemotaxonomic markers for the genus Cephalotes, since they have been identified in the mandibular glands from all members of this genus that have been investigated to date. Minor components identified in the whole head extracts of these ants were 3-methyl-1-butanol, 3-heptanone, 3-hexanol, 2- and 3-methylbutanoic acids, 2-methyl-4-heptanone, 2-phenylethanol and phenol. To our knowledge, this is the first time that 2-methyl-4-heptanone and phenol have been reported in the mandibular gland secretion from any Formicid.     

A comparison of mandibular gland volatiles from ants of the bull horn acacia,Acacia collinsii

GC–MS analyses of dichloromethane extracts of the mandibular glands from three obligate symbiotic Psuedomyrmex ant species of Acacia collinsii from Costa Rica: Pseudomyrmex flavicornis (synonym Pseudomyrmex belti), Psuedomyrmex spinicola, and Psuedomyrmex nigrocincta, showed distinct differences in the 16 ketones, 15 alcohols, 2 aldehydes and 2 carboxylic acids that were identified. Different compounds were the major component from each species: P. flavicornis, 3-octanone; P. spinicola, 4-methyl-3-heptanone; and P. nigrocincta, 3-methyl-2-hexanol. The secretion of P. flavicornis contained 10 compounds not found in the other species, including the two terpene alcohols, citronellol and geraniol. The secretions of P. spinicola and P. nigrocincta had 12 compounds in common, that were not found in P. flavicornis' secretion. The similarity of the mandibular gland secretion of P. spinicola and P. nigrocincta may indicate that they are more closely related to each other than either is to P. flavicornis. The components from the mandibular gland of Crematogaster rochai, another ant associated with this acacia, are 2- and 3-methylbutanoic acid, 3-octanone, 3-octanol, 6-methyl-3-octanol and 3-nonanone.     

Comparative study of the mandibular gland secretion of four species of Myrmica ants

The mandibular glands of the two species of ant, Myrmica ruginodis and Myrmica sabuleti contain a similar mixture of compounds, but the proportions are different. M. sabuleti produces ethanol, propanone, methylpropanal, 3-hexanone, 3-hexanol, 3-heptanone, 3-heptanol, 3-octanone, 3-octanol, 6-methyl-3-octanone, 6-methyl-3-octanol and 3-decanone. With the exception of 3-decanone these compounds were also found in M. ruginodis. These compounds were also found in M. rubra and M. scabrinodis.In both species now studied, the mandibular gland contents attract the workers and cause a large increase in their linear speed. In M. sabuleti these behavioural activities are due to 3-octanone and 3-octanol: the attraction of these two compounds in a synthetic mixture is exactly like that of an isolated mandibular gland; the compounds act in synergy to cause an increase in the ants' linear speed. Workers of M. ruginodis specifically respond to a mixture of ethanol, 3-octanone and 3-octanol: the alcohol only moderates the ethological action of the ketone, which is a true attractant and causes a very large increase in the ants' velocity; ethanol also attracts workers, acting in this respect in synergy with 3-octanone.These chemical and behavioural results are combined with those previously reported (Cammaerts-Tricot, 1973; Morganet al., 1978) to explain the responses of M. rubra, M. ruginodis, M. sabuleti and M. scabrinodis workers to isolated mandibular glands from each of these four species.     

Melatonin Effects on Steroid Production by Rainbow Trout Ovarian Follicles In Vitro: Influence of Stage of Follicle Maturation

Rainbow trout ovarian follicles at four different stages of maturation (very early vitellogenesis, early vitellogenesis, peak vitellogenesis, and pre-ovulatory) were incubated either in Cortland's medium alone, or medium containing melatonin at one of five concentrations (1 × 10^-10, 1 × 10^-8, 1 × 10^-6, 1 × 10^-4 or 1 × 10^-2M) to assess the direct actions of melatonin on basal (non-gonadotrophin stimulated) secretion of 17β-estradiol and testosterone. Testosterone secretion by peak vitellogenic phase follicles was significantly (p < 0.01) reduced by melatonin at 1 × 10^-4 or 1 × 10^-2 M, but there were no other significant effects of melatonin on T secretion. There were no significant effects of melatonin at concentrations of 1 × 10^-10 or 1 × 10^-8 M on 17β-estradiol secretion for any stage of follicular maturation, although for follicles at the peak vitellogenesis stage, melatonin at 1 × 10^-6 M had a significant (p < 0.05) stimulatory effect compared with the controls. Melatonin also stimulated 17β-estradiol secretion by very early vitellogenic stage follicles (1 × 10^-2 M concentration; p < 0.05). At concentrations of 1 × 10^-4 and 1 × 10^-2 M, melatonin significantly (p < 0.01) inhibited 17β-estradiol secretion of peak vitellogenic and preovulatory stage follicles. The findings suggest a stimulatory action of melatonin on steroidogenesis of early stage ovarian follicles, a shift to an inhibitory action of the higher concentrations of melatonin in later stages of development, but with a bimodal action of melatonin (related to hormone concentration) being present during the time of maximum follicular growth.     

Microemulsion and micellar electrokinetic chromatography of steroids

A mixture of ten steroids was separated by microemulsion and micellar (SDS and glycodeoxyholate) electrokinetic chromatography systems. Separations were done on a 50 cm (to the detector) × 50 μm I.D. fused-silica capillary. Complete separation of all the test compounds in the micellar mode was obtained with glycodeoxycholate (50 mM) in 25 mM borate buffer, pH 6.5, as the micelle-forming agent. The best results, however, were obtained using microemulsion electrokinetic chromatography in which higher aliphatic alcohols were used as the microemulsion-forming modifiers. The system consisted of n-hexanol (0.81%), SDS (3.31%) and n-butanol (6.61%) in 20 mM phosphate buffer, pH 10.0 (89.28%, w/w). In the microemulsion mode, linear calibration for steroid standards was obtained in the concentration range 3 × 10⁻⁴ − 3 × 10⁻⁵ mol l⁻¹ with a detection limit of 1 pmol. The method was validated and applied to an 11β-hydroxysteroid dehydrogenase assay in tissues.     

Evaluation of the in vitro methods for micropropagation of Chondracanthus acicularis (Roth) Fredericq (Gigartinales, Rhodophyta): tissue culture and production of protoplasts

Tissue was cultured and protoplasts isolated from the carrageenophyte Chondracanthus acicularis with the aim of developing micropropagation as an alternative to harvesting raw material from natural beds. Both adventitious shoots and filamentous calluses were induced by tissue culture on medium solidified with 0.4–1 % (w/v) agar. Adventitious shoots were mainly produced from discoid bases while filamentous calluses were mainly induced from basal zones and sub-apical explants. A gradient of the regeneration ability was observed from the top to the bottom of the thallus. The discoid base was the most reactive explant and produced the highest number of adventitious shoots compared to basal zones and sub-apical explants, irrespective of the concentration of agar. Protoplasts were isolated enzymatically from the whole thallus using a combination of cellulase R-10 Onozuka, macerozyme R-10, and crude extract of the gland gut of algivorous molluscs. The highest mean yield of protoplasts (1.2?×?10⁶ protoplasts g^?1 fresh weight) was obtained after 16 h of digestion with an enzyme mixture containing 2 % (w/v) cellulase R-10, 1 % (w/v) macerozyme R-10 Onozuka, 4 % (v/v) crude extract of gut gland of Haliotis, 0.8 M mannitol, 50 mM sodium citrate, 0.3 % (w/v) bovine serum albumin. Depending on the conditions, mean protoplast yields ranged from 3.14?×?10⁵ to 1.2?×?10⁶ protoplasts g^?1 fresh weight. Different factors (storage duration, mannitol, sodium citrate, crude extract of the gland gut of algivorous molluscs) were tested to improve the yield of protoplasts but none has a significantly effect.     

Structure of sensilla, olfactory perception, and behaviour of the bedbug, Cimex lectularius, in response to its alarm pheromone

When deprived of the terminal antennal segments, male and female bedbugs failed to respond to their alarm pheromone and to their assembling scent. Trans-oct-2-en-1-al or trans-hex-2-en-1-al, being the major constituents of the former, induce in adults and larvae of Cimex lectularius a typical alarm behaviour resulting in dispersal of assembled bedbugs; the rapidity of escape depends on the aldehyde concentration in the air. The behavioural threshold for adults is about 9×10¹⁴ molecules of trans-oct-2-en-1-al or 6×10¹⁵ molecules of trans-hex-2-en-1-al per ml air.The distal part of the terminal antennal segment of C. lectularius reveals the following sensilla: bristles (type A1), immersed cones (type B1), plates (type B2), grooved pegs (type C), smooth pegs (type D), hairs with even (type E1), and uneven wall thickness (type E2). The number and distribution of these sensilla is relatively constant and similar in both sexes, but differs slightly in neonate larvae. The pegs and hairs of types C, D, E1 and E2 were shown to have porous walls, a prerequisite for olfactory function.Receptor potentials were recorded from olfactory sensilla of types E1 and E2 after stimulation with trans-hex-2-en-1-al and trans-oct-2-en-1-al. The minimal concentration of trans-hex-2-en-1-al evoking a receptor potential is about 2×10¹⁰ molecules per ml air. The above olfactory sensilla were found to respond also to hexan-1-al, but almost no responses to pentan-1-al, butan-1-al, trans-hex-2-ene, and trans-oct-2-ene were observed. A minimum chain length of six carbons atoms and a terminal carbonyl group are molecular prerequisites for optimal odorant activity, while the presence of a Δ²-double bond is not essential for stimulation of the alarm pheromone receptors of the bedbug.     

The effect of aging on prolactin secretion in rat pituitary monolayer culture.

A high basal rate of prolactin (PRL) secretion (.16±.03 μg/well/hr) was produced for over four weeks by pre-confluent male rat pituitary monolayer cell cultures. When the media was changed, a rapid release of microgram quantities of PRL occurred followed by a return to the basal PRL secretory rate by seven hours. Theophylline (3.8×10^?3M), but not dibutyrl cAMP (1×10^?3M), produced a significant (p<.02) increase in PRL secretion, and simultaneous addition of these agents potentiated the PRL secretory rate. TRH (2×10^?8M) had no effect on PRL release by six hours, whereas dopamine (4.9×10^?5M) produced a significant suppression (p<.002) of PRL secretion. In addition, the effects of theophylline, TRH, and dopamine on PRL secretion were similar in cultures of various ages. Ovine prolactin in concentrations up to 50 μg per ml produced no change in PRL secretion during 72 hours of incubation suggesting that PRL feedback control of its own secretion may be transmitted via the hypothalamus. These studies show that a high rate of PRL secretion can be maintained by pre-confluent monolayer cultures for extended periods of time, permitting repeated experimentation on the same wells.     

Synthesis of RNA in isolated polytene nuclei from salivary gland cells of Chironomus thummi

The incorporation of [³H]UTP into RNA by isolated polytene salivary gland nuclei of Chironomus thummi was investigated under different incubation conditions; the labeled RNA fractions were characterized by electrophoresis. The results suggested that at two characteristic ionic conditions most of the RNA synthesized was the product of RNA polymerase I or RNA polymerase II as distinguished by their differential sensitivities to α-amanitin. Electrophoretical analysis of the RNA synthesized under conditions favouring polymerase I showed that this RNA population consisted mainly of four distinct molecular weight fractions within a range between 2.8 × 10⁴ and 2.5 × 10⁶. Under conditions favouring polymerase II two fractions were detected: one with a broad molecular weight distribution around 0.4 × 10⁶ containing considerable amounts of poly(A)-bearing RNA molecules, and a second with a peak at a molecular weight of 2.8 × 10⁴.     

The secretory response in dissociated acini from the rat submandibular gland

Rat submandibular gland was dissociated by enzymatic digestion with collagenase and hyaluronidase, followed by mild mechanical shearing and filtration through a nylon mesh. The dissociated cell populations contained predominantly groups of acinar cells which maintained their acinar arrangement. The morphological and functional viability of the cells was confirmed by electron microscopic examination and a normal secretory response to β-adrenergic or cholinergic stimulation was observed. Both isoproterenol (IPR) and carbachol caused the fusion of secretory granules into large vacuoles which were also continuous with the lumen, and into which the secretory product was released. Secretion was assessed quantitatively from the incorporation of ¹⁴C-glucosamine into the acinar cells and its subsequent release into the culture medium as labelled glycoprotein. IPR stimulated secretion to 125% of untreated controls in the concentration range 5 × 10^?5 to 5 × 10^?7 M, and to 110% of controls at 5 × 10^?8 M, after 40 min incubation. Carbachol stimulated secretion to 131% of controls at 5 × 10^?5 M and to 115% at 5 × 10^?6 M but had no effect at 5 × 10^?7 or 5 × 10^?8 M. The secretory response was blocked by the respective β-adrenergic and cholinergic antagonists, propranolol and atropine. These findings show that dissociated rat submandibular acinar cells provide a useful in vitro model for the study of mucus synthesis and secretion.     

Migration and habitat use of the tropical eels Anguilla marmorata and A. bicolor pacifica in Vietnam

The patterns of use of marine and freshwater habitats by the tropical anguillid eels Anguilla marmorata and A. bicolor pacifica were examined by analysing the otolith strontium (Sr) and calcium (Ca) concentrations of yellow (immature) and silver (mature) stage eels collected in Vietnamese waters. In A. marmorata, the change in the Sr:Ca ratios outside the high Sr:Ca core was generally divided into three patterns: (1) typical catadromous life history pattern; (2) constant residence in brackish water; and (3) habitat shifting between sea and brackish waters with no freshwater life. In A. bicolor pacifica, no eels had a general life history as freshwater residents. The eels were also divided into three patterns: (1) constant residence in sea water; (2) constantly living in brackish water; and (3) habitat shifting from brackish to sea water with no freshwater residence. The mean Sr:Ca ratio value after recruitment to coastal waters ranged from 1.73 to 5.67 × 10^?3 (mean 3.2 × 10^?3) in A. marmorata and from 2.53 to 6.32 × 10^?3 (mean 4.3 × 10^?3) in A. bicolor pacifica. The wide range of otolith Sr:Ca ratios in both species indicated that the habitat use of these tropical eels was facultative among fresh, brackish, and marine waters during their growth phases after recruitment to coastal areas. Tropical eel species may have the same behavioural plasticity as temperate anguillid species regarding whether to enter freshwater or to remain in estuarine and marine environments.     

The DNA content of sperm and hemocyte nuclei of the silkworm,Bombyx mori L.

To estimate the size of the haploid genome of the silkworm, Bombyx mori (Lepidoptera), amounts of Feulgen-DNA staining in individual nuclei of primary spermatocytes, spermatids, maturing sperm, and larval or pupal hemocytes were determined with an integrating microdensitometer and compared with the Feulgen-DNA levels found for chicken erythrocyte nuclei, or the sperm and erythrocyte nuclei of Xenopus laevis that were included with each Bombyx preparation as empirical reference standards of 2.5, 3.15, and 6.3×10^?12 g DNA per cell, respectively. Under these conditions, the haploid male genome of B. mori was estimated as 0.52±0.01 (S.E.)×10^?12 g DNA, corresponding to a molecular weight of roughly 3.1×10¹¹ daltons. From similar measurements of Feulgen-stained hemocyte nuclei, approximately 1.0±0.05 (S.E.)×10^?12 g DNA was estimated for the diploid or 2C male genome of Bombyx. These values compare favorably with estimates of genome size based upon analysis of the kinetics of reassociation of DNA isolated from B. mori and provide an independent basis for assessing the degree of polyploidy achieved by the giant nuclei in the posterior silk gland prior to its secretion of fibroin at the end of the fifth larval instar.     

Detection of propeptides of AlpA and AlpB lytic endopeptidases from Lysobacter sp. XL1 by the sandwich enzyme immunoassay based on monoclonal antibodies

Extracellular lytic endopeptidases AlpA and AlpB of the Gram-negative bacterium Lysobacter sp. XL1 have a high degree of homology and are synthesized as preproproteins consisting of a signal peptide, a propeptide, and the mature protein. In the present work, two monoclonal antibodies against the AlpA propeptide (ProA) and eleven antibodies against the AlpB propeptide (ProB) have been obtained. The affinity constants for antibodies to ProA were 2.9 × 10⁹ and 3.5 × 10⁹ M^?1, and those for antibodies to ProB were from 1.5 × 10⁸ to 2.2 × 10⁹ M^?1. The antibodies showed no immune cross-reactivity with each other and with mature forms of the enzymes. On the basis of monoclonal antibodies, a sandwich enzyme immunoassay has been developed, which makes it possible to detect these propeptides in the dissolved native form. The linear range of the detection of ProA was 1.5–100.0 ng/mL with an error of measurement of 6%, and that of the determination of ProA was 0.2–6.25 ng/mL with an error of measurement of 6%. By using the assay, propeptides ProA and ProB were detected in cell lysates of Lysobacter sp. XL1 in an amount of 1.18 ± 0.03 and 0.096 ± 0.002 ng per 1 OD540 of bacterial culture, respectively. The immunochemical assay for the detection of different forms of AlpA and AlpB can be useful in solving the problems associated with their secretion into environment.     

Effects of papaverine on basal and on isoproterenol-stimulated renin secretion from rat kidney slices

Papaverine inhibited the basal renin secretion of rat kidney slices incubated in a physiological salt solution at 37°C. Inhibition was concentration-dependent; secretion was 99 ± 0.2 % inhibited by 5 × 10^?4 M papaverine, and 8 × 10^?5 M was the estimated ED₅₀. In contrast, 2 × 10^?4 M IBMx (3-isobutyl-1-methyl-xanthine) increased the rate of secretion from 215 ± 17 to 366 ± 30 ng hr^?1mg^?1/20 min (p < 0.001). Isoprotenol (4 × 10^?7, 8 × 10^?7, and 5 × 10^?6 M) stimulated renin secretion in a concentration-dependent manner; the stimulatory effects were antagonized by papaverine but unaffected by IBMx. Thus, two known inhibitors of phosphodiesterase--IBMx and papaverine--produce sharply contrasting effects on basal and on isoproterenol-stimulated renin secretion from rat kidney slices.     

A multicomponent mandibular gland secretion in the ponerine ant Bothroponera soror (Emery)

The ponerine and Bothroponera soror has a complex mandibular gland secretion in which certain individual components release different behavioural responses. 2-undecanone releases alerting and orientation, 2-undecanol attraction and methyl-6-methylsalicylate, stinging. Field observations indicate that this multicomponent pheromone system enables small groups of ants to immobilize larger prey items.     

Phéromones agrégeant les ouvrières de Myrmica rubra

The workers of Myrmica rubra aggregate around a source of one of their secretions, which can be called ‘alarm pheromone’, and also around workers of Lasius flavus. The mechanism of these aggregations differ.Both L. flavus workers and a solution in liquid paraffin of 3-octanol, one of the mandibular gland compounds, act as an arrestant for the workers of M. rubra. Both Dufour's gland secretion and a source of 3-octanone, the major compound of the mandibular gland secretion, are true attractants.The poison gland secretion, a mixture of 3-octanone and 3-octanol in liquid paraffin and a solution in liquid paraffin of 3-nonanone, a minor mandibular gland compound, all induce klinokinesis. The secretion of the mandibular glands and the secretion of the venom apparatus both cause positive klinokinesis and taxis. These locomotory reactions increase the probability that an object, marked by nest mates with these secretions, will be detected by several workers.When presented alone, 3-octanone is the only attractive compound in the mandibular gland secretion. However, a mixture of 3-octanone and 3-octanol (15 per cent of 3-octanol in the vapour phase) is detected more easily by the ants. The diffusion coefficients of the two compounds are different, and a mixture of these substances creates not only a quantitative but also a qualitative odour gradient. This may explain the synergy of the mixture.     

The antagonistic effect of dexamethasone and insulin on alpha-fetoprotein secretion by cultured H4-II-E-C3 cells derived from the Reuber H-35 hepatoma.

Non-confluent monolayers of H4-II-E-C3 cells were maintained in serum-free media. Dexamethasone alone (5 × 10^?7M) stimulated α-fetoprotein secretion 2- to 4-fold while insulin alone (8.7 × 10^?8M) inhibited α-fetoprotein secretion by 20%. When dexamethasone (5 × 10^?7 to 5 × 10^?9M) and insulin (8.7 × 10^?8 to 8.7 × 10^?11M) were added simultaneously, insulin diminished the stimulatory effect of dexamethasone. When α-fetoprotein secretion was elevated by dexamethasone and the medium was replaced by media containing either insulin or no hormones, the rate of α-fetoprotein secretion diminished more rapidly with the insulin-supplemented medium. Alone or in combination, insulin and dexamethasone had little effect on albumin secretion.