The effect of raphé nuclei lesions on striatal tyramine concentration and dopamine turnover in the rat

This is an investigation of the effects of electrolytic lesions (1 mA, 10s, anodal) on the median and dorsal raphé nuclei of Wistar rats on the striatal concentrations ofp-tyrosine,p-tyramine,m-tyramine, DA, DOPAC, and HVA. The extent of the lesions was estimated in terms of the depletion of 5-hydroxytryptamine and 5-hydroxyindole acetic acid as well as histological examination of the lesioned area. The results show that the raphé nuclei lesions increased rat striatal levels of DOPAC and HVA while levels of DA were unaffected, an effect that was observed within the first day after the lesions were made. The increases in DOPAC and HVA were accompanied by a reduction in striatalp-tyramine and an increase inm-tyramine. The results further support the existence of a reciprocal relationship betweenp-andm-tyramine concentration and dopamine metabolism. Previous experiments have demonstrated depletion ofp-TA following nigral lesions. The present results are, therefore, important in relation to tyramine distribution in brain. Thep-andm-tyramine concentrations were not reduced at 7 days after the raphé nuclei lesions indicating that if the striatal tyramine-containing neurons exist, they do not originate in or pass through the dorsal or median raphé nuclei.     

The Effect of Some Precursor Amino Acids and Enzyme Inhibitors on the Mouse Striatal Concentration of Tyramines and Homovanillic Acid

Abstract: The parenteral administration of L-phenylalanine or p -tyrosine increases the mouse striatal concentration of p -tyramine, an effect that is enhanced by monoamine oxidase inhibition and reduced by an L-aromatic aminoacid decarboxylase inhibitor. Striatal m -tyramine was increased following administration of L-phenylalanine or m -tyrosine and enhanced further by monoamine oxidase inhibition. It was also observed that m -tyrosine is a better substrate for decarboxylation than p -tyrosine, and that p -tyrosine decarboxylation was blocked by NSD 1055, while that of m -tyrosine was enhanced. The results obtained indicate that both isomers of tyramine are formed in the mouse striatum by hydroxylation of L-phenylalanine to p - or m -tyrosine followed by decarboxylation by a specific decarboxylase; an alternative pathway could be first the decarboxylation of phenylalanine to β-phenylethylamine, followed by its hydroxylation to p - or m -tyramine.     

Analysis of biogenic amines in plasma of hypertensive patients and a control group

Procedures were developed for the determination of 17 circulating amines using gas chromatography-negative ion chemical ionisation mass spectrometry. The amines were quantified against their appropriate deuterated isotopomers. The mean concentrations and ranges of catecholamines and trace amines were high compared with previous studies. In comparison with nonhypertensives, plasma from hypertensives had higher concentrations of the following amines: noradrenaline (t=4.0%); normetanephrine (t=6.1%) and metanephrine (t=1.9%). There were no significant differences between 5HT levels in plasma from hypertensives and controls. The following trace amine could be detected in variable amounts in plasma:p-tyramine,m-tyramine,p-octopamine,m-octopamine,p-synephrine,m-synephrine, and salsolinol. The trace amines melatonin,N-acetyl 5HT, tryptamine, 6-hydroxymelatonin and 5-methoxytryptamine could not be detected in plasma with limits of detection lying in the range 20–100 pg ml^–1.     

Simultaneous extraction and separation of trace amines of biological interest

A method is described for the simultaneous extraction and separation of the trace amines 2-phenylethylamine, m-tyramine, p-tyramine, p-octopamine, normetanephrine, and 3-methoxytyramine. The method involves acetylation in aqueous solution, specific hydrolysis of phenolic acetate groups, derivatization with trifluoroacetic anhydride and analysis on a gas chromatograph equipped with an electron-capture detector. Analyses utilizing both packed glass columns and glass capillary columns are described.The method possesses the potential for quantitative as well as qualitative analysis, with one or more of the following amines employed as internal standards: benzylamine, 3-phenylpropylamine, tranylcypromine, and 2-(4-chlorophenyl)ethylamine.     

Effects of Aging on p- and m-Octopamine, Catecholamines, and Their Metabolizing Enzymes in the Rat

Abstract: Functions of octopamine in the mammalian brain are still not well known. An important aspect of this problem is the relationship between octopamines and catecholamines. Previous data have shown that their respective ontogenic evolutions are not parallel. Do the changes in brain related to aging also differentially affect these two groups of molecules? In order to check this point, the brain levels of p- and m-octopamine, p-tyramine, noradrenaline, and dopamine, as well as the activities of metabolizing enzymes, were determined in young adult and aging rats (20–26 months). Unlike catecholamines, there is a drastic decrease of p-octopa-mine after 20 months of age in the hypothalamus and telencephalon. p-Tyramine levels are also lowered. This change appears to be due to a decrease of the aromatic L-amino acid decarboxylase activity. These data, as those of ontogenic studies, confirm that p-octopamine and catecholamine metabolisms may have some independent steps and, moreover, that p-octopamine may have a role in the normal activity of the brain.     

The analysis of biogenic amines in the thoracic nervous system of the locust,Schistocerca gregaria,by gas-chromatography negative ion chemical ionization mass spectrometry (GC-NICIMS)

Biogenic amines in single ventral thoracic nerve cords of the locust, Schistocerca gregaria, have been identified and quantified by an extraction-derivatization procedure involving their reaction with ditrifluoromethylbenzoyl chloride (DTFMB) in the aqueous phase followed by extraction into an organic solvent, hydrolysis of phenolic esters and conversion of free hydroxyl groups to trimethylsilyl ethers. Subsequent analysis of these DTFMB-TMS derivatives by GC-NICIMS revealed that the molecular ion carried most (> 60%) of the ion current which made the method highly specific and gave a limit of detection below the picogram level. This publication establishes unequivocally that the principal amines in locust ventral thoracic nerve cord are p-tyramine, p-octopamine, dopamine and noradrenaline. 5-Hydroxytryptamine was determined using a previously published GC-NICIMS technique (Markey et al., Biomed. Mass Spectromet. 7, 301–304, 1981).     

Life Cycle of the Mulberry Longicorn Beetle,Apriona germari Hope on an Artificial Diet

Mulberry longicorn beetle, Apriona germari, was reared on an artificial diet to investigate its life cycle. Average egg period was 17.95 days. Most larvae pupated at the 8th (33.3%) or 9th (33.3%) instars, but others emerged from the 7th to the 11th instars. The total duration of larval stage from the 1st to the end of the 9th and the 11th instars were 176.2 and 251.5 days, respectively. For terminatiopn of diapause and acceleration of pupation, low temperature treatment at 5°C for 60 days was highly effective. Average pupal period for female and male was 19.3 and 18.4 days, respectively. Average longevity of adults was similar with 40.5 days for female and 44.3 days for male. Mating had occurred from about 10 days after the adult emergence, and then a female adult laid one or two eggs per day. Average number of eggs oviposited by a female was approximately 47.7. Total life span of A. germari, when reared on an artificial diet in the laboratory, ranged broadly from 197.5 days to 331.5 days mainly depending on the larval period.     

MASS FRAGMENTOGRAPHY OF PHENYLETHYLAMINE, m- AND p-TYRAMINE AND RELATED AMINES IN PLASMA, CEREBROSPINAL FLUID, URINE, AND BRAIN

—A mass fragmentographic method for the assay of phenylethylamine (PEA) and a number of related amines in several biological materials is described. The gas chromatographic column employed for this analysis is a 12ft 1/8 in. o.d. steel column packed with 0.5% OV₂₂+ 2% SE54 + 1% OV₂₁₀ coated on 80/100 mesh chromosorb W (HP). The mass spectral characteristics of these amines are illustrated, compared, and discussed. Of the various monoamines which could be measured, only PEA, m- and p-tyramine were detected in measurable quantities. Phenylethanolamine and p-octopamine were found in trace amounts in urine, plasma, cerebrosponal fluid, and rat brain. No diurnal variation in the urinary excretion of PEA, m- and p-tyramine was observed. Plasma concentration of PEA or p-tyramine did not significantly change 1 h after eating a breakfast. Furthermore, consuming 200 g of Cadbury milk chocolate containing about 1 mg of PEA, 0.1 mg of phenylethanolamine and 10 mg of p-tyramine did not significantly alter urine excretions of these three amines. In the brain, as has been reported by others, we found that PEA and p-tyramine are not evenly distributed and that the highest concentrations are found in the hypothalamus and caudate. From the results obtained we concluded that PEA, m- and p-tyramine are probably produced from endogenous sources and that the direct contribution of diet to their urine excretion is small.     

The effect of various amino acids and drugs on thepara-andmeta-hydroxyphenylacetic acid concentrations in the mouse caudate nucleus

Injection ofl-p-tyrosine (800 mg/kg, 2 h) increased the mouse striatalpara-hydroxyphenylacetic acid (p-HPAA) concentrations. A smaller dose ofd,l-m-tyrosine (20 mg/kg, 2h) produced a larger increase in mouse striatalmeta-hydroxyphenylacetic acid (m-HPAA) concentrations. The administration ofl-phenylalanine to mice caused a slight increase in thep-HPAA concentrations in the corpus striatum after 2h while a larger dose ofl-phenylalanine (800 mg/kg) produced a greater increase. Eight hours followingl-phenylalanine injection,p-HPAA concentrations were still elevated. Withd-phenylalanine a significant increase was observed at eight hours after drug administration.Two drugs which reduce dopamine synthesis, -methyl-para-tyrosine and apomorphine, decreasedm-HPAA striatal concentrations without affectingp-HPAA concentrations. From these results, it is proposed that tyrosine hydroxylase activity determinesp-HPAA concentrations by regulatingp-tyrosine availability. This enzyme may also synthesizem-tyrosine which is subsequently decarboxylated to formm-tyramine and then oxidatively deaminated to formm-HPAA.     

Determination and significance of l-tyrosine O-sulphate and its deaminated metabolites in normal human and mouse urine

Methods were developed for the determination of the O-sulphate esters of l-tyrosine, p-hydroxyphenylpyruvate, p-hydroxyphenylacetate and p-hydroxybenzaldehyde in human urine. The amounts of these esters normally present in human female urine were determined. The quantities and specific radioactivities of l-tyrosine O-sulphate and p-hydroxyphenylpyruvate O-sulphate in mouse urine after labelled tyrosine had been fed were determined and were consistent with the hypothesis that the sole source of p-hydroxyphenylpyruvate O-sulphate was l-tyrosine O-sulphate. It is suggested that the turnover of known polypeptides containing l-tyrosine O-sulphate residues can account for only a portion of the quantities of the ester and its metabolite(s) that are present in normal female human urine.     

Effects of nutritional stress on brain tyramine concentration and dopamine turnover

This is an investigation of the effect of nutritional stress at various ages on the levels of thep- andm-isomers of tyramine in the caudate nucleus of the rat. For comparison, the effects of nutritional stress on the concentration and turnover of dopamine were also studied. Nutritional stress induced in pre-weaning (3 weeks of age) or post-weaning (up to 9 weeks of age) rats resulted in a decrease in the concentration ofp-tyramine and an increase in the concentration ofm-tyramine in the caudate nucleus. Dopamine concentration or turnover in the caudate nucleus was not affected by pre-weaning undernutrition; in the olfactory tubercles, however, a significant decrease was observed in dopamine turnover, calculated from the decrease in homovanillic acid levels after monoamine oxidase inhibition. The results suggest the changes observed are dependent on the availability of the amino acid precursorsp- andm-tyrosine and their competition towards aromatic-l-amino acid decarboxylase.     

Application of Multi-vitamins as Supplementary Nutrients on Biological and Economical Characteristics of Silkworm Bombyx mori L

In order to investigate the effects of supplementary nutrients on silkworm, Bombyx mori, an experiment was conducted with multi-vitamins treatments. Leaves enriched with multi-vitamins (1, 2.5 and 5%) were fed once a day to 4th and 5th instar silkworm larva. The supplementation of the leaves was done by spraying the treatments on them. These treatments resulted in a significant increase in biological and economical parameters such as larval weight, female and male cocoon weight, pupal weight and egg productivity when compared with normal control. Multi-vitamins of 2.5% treatment increased the larval weight by 10.2%, which had the most weight enhancement in the fifth day of 5th instar larvae. However, 5% concentration of multi-vitamins decreased some biological characteristics. These treatments resulted in 4.7% increase of cocoon's weight. In most of the moths the number and weight of eggs had significant difference compared to control, but these supplementary materials caused relatively less egg hatching.     

Dual enzyme-activated irreversible inhibition of monoamine oxidase

(E)-β-Fluoromethylene-m-tyrosine and related amino acids were synthesized from acetophenone derivatives and shown to be dual enzyme-activated inhibitors of monoamine oxidase. These substances are decarboxylated by hog kidney aromatic l-amino acid decarboxylase liberating (E)-β-fluoromethylene-m-tyramine derivatives which, in turn, are enzyme-activated inhibitors of rat brain mitochondrial monoamine oxidase.     

m-OCTOPAMINE, p-OCTOPAMINE AND PHENYLETHANOLAMINE IN RAT BRAIN: A SENSITIVE, SPECIFIC ASSAY AND THE EFFECTS OF SOME DRUGS

Abstract— An enzyme radiochemical assay for p -octopamine, m -octopamine (norphenylephrine) and phenylethanolamine based on the N -methylation of these amines by the enzyme phenylethanolamine N -methyl transferase ( S -adenosyl- l -methionine: phenylethanolamine N -methyl transferase (EC 2.1.1.28) has been developed. [³H]Methyl- S -adenosyl- l -methionine was used as methyl donor. The reaction products are converted to their dansyl derivatives and separated by TLC in three different solvent systems prior to liquid scintillation counting. The method exhibits a sensitivity of less than 10 pg for each amine and is suitable for the measurement of endogenous p -octopamine levels in mammalian brain. The highest levels of p -octopamine were found in the hypothalamus (3.4 ng/g) but despite the sensitivity of the assay, neither phenylethanolamine nor m -octopamine could be detected. After MAO inhibition, however, both of these amines were found to be present. p -Octopamine was increased substantially in all brain regions following the administration of an MAO inhibitor, whereas pretreatment with reserpine produced a significant decrease in the hypothalamus.     

N-β-alanyldopamine and N-acetyldopamine occurrence and synthesis in the central nervous system of Manduca sexta (L.)

N-β-Alanyldopamine (NBAD), N-acetyldopamine (NADA), dopamine (DA), and 3,4-dihydroxyphenylalanine (DOPA) were detected in the brain and ganglia of the central nervous system of larval and adult tobacco hornworms, Manduca sexta, by reversed phase HPLC with electrochemical detection. NBAD predominated in larval neural tissue during development of the fifth instar and increased to peak concentrations of 936, 650 and 263 nmol g⁻¹ in the abdominal ganglia, subesophageal plus thoracic ganglia and brain, respectively, at the wandering stage of development. Concentrations of all catecholamines decreased in the pharate pupa and were generally lowest in the adult nerve cord. DA was the second most abundant catecholamine in larval ganglia, but the primary catecholamine in adult ganglia. Relatively high levels of DOPA also occurred in the ganglia of wandering larvae but not at other times. NADA was detected only in the abdominal ganglia of day 3 larvae. N-Acyltransferases that catalyze synthesis of NBAD and NADA from DA also were present in abdominal ganglia, as demonstrated by analysis of in vitro cultures in which exogenous DA stimulated synthesis of both N-acylated catecholamines. Maximal NBAD synthesis occurred in ganglia removed from wandering stage larvae (9.3 nmol g⁻¹ day⁻¹), whereas NADA synthesis was highest in ganglia from pharate pupae (7.3 nmol g⁻¹ day⁻¹). Thus, N-β-alanylation and N-acetylation are competing metabolic reactions for DA in the hornworm's nervous system. The role played by the N-acylated catecholamines in M. sexta neurophysiology is unknown, but these compounds may be storage or inactive forms of the putative neurotransmitter DA.     

Partial purification and properties of an enzyme from rat liver that catalyses the sulphation of l-tyrosyl derivatives

1. An enzyme that catalyses the transfer of sulphate from adenosine 3′-phosphate 5′[³⁵S]-sulphatophosphate to l-tyrosine methyl ester and tyramine was purified approx. 70-fold from female rat livers. 2. The partially purified preparation is still contaminated with adenosine 3′-phosphate 5′-sulphatophosphate–phenol sulphotransferase (EC 2.8.2.1), but a partial separation of the two enzymes can be achieved by chromatography on columns of Sephadex G-200 and DEAE-Sephadex. 3. The enzyme responsible for the sulphation of l-tyrosine methyl ester and tyramine is activated by dithiothreitol, 2-mercaptoethanol and GSH, the degree of activation being more marked with preparations previously stored at 0 or −10°C. In contrast, the enzymic sulphation of p-nitrophenol is inhibited by all three thiols. Again, there is a quantitative difference in the degree of inhibition of the two enzymes by o-iodosobenzoate, p-chloromercuribenzoate, N-ethylmaleimide and iodoacetate. 4. Mixed-substrate experiments support the hypothesis that the enzyme responsible for the sulphation of l-tyrosine methyl ester and tyramine is separate from that responsible for the sulphation of p-nitrophenol. However, p-nitrophenol is a potent inhibitor of the sulphation of both tyrosyl derivatives whereas these latter compounds have no effect on the sulphation of p-nitrophenol.     

Microspectrofluorimetric identification of m-hydroxyphenylethylamines (m-tyramines) in central and peripheral monoamine neurons

Summary Catecholamines and m-tyramine derivatives form strongly fluorescent products on formaldehyde gas treatment according to the method of Falck and Hillarp with maximal emission at 480 and 420 m. respectively. Administration of the m-tyramine compounds m-tyrosine, -methyl-m-tyrosine and 4, -dimethyl-m-tyramine caused a depletion of the green fluorescence (max. 480 m) in both central and peripheral catecholamine neurons with a concomitant appearance of a blue fluorescence (max. 420 m) due to uptake and accumulation of the administered m-tyramine derivatives. Injection of metaraminol gave the same results in sympathetic adrenergic neurons while of the central catecholamine neurons only the dopamine nerves in the median eminence were depleted and showed uptake and accumulalation of metaraminol.Abbreviations used NA noradrenaline - DA dopamine - -MMT -methyl-m-tyrosine - 5-HT 5-hydroxytryptamine     

The Effect of Mesencephalic Lesions on Tyramine and Dopamine in the Caudate Nucleus of the Rat

Abstract: The dopamine (DA)-containing nerve terminals in the caudate nucleus arise from cell bodies located in the substantia nigra (pars compacta), and it is possible that p-tyramine- and m-tyramine-containing neurons may also exist in this nucleus. We have studied the effects of unilateral electrolytic lesions of the pars compacta in rat on levels of DA, p-tyramine, m-tyramine, and homovanillic acid in the caudate nucleus after various survival times. At 12 and 24 h following lesioning the ipsilateral level of p-tyramine was significantly reduced compared with the contralateral side, whereas the concentrations of m-tyramine, DA, and homovanillic acid were significantly increased. Thus, in the short term, the lesion results in an increase in DA turnover, which is accompanied by an increase in m-tyramine levels and a decrease in p-tyramine levels. Similar changes occur following pharmacological treatments (chlorpromazine, d-amphetamine, l-DOPA) that increase DA turnover. At survival times of 2, 11, and 25 days, the ipsilateral concentrations of m-tyramine, DA, and homovanillic acid were reduced along with p-tyramine. These longer-term alterations in amine levels are most likely a consequence of degeneration of nigro-striatal axons. Placement of a lesion 1 mm dorsal to the usual position centering on the pars compacta produced different biochemical changes from those seen after the pars compacta lesion. One day following this lesion the concentration of p-tyramine was slightly reduced; DA was unaffected, but the concentration of m-tyramine was profoundly increased, even more so than after the pars compacta lesion. This could indicate the existence of specific m-tyramine-containing cell bodies located dorsal to the substantia nigra. The results suggest that p- and m-tyramine in the caudate nucleus originate from neurons in or close to the substantia nigra. The results in the short term following the lesion support the observation that there is an inverse relationship between p-tyramine concentration and DA turnover in the caudate nucleus.     

A non-destructive method for identifying the sex of ant larvae

The differences between adult male and female ants are often striking and obvious, yet both sexes appear virtually identical at the larval stage. Current methods for determining larval sex rely on genetic analyses or histology, both of which require killing all larvae examined. Here, we describe a method for identifying larval sex in vivo based on visible differences in genital imaginal discs. Using a light microscope, clear differences in genital disc morphology were observed between male and female larvae of the ponerine ant Harpegnathos saltator. Next, we investigated whether this technique could be broadly applied within ants and found similar differences in genital discs between male and female larvae of Aphaenogaster cockerelli and Camponotus floridanus. Taken together, our results show that genital discs can be used as a reliable indicator of larval sex in species from at least three major ant subfamilies. This technique should facilitate research into topics where information about larval sex is required.     

Simultaneous determination of molting and juvenile hormone titers of the greater wax moth

A simple and rapid extraction procedure was developed to determine simultaneously the molting hormone (MH) and juvenile hormone (JH) activity in a single insect tissue sample. From the onset of the last larval stage to adult eclosion of the greater wax moth, Galleria mellonella, three JH peaks were noted: at the time of the sixth larval ecdysis, 1 day before the seventh larval ecdysis, and at the time of adult eclosion. Three MH peaks were recorded for the male: at 1 day before the sixth larval ecdysis, 1 day before the seventh larval ecdysis, and 2 days after pupation. In the female, a fourth peak was shown at the time of adult eclosion. This fourth peak exhibits the highest molting hormone activity of all samples, 1600 Musca units/g of fresh tissue or an equivalent of 5.6 μg/g of ecdysterone. Eighty per cent of this MH accumulated in the ovary. The significance of MH and JH titers as related to the endocrine regulation of development is discussed in the light of this finding.