The accumulation of p-hydroxyamphetamine by brain homogenates and its role in the release of catecholamines

p-Hydroxyamphetamine (p-OHA) is accumulated by synaptosome enriched preparations from both striatal and cortical tissues. In studies with P₂ preparations from rat cortex the accumulation of $\text{p-}\text{OHA}\text{-[}{}^3\text{H}\text{]}$ was shown to be temperature dependent but different from the process involved in the accumulation of norepinephrine-[³H](NE[³H]) by this tissue. The uptake of p-OHA was less sensitive to DMI and cocaine and had a different time dependency. The accumulation of p-OHA was concentration dependent and did not show evidence for saturation at concentrations up to 10 μM, The relationship between p-OHA uptake and catecholamine release from the striatum and cortex was also examined. The results suggest that much of the observed cortical uptake of p-OHA is not due to the neuronal carrier for norepinephrine.     

Determination of extraction constant,true partition coefficient and formation constant of ion-pair complexes of quaternary ammonium salts,tetrabutylammonium bromide and isopropamide iodide.with some organic anions by a solvent extraction technique

A new method of determining the extraction constant (K_e, the true partition coefficient (TPC) and the formation constant (K_f) of ion-pairs, was developed by the solvent extraction technique. K_e and TPC were estimated from the reciprocals of the intercept and the slope of the regression line obtained by plotting

$\text{B}{}^{\mathrm{T}}{}_{\mathrm{W}}\text{APC ? dA}\text{vs}\text{B}\text{B}{}^{\mathrm{T}}{}_{\mathrm{W}}\text{dA}\text{APC ? dA}\text{+}\text{A}{}^{\mathrm{T}}{}_{\mathrm{W}}\text{+}\text{B}{}^{\mathrm{T}}{}_{\mathrm{W}}$

in the following equation.

$\text{B}{}^{\mathrm{T}}{}_{\mathrm{W}}\text{APC ? dA}\text{=}\text{1}\text{K}{}_{\mathrm{e}}\text{+}\text{B}\text{B}{}^{\mathrm{T}}{}_{\mathrm{W}}\text{dA}\text{APC ? dA}\text{+}\text{A}{}^{\mathrm{T}}{}_{\mathrm{W}}\text{+}\text{B}{}^{\mathrm{T}}{}_{\mathrm{W}}\text{x}\text{1}\text{TPC}$

where [A^T_W] and [B^T_W] are the total concentrations of the cationic compound A and that of the anionic compound B in the aqueous phase respectively, APC is the apparent partition coefficient of A, dA is the partition coefficient of cation A⁺. K_f, which is expressed by K_e/TPC, was then calculated. These constants were determined for the ion-pair extraction of tetrabutylammonium bromide and isopropamide iodide with 4 organic anions, i.e. benzoic acid, p-toluenesulfonic acid, salicylic acid and taurodeoxycholic acid. This new method might be applicable to other ion-pairs without further assumptions except that the molar ratio of the ion-pair formation be 1 : 1.     

Effects of exposure to ozone on susceptibility to experimental tuberculosis

Exposure of mice to 1.96 $\text{mg}\text{m}{}^3$ ozone (O₃) 3 $\text{h}\text{day}$, 5 days/week, for up to 8 weeks beginning at 1 or 2 weeks after challenge with Mycobacterium tuberculosis R 1Rv resulted in significant enhancement of bacterial titers in the lungs at 5 through 8 weeks after challenge when compared to mice exposed to filtered air. Exposure to lower concentrations of O₃ did not produce any significant changes compared to controls.Exposure of guinea pigs to 2.9 $\text{mg}\text{m}{}^3$ O₃ for 3 h immediately after challenge with M. tuberculosis resulted in a suppression of the cutaneous delayed hypersensitivity response, without affecting the serum hemagglutination antibody titers. However, exposure of guinea pigs to 0.98 $\text{mg}\text{m}{}^3$ O³ 3 $\text{h}\text{day}$ for 5 days, initiated within 3 h after the infectious challenge, enhanced hemagglutination antibody titers initially, but the delayed hypersensitivity reaction did not differ from controls.     

Carbon disulphide tetratogenicity and postnatal effects in rat

Pregnant albino rats were exposed to carbon disulphide vapour in concentrations of 50, 100 or 200 $\text{mg}\text{m}{}^3$throughout gestation. Two successive generations (F₁ and F₂) were studied.Concentration levels of 100 and 200 $\text{mg}\text{m}{}^3$ produced marked dose-related impairment in the prenatal development of the F₁ progeny, with increase of early embryonal lethality, reduction in foetal weight and a high incidence of malformations affecting mostly the brain and limbs. Postnatal viability, body weight, lipid and energy metabolism and behaviour were also impaired. Behavioral deviations were observed even at 50 $\text{mg}\text{m}{}^3$.After reaching sexual maturity the F₁ rats were mated within their experimental groups, but no further carbon disulphide exposure was applied. The adverse effects on progeny were still detectable in the F₂ generation. Structural abnormalities of the same type as those found in the F₁ at 100 and 200 $\text{mg}\text{m}{}^3$ exposure were observed in their progeny and, postnatally, statistically significant behavioral changes were observed in the progeny of all test groups.     

Adenosine receptor interactions and anxiolytics

$\text{[}{}^3\text{H}\text{]-N}{}^6\text{-}\text{cyclohexyladenosine}$ and [³H]-1,3-diethyl-8-phenylxanthine label the A₁ subtype of adenosine receptor in brain membranes. The affinities of methylxanthines in competing for A₁ adenosine receptors parallel their potencies as locomotor stimulants. The adenosine agonist N⁶-(-phenylisopropyl) adenosine is a potent locomotor depressant. Both diazepam and $\text{N}{}^6\text{-(}\text{l}\text{-}\text{phenylisopropyl}\text{)}\text{adenosine}$ cause locomotor stimulation in a narrow range of subdepressant doses. Combined stimulant doses of the two agents depress motor activity, as do larger doses of either one, given separately.Evidence supporting and against the hypothesis that some of the actions of benzodiazepines are mediated via the adenosine system is reviewed. A number of compounds interact with both systems, probably because of physico-chemical similarities between adenosine and diazepam. It is concluded that of the four classic actions of benzodiazepines, the sedative and muscle relaxant (but not anxiolytic or anticonvulsant) actions could possibly be mediated by adenosine.     

The Ah regulatory gene product. Survey of nineteen polycyclic aromatic compounds' and fifteen benzo[a]pyrene metabolites' capacity to bind to the cytosolic receptor

The capacity of 19 polycyclic aromatic compounds and 15 benzo[a]pyrene metabolites to displace $\text{[1,6-}{}^3\text{H}\text{]2,3,7,8-}\text{tetrachlorodibenzo}\text{-p-}\text{dioxine}\text{([}{}^3\text{H]Tcdd}\text{)}$ from the mouse liver cytosolic Ah receptor was examined. We compared our data with various parameters taken from previously published results: the capacity of seven polycyclic hydrocarbons to induce aryl hydrocarbon hydroxylase (AHH) activity in human cell cultures, the capacity of 10 polycyclic hydrocarbons to induce azo dye N-demethylase activity in rat liver, the capacity of 6 polycyclic hydrocarbons to shorten zoxazolamine paralysis times in the intact rat, and the capacity of 15 benzo[a]pyrene metabolites to induce AHH activity in rat hepatoma H-4-II-E cultures. An excellent correlation is seen between the capacity to displace the radioligand from the Ah receptor and the capacity to induce these monooxygenase activities. Differences in the rate of cellular uptake and formation of alkali-extractable metabolites of dibenzo[a,h]anthracene, 3-methylcholanthrene, and benzo[a]anthracene in Hepa-1 mouse hepatoma cell cultures do not account for differences in the capacity of these three polycyclic hydrocarbons to displace [³H]TCDD from the Ah receptor.     

Similar activities of nerve growth factor and its homologue proinsulin in intracellular hydrogen peroxide production and metabolism in adipocytes: Transmembrane signalling relative to insulin-mimicking cellular effects

Generation of hydrogen peroxide in adipocyte plasma membrane and its intracellular metabolism and regulatory role have been shown by Mukherjee and co-workers to be a major effector system for insulin [Fedn Proc.35, 1694 (1976); Archs Biochem. Biophys.184, 69 (1977); Biochem. Pharmac.27, 2589 (1978); Fedn Proc.37, 1689 (1978); and Biochem. Pharmac.29, 1239 (1980)]. The possible involvement of this mechanism in the action of structurally similar polypeptides having some insulin-like metabolic effects was investigated. The β-subunit of nerve growth factor (2.5 S NGF, mol. wt 13,500) which has a striking structural homology with proinsulin and has been reported to exert certain insulin-like metabolic effects in its own target tissues (e.g. growing neurites and sympathetic ganglia), and the insulin-derived polypeptides, desalanine-insulin and desoctapeptide-insulin, as well as proinsulin, were examined for their effects on rat adipocytes, employing the technique of formate oxidation. Both NGF and proinsulin caused increased [¹⁴C]formate oxidation, showing similar intrinsic activities, up to a maximum of 140–160% of the basal rate; insulin increased the rate to 190–210% of the basal rate. The relative potencies of the hormones toward H₂O₂ formation and stimulation of the pentose phosphate pathway activity were: insulin $\text{(}\text{EC}{}_{50}\text{: 2.5 × 10}{}^{\mathrm{?11}}\text{M}\text{)}$, desalanine-insulin $\text{(}\text{EC}{}_{50}\text{: 2.5 × 10}{}^{\mathrm{?10}}\text{M}\text{)}$ , proinsulin $\text{(}\text{EC}{}_{50}\text{: 8 × 10}{}^{\mathrm{?9}}\text{M}\text{)}$, and NGF $\text{(}\text{EC}{}_{50}\text{: 10}{}^{\mathrm{?9}}\text{M}\text{)}$. The biologically inactive derivative, desoctapeptide-insulin, did not stimulate glucose oxidation, although it caused a small increase in formate oxidation, with an $\text{EC}{}_{50}\text{of}\text{5 × 10}{}^{\mathrm{?7}}\text{M}$, indicating a suboptimal level of H₂O₂ formation in the elevation of the hexose monophosphate shunt activity. 3-Amino-1,2,4,-triazole (50 mM), which irreversibly decomposes the peroxidatic compound II of the catalase: H₂O₂ complex, inhibited formate oxidation to a greater extent in the hormone-treated cells than in the control cells, whereas sodium azide, an inhibitor of the hemoprotein, catalase, completely inhibited it. The abilities of the polypeptides to stimulate H₂O₂ formation correlated with their abilities to promote lipogenesis from [U-¹⁴C]-D-glucose, as expected of insulin. The cellular GSH/GSSG ratio increased concomitantly with the stimulation of glucose oxidation via the shunt, indicating a tight coupling between these processes. The results confirm that the hydrogen peroxide production is a common basis of the metabolic actions of growth-promoting polypeptide hormones or mitogens beyond their respective receptors.     

Tissue distribution of histamine in a mutant mouse deficient in mast cells: Clear evidence for the presence of non-mast-cell histamine

The contents of histamine in various tissues of mutant mice deficient in mast cells ($\text{W}\text{W}{}^{\mathrm{v}}$) and in congenic normal mice (+/+) were determined by high-performance liquid chromatography and were compared. In spite of the absence of mast cells in $\text{W}\text{W}{}^{\mathrm{v}}$ mice, the histamine content of their whole bodies was about 5–10% of that of +/+ mice. The skin, heart and lungs of $\text{W}\text{W}{}^{\mathrm{v}}$ mice contained negligible amounts of histamine (about 2% of that in +/+ mice), but the liver, kidneys and spleen contained appreciable histamine (8–15% of that in +/+ mice), and the brain and stomach contained much histamine (45 and 34%, respectively, of that in +/+ mice). These results indicate the presence of non-mast-cell histamine, especially in the brain and stomach, where it may play important physiological roles.     

Effect of exposure to nitrogen dioxide on t and b cells in mouse spleens

Effects of exposure to nitrogen dioxide (NO₂) on thymus-derived (T) and bursa-derived (B) cells were studied in albino mice. The mice were exposed continuously 24 $\text{h}\text{day}$ to 940 $\text{μg}\text{m}{}^3$ NO₂ and to 188 $\text{μg}\text{m}{}^3$ NO₂ with daily 3-h peaks 5 $\text{days}\text{week}$ of either 470, 940 or 1880 $\text{μg}\text{m}{}^3$ NO₂. After 1, 3, 6, 9 and 12 months of exposure, single-cell suspensions were prepared from spleen and incubated with phytohemagglutinin (PHA) or bacterial lipopolysaccharide (LPS). The PHA and LPS responses from mice exposed to NO₂ were generally depressed when compared with those in mice exposed for the same time periods to filtered air.     

Correlation of biologic data with physico-chemical properties among the vinca alkaloids and their congeners.

Displacement of [³H]vinblastine binding to tubulin by other Vinca alkaloid derivatives has been demonstrated to be a competitive process, allowing for determination of the association constant of each drug. Correlation of LD₅₀ data and anti-P-388 activity was found with log P and log K_a, according to the equations: $\text{log}\text{LD}{}_{50}\text{= 0.129 (}\text{log}\text{P)}{}^2\text{? 0.522}\text{log}\text{P ? 0.479}\text{log}\text{K}{}_{\mathrm{a}}\text{+ 4.652}\text{log}\text{P ? 388 = 0.222 (}\text{log}\text{P)}{}^2\text{? 1.059}\text{log}\text{P ? 0.520}\text{log}\text{K}{}_{\mathrm{a}}\text{+ 5.366}$. Vincristine and desacetylvinblastine were the two most active agents in this series. That the latter drug had significant biologic activity was of considerable interest, since it is known to be a human metabolite.     

Genotoxicity of N-nitrosothiazolidine in microbial and hepatocellular test systems

The genotoxicity of N-nitrosothiazolidine was studied in a microbial system and in a hepatocellular system. The compound showed positive responses in both tests, exhibiting weak mutagenicity at the lowest level tested (1 mg/plate) in the rec assay in Bacillus subtilis, and inducing statistically significant levels of DNA repair in primary hepatocyte cultures at concentrations ranging from 2 × 10^?4 to $\text{2 × 10}{}^{\mathrm{?3}}\text{m}$.     

N-[2(o-iodophenoxy)ethyl]cyclopropylamine hydrochloride (LY121768), a potent and selective irreversible inhibitor of type a monoamine oxidase

The effects of N-[2-(o-iodophenoxy)ethyl]cyclopropylamine hydrochloride (LY121768) on types A and B monoamine oxidase (MAO) assayed with radiocarbon-labeled serotonin and phenyl-ethylamine, respectively, were studied in vitro and in vivo. Type A MAO from rat brain was inhibited in vitro by LY121768 with an ic₅₀ of 4 × 10^?10 M, whereas 2500 times higher concentrations of LY121768 $\text{(}\text{ic}{}_{50}\text{= 1 × 10}{}^{\mathrm{?6}}\text{M}\text{)}$ were required to inhibit type B MAO. The inhibition of type A MAO increased with time of incubation of LY121768 with enzyme prior to substrate addition and persisted after dialysis, indicative of irreversible inhibition. The irreversible inactivation was prevented by harmaline, a reversible, competitive inhibitor of type A MAO, indicating a requirement for catalytic activity of MAO in the time-dependent inactivation by LY121768. In rats, LY121768 selectively inhibited type A MAO in brain and in liver at low doses. The inhibition of type A MAO persisted for several days after a single 10 mg/kg i.p. dose of LY121768 and was associated with a significant increase in brain dopamine, norepinephrine and epinephrine concentrations and a significant decrease in the concentration of the dopamine metabolites, homovanillic acid and 3.4-dihydroxyphenylacetic acid. The inactivation of type A MAO by LY121768 in vivo was prevented by co-administration of harmaline, indicating a similar mechanism for the in vivo inactivation as for the in vitro inactivation of MAO by LY121768. A reasonable inference from these data and from previous literature is that LY121768 acts as a “suicide substrate” for MAO and inactivates the enzyme by formation of a reactive intermediate which binds covalently to the enzyme. The presence of iodine in the LY121768 molecule not only confers high selectivity for type A MAO but offers a site for radionuclide introduction that might be a useful means of labeling type A MAO in vitro or in vivo for various purposes.     

Mechanisms by which quipazine,a putative serotonin receptor agonist,alters brain 5-hydroxyindole metabolism

Quipazine (2-[1-piperazinyl] quinoline maleate) was shown to increase serotonin and decrease 5-hydroxyindoleacetic acid concentrations in whole brain, several brain regions, and the spinal cord of rats 1 hr after its administration (10 mg/kg, i.p.). In animals with transected spinal cords, quipazine induced stronger activation of extensor reflexes than 5-hydroxytryptophan, chlorimipramine, or Lilly 110140. This response could be blocked by methiothepin. In slices of rat cerebral cortex, quipazine inhibited the uptakes of [³H]-serotonin (EC₅₀ = 10^?6 M) and [³H]-norepinephrine ($\text{EC}{}_{50}\text{= 2 × 10}{}^{\mathrm{?6}}\text{m}$); it was equipotent with Lilly 110140 in inhibiting serotonin uptake, but less potent than chlorimipramine ($\text{EC}{}_{50}\text{= 10}{}^{\mathrm{?7}}\text{m}$). Quipazine administration to rats did not inhibit monoamine oxidase activity, and actually elevated brain tryptophan levels. These observations suggest that the effects of quipazine on brain serotonin and 5-hydroxyindoleacetic acid concentrations could have been caused by direct activation of central serotonin receptors (which would secondarily decrease impulse flow along serotonergic neurones), or by the inhibition of serotonin reuptake, or by both mechanisms.     

Effect of polychlorinated biphenyls on the immune responses of rhesus monkeys and mice.

The relationship between lipid peroxidation, glutathione (GSH) content, and CCl₄-induced toxicity was investigated in rat hepatocytes isolated by a collagenase-perfusion technique. Two chemical initiators of lipid peroxidation, ferric ions complexed with adenosine diphosphate ($\text{ADP}\text{Fe}{}^{\mathrm{3+}}$) and diethyl maleate, were studied for comparison. CCl₄ caused a reduction of intracellular K⁺ and release of alanine aminotransferase (ALT) into the medium, but no evidence of lipid peroxidation, as measured by the absorbance of thiobarbituric acid (TBA)-reacting materials and lipid-extract diene conjugation. $\text{ADP}\text{Fe}{}^{\mathrm{3+}}$ caused lipid peroxidation, but only a small loss of K⁺. Diethyl maleate caused a greater amount of lipid peroxidation and cell damage than did $\text{ADP}\text{Fe}{}^{\mathrm{3+}}$. Neither response appeared to be related to the GSH content, which was reduced by diethyl maleate, but not by $\text{ADP}\text{Fe}{}^{\mathrm{3+}}$, and by CCl₄ only at the highest dose. The results suggest that lipid peroxidation is not a requisite step in CCl₄-induced toxicity in isolated hepatocytes.     

Dansylarginine N-(3-ethyl-1,5-pentanediyl)amide: A potent and selective fluorescent inhibitor of butyrylcholinesterase

Interactions between dansylarginine N-(3-ethyl-1,5-pentanediyl)amide (DAPA) and the cholinesterases were examined by the techniques of enzyme kinetics and fluorescence spectroscopy. When tested with partially purified enzyme preparations, DAPA was a potent inhibitor of butyrylcholinesterase $\text{(}\text{IC}{}_{50}\text{= 2 × 10}{}^{\mathrm{?7}}\text{M}\text{)}$ but not of acetylcholinesterase $\text{(}\text{IC}{}_{50}\text{= 4 × 10}{}^{\mathrm{?4}}\text{M}\text{)}$. For a detailed study of the effects of DAPA on butyrylcholinesterase (BuChE), the enzyme was purified to homogeneity from horse serum, with the aid of affinity chromatography on N-methyl acridinium. The kinetics of the inhibition of purified BuChE by DAPA were complex, having both competitive and non-competitive features, and it was not possible to estimate K_i unambiguously. Spectroscopic measurements showed that the fluorescence of the dansyl moiety was strongly affected by the binding to BuChE. With excitation at 330 nm, total fluorescence emission from bound DAPA (at 450 nm and above) was 21-fold greater than from free DAPA. In a titration experiment, this enhancement of fluorescence intensity was used to calculate that each monomer of BuChE has two apparently independent DAPA-binding sites with a K_d of 4.5 × 10^?7 M. Further measurements showed that the fluorescence emission of bound DAPA was markedly blue-shifted (to 502 nm from 570 nm in free solution) and that the fluorescence lifetime of this form was greatly prolonged (to 24 nsec from 2.7 nsec). These observations indicate that the high affinity binding sites on BuChE lock DAPA in a highly non-polar environment.     

Acute tobacco smoke exposure alters the profile of metabolites produced from benzo[a]pyrene by the isolated perfused rabbit lung

The influence of whole tobacco smoke or the gas phase from smoke on the metabolism of $\text{[}{}^{14}\text{C]benzo}\text{[a]}\text{pyrene}$ was e xamined using the isolated perfused rabbit lung model. Fresh whole tobacco smoke mixed with the air ventilating the perfused lung produces an immediate and dose related decrease in the metabolism of $\text{[}{}^{14}\text{C]benzo}\text{[a]}\text{pyrene}$. The metabolites of $\text{[}{}^{14}\text{C]benzo}\text{[a]}\text{pyrene}$, diols, quinones, phenols and polar compounds are generally decreased in quantity. At the lowest level of smoke administered the percentage of BP-7,8-diol produced is increased dramatically. The results indicate that one of the factors contributing to the carcinogenicity of tobacco smoke may be its ability to produce an immediate alteration in the pulmonary metabolism of polycyclic aromatic hydrocarbons.     

Brain metabolite concentrations and redox states in rats fed diets containing 1,3-butanediol and ethanol

Both ethanol and its dimer 1,3-butanediol (BD) are substrates for alcohol dehydrogenase in liver and thus have many similar effects upon metabolite concentrations and redox states in that organ. Although the mechanism by which ethanol exerts its effects on the brain is not known, it must differ from that in liver since brain contains insignificant amounts of alcohol dehydrogenase. The effects of BD, which does not produce intoxication, and ethanol upon brain were compared in an attempt to determine which changes in metabolite content are related to depression of the CNS. Diets containing 47% of calories as ethanol, BD, or glucose were pair-fed to rats for 62 days. The brains were then removed and frozen with a new apparatus which prevents postmortem changes, and concentrations of metabolites were determined. Substitution of BD for glucose in the diet caused a decrease in the brain content of glucose, lactate and α-oxoglutarate and an increase in glutamate and citrate. Substitution of ethanol for glucose caused only a decrease in the brain content of glucose and an increase in citrate. The ethanol diet, as compared with the BD diet, caused an elevation of the brain content of glucose and a decrease in glutamate. Both BD and ethanol caused a decrease in the free cytoplasmic $\text{[}\text{NADP}{}^{\mathrm{+}}\text{]}\text{[}\text{NADPH}\text{]}$ ratio in brain without changing the $\text{[}\text{NAD}{}^{\mathrm{+}}\text{]}\text{[}\text{NADH}\text{]}$ of cytoplasm or mitochondria.Except for the differences in effect upon glucose and glutamate, BD and ethanol appear to act similarly on the metabolite content of rat brain. It is therefore concluded that the brain is resistant to changes of the measured metabolites during the process of chronic ethanol ingestion. It is further suggested that the small changes observed in the cytoplasmic $\text{[}\text{NADP}{}^{\mathrm{+}}\text{]}\text{[}\text{NADPH}\text{]}$ ratio after ethanol feeding are not related to the depression of CNS activity associated with ethanol ingestion since they also occur after feeding BD.     

A study of norepinephrine metabolism in rat brain using a double label technique

Using a double-label procedure, the incorporation of endogenously-derived ³⁵SO₄ into phenylethylene glycol sulfates (PGS) was estimated. When [³H]norepinephrine and [³⁵S]cysteine were injected concomitantly into the brain, about 30–80 percent of the tritium and about 4 percent of the ³⁵S retained in the brain 1 hr later were in PGS. In B₆-deficient rats, the proportion of ³⁵S was increased as was the ${}^{35}\text{S}{}^3\text{H}$ ratio. Probenecid caused a significant increase in the amount of PGS found in the brain, but a minimal enrichment of ³⁵S was observed, suggesting that there was little or no effect on sulfotransferases. Cysteine in high concentrations inhibits the incorporation of tritium into PGS.     

Hydrocarbons and metabolites in english sole (Parophrys vetulus) exposed simultaneously to [3H]benzo[a]pyrene and [14C]naphthalene in oil-contaminated sediment

English sole (Parophrys vetulus) were exposed to $\text{[}{}^3\text{H]benzo}\text{[a]}\text{pyrene (B}\text{[a]}\text{P}\text{)}$ and [¹⁴C]naphthalene (NPH) in sediment containing 1% Prudhoe Bay crude oil (PBCO). Bioeoncentration values (pmoles of hydrocarbon equivalents in g of dry tissue/pmoles of hydrocarbon equivalents in g of sedimentassociated water (SAW)) for NPH were greater than corresponding values for B[a]P in tissues of fish exposed for 24 h. However, from 24 to 168 h of the exposure, a substamial decline (P < 0.05) in NPH-derived radioactivity and a significant (P < 0.05) increase in B[a]P-derived radioactivity occurred in most of the tissues examined. When fish were transferred for 24 h to sediment free of radioactivity and PBCO, the retention of B[a]P-derived radioactivity in the tissues of fish was considerably greater than that for NPH.Metabolites of B[a]P and NPH in sediment, SAW, liver and bile of fish were characterized by thinlayer chromatography (TLC). For liver, a two-dimensional TLC was devised to separate B[a]P and its metabolites from liver lipids. An important finding was that liver of English sole metabolized B[a]P to a far greater extent than NPH; at 24 h after the exposure, the ratio of concentrations of B[a]P to its metabolites was 1 to 49 whereas that for NPH was 6 to 1. Larger proportions of glucuronide conjugates than sulfate conjugates of both NPH and B[a]P were present in bile of English sole. Naphthalene was largely converted into a glucuronide conjugate of l,2-dihydro-l,2-dihydroxynaphthalene. A number of metabolites of B[a]P known to be toxic to mammals were detected in both liver and bile including 7,8-dihydro-7,8-dihydroxy B[a]P and its conjugates.These findings of extensive metabolism of B[a]P by fish liver very probably explain why B[a]P is usually not detected in liver of fish even when considerable concentrations of B[a]P are detected in the environment of the fish.     

Inhalation studies on the biotransformation and elimination of [14C] trichlorofluoromethane and [14C] dichlorodifluoromethane in beagles

The possible biotransformation of trichlorofluoromethane (FC-11) and dichlorodifluoromethane (FC-12) was investigated in 4 male and 2 female adult Beagles after a short (6- to 20-min) inhalation. Dogs were anesthetized with ketamine and succinylcholine, intubated, and ventilated artificially. Trichlorofluoromethane (1000–5000 ppm, $\text{v}\text{v}$) or dichlorodifluoromethane 38000–12,000 ppm, $\text{v}\text{v}$) containing up to 180μ Ci of $\text{[}{}^{14}\text{C}\text{]}\text{fluorocarbon}$ was delivered from 110-liter Teflon bags, and all exhalations were collected via a nonrebreathing valve in similar bags for 1 hr. Venous blood samples were withdrawn at appropriate times and assayed for fluorocarbon-associated radioactivity. Exhalation bags were assayed for $\text{[}{}^{14}\text{C}\text{]}\text{fluorocarbon}$ and ¹⁴CO₂. Urine was collected for up to 3 days and assayed for ${}^{14}\text{C}$ metabolites as nonvolatile radioactivity. In some experiments animals were sacrificed 24 hr after exposure and tissues were removed for determination of nonvolatile radioactivity. Essentially all of the administered (inhaled) fluorocarbon was recovered in the exhaled air within 1 hr. Only traces of radioactivity were found in urine or exhaled carbon dioxide. All tissues contained measurable concentrations of nonvolatile radioactivity 24 hr after exposure but together represented less than 1% of the administered dose. It is not possible to determine if these trace levels are associated with metabolites of the fluorocarbons or with the unavoidable radiolabeled impurities present in the administered gas mixture. Neither phenobarbital pretreatment (60 mg/day for 3 days) nor prolonged exposure (50–90 min) produced any alteration of these results. Thus, it can be concluded that FC-11 and FC-12 are relatively refractory to biotransformation after a short inhalation exposure and that they are rapidly exhaled in their unaltered chemical form.