Relationship of metabolism of 2′-, 3′- and 5′-adenine nucleotides to presynaptic inhibition of transmitter release in rat vas deferens

Summary In the isolated rat vas deferens stimulated at 0.2 Hz, a series of 2, 3-, and 5-substituted adenine nucleotides all inhibited the twitch responses, their actions being potentiated by the nucleoside transport inhibitors, HNBTGR, NBMPR and dipyridamole.The metabolism of these nucleotides was examined utilising HPLC analysis of the bathing medium after exposure to 30 M nucleoside or nucleotide for 5 min. 5-AMP, 5-ADP, 5-ATP, and NAD⁺ were all partially hydrolysed to adenosine, the relative extent of this being 5-AMP>5-ADP=5-ATPNAD⁺. However, the other nucleotides examined were not detectably converted to adenosine or to adenosine deamination products.These results indicate that the 2-, 3- and 5-substituted nucleotides studied act at a P₁-purinoceptor in rat vas deferens to inhibit neurotransmission and, with the exception of 5-AMP, 5-ADP, 5-ATP and NAD⁺, all appear to act directly at this receptor. However, the 5-adenine nucleotides (AMP, ADP and ATP) and NAD⁺ all appear to act at least partially indirectly subsequent to their hydrolysis to adenosine.Abbreviations. The following abbreviations are used ADA adenosine deaminase (EC 3.5.4.4) - 5-ADP adenosine 5-diphosphate - 2,5-ADP adenosine 2,5-diphosphate - 3 5-ADP, adenosine 3,5-diphosphate - 2-, 3 or 5-AMP adenosine 2-, 3-, or 5-monophosphate - 5-ATP adenosine 5-triphosphate - cNADP⁺ -nicotinamide dinucleotide 2,3-cyclic monophosphate - CoA coenzyme A - HNBTGR 6-(2-hydroxy-5-nitrobenzyl)-thioguanosine - NAD⁺ -nicotinamide adenine dinucleotide - NADP⁺ -nicotinamide adenine dinucleotide phosphate - NBMPR 6-(4-nitrobenzylthio)-purine riboside     

Metabolism and presynaptic inhibitory activity of 2′,3′ and 5′-adenine nucleotides in rat vas deferens

Summary In the isolated rat vas deferens stimulated at 0.2 Hz, [¹⁴C]labelled 5-AMP, 5-ADP and 5-ATP (10 M) inhibited twitch responses, were broken down to [¹⁴C]adenosine in the medium and incorporated into [¹⁴C]adenine ribonucleotides in the tissue. Pretreatment of tissues with 6-(2-hydroxy-5-nitrobenzyl)-thioguanosine (NBTGR), a potent inhibitor of adenosine transport, potentiated the presynaptic inhibitory action of these 5 nucleotides and reduced their incorporation in [¹⁴C]adenine nucleotides, but did not alter the appearance of [¹⁴C]adenosine in the medium.A series of 2, 3 and 5-substituted adenine nucleotides (10 M) inhibited the twitch responses of the vas deferens stimulated at 0.2 Hz. This effect was potentiated by NBTGR. Addition of exogenous adenosine deaminase very significantly reduced the inhibitory actions of adenosine, 5-AMP, 5-ADP and 5-ATP and also reduced those of 2, 5-ADP, NAD⁺ and dePCoA. The inhibitory actions of the other 2, 3 and 5 adenine nucleotides studied were not altered by exogenous adenosine deaminase.These results indicated that the presynaptic inhibitory actions of 5-AMP, 5-ADP and 5-ATP in rat vas deferens predominantly result from their prior hydrolysis to adenosine whereas the 2, 3 and 5-substituted adenine nucleotides appear to act mainly directly to inhibit transmitter release.Abbreviations. The following abbreviations are used 5-ADP 5-adenosine diphosphate - 2,5-ADP 2,5-adenosine diphosphate - 3,5-ADP 3,5-adenosine diphosphate - 2,3 or 5-AMP 2,3 or 5-adenosine monophosphate - 5-ATP 5-adenosine triphosphate - CoA coenzyme A - 2,3-cAMP 2,3-cyclic adenosine monophosphate - cNADP⁺ -nicotinamide dinucleotide 2,3-cyclic monophosphate - dePCoA dephosphocoenzyme A - NAD⁺ -nicotinamide adenine dinucleotide - NADP⁺ -nicotinamide adenine dinucleotide phosphate - NBTGR 6-(2-hydroxy-5-nitrobenzyl)-thioguanosine - oxid CoA oxidized-coenzyme A     

The Solution Conformations of Lidocaine Analogues

IR and ¹H NMR studies in CDCl₃ and CCl₄ of a series of tertiary aminoxylidides with the amino group in the 2 to 6 position of the acyl chain are described. Lidocaine, diethylaminoaceto-2,6-xylidide, forms an intramolecular five-membered ring hydrogen-bonded monomer at all concentrations in both solvents. -Diethyl-amino-propiono-2,6-xylidide forms an intramolecular six-membered ring hydrogen-bonded monomer in CDCl₃ and CCl₄ but a trans intermolecularly associated species is the major form present at high concentrations in CCl₄. The longer-chain homologues are mixtures of nonassociated trans and cis monomers at low concentrations but associated trans forms predominate at high concentrations. Evidence for the presence of a hydrogen-bonded seven-membered ring intramolecular monomer in CDCl₃ for -diethylaminobutyro-2,6-xylidide is presented. The relationship between the molecular conformation and the partition coefficient is discussed.     

The in vitro/in vivo comparative metabolism of 4-aminobiphenyl using isolated hepatocytes

The metabolism of 4-aminobiphenyl by isolated hepatocytes from various species was compared with urinary metabolite profiles in the same species. Radioactive compounds in concentrates of ether extracts from hepatocytes or urine following hydrolysis were analysed by TLC and reversed phase HPLC in conjunction with radioactivity monitoring and synthetic standards.The major metabolites from hepatocytes and in urine were 4-acetamidobiphenyl, 3-hydroxy-4-aminobiphenyl 4-hydroxy-4-aminobiphenyl and 4-hydroxy-4-acetamidobiphenyl. Oxidation of the amine nitrogen gave hydroxylamino, nitroso and nitro compounds. Minor metabolites were 2-hydroxy amine and amide, the hydroxamic acid and the oxamic acid. The urinary metabolite profiles correlated well with those from hepatocytes for each species.Abbreviations Used 4-ABP 4-aminobiphenyl - AA 4-acetamidobiphenyl - A3-OH 3-hydroxy-4-aminobiphenyl - A4-OH 4-hydroxy-4-aminobiphenyl - A2-OH 2-hydroxy-4-aminobiphenyl - AA4-OH 4-hydroxy-4-acetamidobiphenyl - AA3-OH 3-hydroxy-4-acetamidobiphenyl - AA2-OH 2-hydroxy-4-acetamidobiphenyl - AAN-OH N-hydroxy-4-acetamidobiphenyl - NBP 4-nitrobiphenyl - AN-OH 4-hydroxylaminobiphenyl - NOBP 4-nitrosobiphenyl Dedicated to Professor Dr. med. Herbert Remmer on the occasion of his 65th birthday     

Amino Acid Ester Prodrugs of Floxuridine: Synthesis and Effects of Structure,Stereochemistry, and Site of Esterification on the Rate of Hydrolysis

Purpose. To synthesize amino acid ester prodrugs of floxuridine (FUdR) and to investigate the effects of structure, stereochemistry, and site of esterification of promoiety on the rates of hydrolysis of these prodrugs in Caco-2 cell homogenates. Methods. Amino acid ester prodrugs of FUdR were synthesized using established procedures. The kinetics of hydrolysis of prodrugs was evaluated in human adenocarcinoma cell line (Caco-2) homogenates and pH 7.4 phosphate buffer. Results. 3-Monoester, 5-monoester, and 3,5-diester prodrugs of FUdR utilizing proline, L-valine, D-valine, L-phenylalanine, and D-phenylalanine as promoieties were synthesized and characterized. In Caco-2 cell homogenates, the L-amino acid ester prodrugs hydrolyzed 10 to 75 times faster than the corresponding D-amino acid ester prodrugs. Pro and Phe ester prodrugs hydrolyzed much faster (3- to 30-fold) than the corresponding Val ester prodrugs. Further, the 5-monoester prodrugs hydrolyzed significantly faster (3-fold) than the 3,5-diester prodrugs. Conclusions. Novel amino acid ester prodrugs of FUdR were successfully synthesized. The results presented here clearly demonstrate that the rate of FUdR prodrug activation in Caco-2 cell homogenates is affected by the structure, stereochemistry, and site of esterification of the promoiety. Finally, the 5-Val and 5-Phe monoesters exhibited desirable characteristics such as good solution stability and relatively fast enzymatic conversion rates.     

Relaxation of hormonally stimulated smooth muscular tissues by the 8-bromo derivative of cyclic GMP

Summary Substances that cause contraction or relaxation of smooth muscle have been shown to increase intracellular levels of cyclic GMP. Because of the unclear role of cyclic GMP in the control of smooth muscle tone, cyclic GMP derivatives were exogenously applied to various smooth muscle preparations and their effects on tissue tone were studied.Whereas the basal tone of the rat ductus deferens was not affected by exogenous cyclic GMP or its dibutyryl or 8-bromo derivatives, the contractile responses of this tissue to noradrenaline and acetylcholine were depressed by preincubation with 10 M 8-bromo cyclic GMP (Br-cGMP). The 8-bromo derivatives of 2:3-cyclic GMP, 5-GMP and guanosine were without effects. Cyclic AMP levels were not changed by Br-cGMP. The frequency of oxytocin-stimulated rat uteri was also depressed by Br-cGMP (10 M). In helical strips of rat and rabbit aortae, Br-cGMP (1–100 M) caused a concentration-dependent, rapid decrease in noradrenaline-stimulated tissue tension. Br-2:3-cyclic GMP was ineffective. Noradrenaline-stimulated strips from hog spleen arteries were less sensitive to Br-cGMP than aortic tissue. In ductus deferentes and aortic strips stimulated by K⁺ at a depolarizing concentration, Br-cGMP caused less relaxation than under hormonal stimulation.These findings support the concept that cyclic GMP is involved in the control of smooth muscle tone and that hormone- and drug-induced elevations of the cyclic GMP level can reduce contractile responses to neurotransmitters and hormones.Abbreviations cGMP Guanosine 3:5-monophosphate, cyclic GMP - dibutyryl cGMP N², 2-O-dibutyryl guanosine 3:5-monophosphate - Br-cGMP 8-bromo guanosine 3:5-monophosphate - Br-2:3-cGMP 8-bromo guanosine 2:3-monophosphate - Br-GMP 8-bromo guanosine 5-monophosphate - Br-Guo 8-bromo guanosine, Br-guanosine - cAMP adenosine 3:5-monophosphate, cyclic AMP - dibutyryl cAMP N⁶, 2-O-dibutyryl adenosine 3:5-monophosphate - Br-cAMP 8-bromo adenosine 3:5-monophosphate This work was supported by grants from the Deutsche Forschungsgemeinschaft. Preliminary reports were presented (Schultz, 1977b; Schultz et al., 1978).     

The Liposome Partitioning System for Correlating Biological Activities of Imidazolidine Derivatives

The partitioning of 10 imidazolidines in various liposome/buffer systems (log K _m) has been determined and compared to partitioning in the n-octanol/buffer system (log P). The log K _m, which was generally greater than the log P, increased or decreased upon the addition of dicetylphosphate (DCP) or stearylamine (STA), respectively, to dimyristoylphosphatidylcholine (DMPC) liposomes. Quantitative correlations of ₂-adrenergic potencies of imidazolidines have been made by regression analyses with log P, log K _m, binding affinity, and intrinsic activity. Both central and peripheral potencies correlated with log K _m but not with log P Multiple regressions yielded improved predictable quantification of these potencies. Thus, the liposomal membrane system shows certain advantages over the n-octanol/buffer system for the prediction of biological activities of the imidazolidines.     

The binding spectrum of narcotic analgesic drugs with different agonist and antagonist properties

Summary Four groups of narcotic analgesic drugs have been assessed for their opiate activities by using three binding assays and three pharmacological bioassays. In the binding assays, their inhibition constants (K _I, nM) were determined against the binding of the -ligand, [³H]-[d-Ala ² ,MePhe ⁴ , Gly-ol⁵]enkephalin, of the -ligand, [³H]-[d-Ala ² ,d-Leu ⁵]enkephalin and of the -ligand, [³H]-(±)-ethylketazocine after suppression of - and -binding by 100 nM of the unlabelled -ligand and 100 nM of the unlabelled -ligand. The pharmacological agonist or antagonist activities were assayed on the guinea-pig ileum, mouse vas deferens and rat vas deferens.The first group of compounds were pure agonists in all three pharmacological bioassays. The majority of the compounds showed preference to -binding but phenazocine and particularly etorphine had also high affinities to the - and -binding sites.The second group consisted of N-allyl and N-cyclopropylmethyl homologues of the morphine, 3-hydroxymorphinan and normetazocine series which had agonist and antagonist activities in the guinea-pig ileum and mouse vas deferens but were pure antagonists in the rat vas deferens. In the binding assays, -binding and -binding were prominent.The third group was made up by the ketazocine-like compounds which in the guinea-pig ileum and mouse vas deferens were pure agonists and in the rat vas deferens pure antagonists. The binding spectrum showed particularly high binding to the -binding site.The fourth group was the antagonists which were devoid of agonist activity with the exception of diprenorphine and Mr 2266 which had retained some agonism. The binding spectrum showed considerable variation, naloxone in low concentration being a selective -antagonist, Mr 2266 having high affinities to the - and -binding sites and diprenorphine having considerable affinities to the -, - and -binding sites.Since each of the four groups of compounds, whether pure agonists, agonist-antagonists, ketazocine-like drugs or pure antagonists, shows independent varittions in the affinities to the - and -binding sites, their different pharmacological behaviour cannot be solely due to difference in the binding spectra.     

Rat diaphragm cyclic nucleotide-phosphodiesterase: Influence of drugs affecting skeletal muscle contractility

Summary In the present study a phosphodiesterase was partly purified from rat diaphragm and its properties as well as the effects of some drugs known to affect neuromuscular transmission were examined.The enzyme preparation had a pH optimum of 7.0–8.0 As for phosphodiesterase of other organs, the activity was dependent on Mg²⁺ and mainly located in the 100 000×g supernatant. It showed two apparent K _m values (6.4 and 390 M) for the cyclic adenosine-3,5-monophosphate hydrolysis. Various drugs inhibited diaphragm phosphodiesterase non-competitively in the following order of potency: eupaverine papaverine > 1-hexyl-3,7-dimethylxanthine > Ro 7-2956 > theophylline > d-tubocurarine > hydrochlorothiazide. Succinylcholine was ineffective.Of the cyclic nucleotides tested here only cyclic guanosine-3,5-monophosphate elicited an inhibiton at low concentrations (K _i=7M), while cyclic inosine-3,5-monophosphate and cyclic N₆-2-O-dibutyryl-adenosine-3,5-monophosphate inhibited only in high concentrations. Cyclic uridine-3,5-monophosphate did not inhibit phosphodiesterase. The type of inhibition was apparently competitive for cyclic N₆-2-O-dibutyryl-adenosine-3,5-monophosphate and cyclic guanosine-3,5-monophosphate, and non-competitive for cyclic inosine-3,5-monophosphate.The present findings on phosphodiesterase inhibitors agree well with our earlier results on the ability of these drugs (except d-tubocurarine) to increase muscular contractility. It is suggested that their mode of action might be facilitation of the release of acetylcholine from motor nerve endings via the accumulation of cyclic adenosine-3,5-monophosphate.     

Identification of the Diastereomers of Pentobarbital N-Glucosides Excreted in Human Urine

A study was undertaken to determine if humans excreted pentobarbital N-glucosides as urinary metabolites following oral administration of pentobarbital. (lRS,5RS)-l--D-Glucopyranosyl) pentobarbital ((lRS,5RS)-PTBG) was isolated from the urine of one subject. The two diastereomers, (lRS,5R)-PTBG and (lRS,5S)-PTBG were separated and found to be identical to synthetic standards when compared using HPLC retention times coupled with UV (with and without post-column ionization) and mass spectrometry (HPLC/ MS). A HPLC method was developed for detecting and quantifying (lRS,5R)-PTBG, (lRS,5S)-PTBG and pentobarbital in urine. Following a single oral dose of sodium pentobarbital to male subjects (n = 6), 1.6–6.2% of the pentobarbital dose was excreted as (lRS,5S)-PTBG over 60 hours. (lRS,5R)-PTBG was also detected in one subject and accounted for 0.3% of the pentobarbital dose. Using a modified HPLC system, the four pentobarbital N-glucosides were resolved and analysis of a partially purified pentobarbital N-glucoside extract from one subject indicated that only (lR,5R)-PTBG and (lS,5S)-PTBG could be detected as urinary excretion products. These results indicate that the side chain chirality of pentobarbital may influence the observed enantioselectivity for the formation and/or urinary excretion of the pentobarbital N-glucosides.     

Toxicokinetic interactions between chlorinated aromatic hydrocarbons in the liver of the C57BL/6J mouse: I. Polychlorinated biphenyls (PCBs)

2,2,4,4,5,5- (PCB 153), 2,3,3,4,4,5- (PCB 156) and 3,3,4,4,5,5-hexachlorobiphenyl (PCB 169) were administered orally to three groups of C57BL/6J mice using single doses of 1.5–109.1 mg/kg. Two other groups of mice received binary mixtures of PCB 153 and 156 or PCB 153 and 169. The hepatic deposition, elimination, CYP1a and CYP2b dependent enzyme activities were studied during a 77-day period. Some interactive effects on hepatic deposition and elimination were observed, resulting in increased deposition and faster elimination. These effects were most pronounced for the PCBs 156 and 169. A potentiating effect on hepatic CYP1a dependent 7-ethoxyresorufin-O-deethylation (EROD) activity was observed for the combination of PCB 156 and 153. Based on the results from the present study and earlier studies, it is suggested that the potentiating effect on EROD activity might be caused by a mechanism that is governed by at least two factors. The first is a toxicokinetic modulation of hepatic retention. The second factor is probably an elevation of hepatic Ah receptor levels by PCB 153.     

Adenosine 3′,5′-monophosphate in cultured neuroblastoma cells: Effect of adenosine,phosphodiesterase inhibitors and benzazepines

Summary The effect of various neurohormones on intracellular levels of adenosine 3,5-monophosphate were evaluated in a neuroblastoma cell line both, in the presence and in the absence of the phosphodiesterase inhibitors isobutylmethylxanthine and papaverine. Without the phosphodiesterase inhibitors only prostaglandin E₁ increased intracellular adenosine 3,5-monophosphate levels. In the presence of isobutylmethylxanthine and/or papaverine, however, adenosine stimulated adenosine 3,5-monophosphate formation and the effect of prostaglandin E₁ was greatly potentiated. Treatment of the cells with dopamine, 5-hydroxytryptamine, noradrenaline, adrenaline, histamine and prostaglandin F₁ was without effect on adenosine 3,5-monophosphate levels either in the presence or absence of the phosphodiesterase inhibitors. The adenosine concentration for a half maximal effect was about 75 M. The effect of 0.1 mM adenosine was not antagonized by 1 mM theophylline. Several adenosine analogs were tested and found to have little or no effect on adenosine 3,5-monophosphate levels in neuroblastoma N4TG3. Diazepam and to a lesser extent chlordiazepoxide act like phosphodiesterase inhibitors when incubated together with prostaglandin E₁.Part of this work was done during a visit of the authors to NIH, U.S.A., J. S. being a fellow of the Deutsche Forschungsgemeinschaft and B. H. of the Max-Planck-Gesellschaft.     

Cyanine-related compounds: a novel class of potent inhibitors of extraneuronal noradrenaline transport

Summary The neurotransmitter noradrenaline is removed from the extracellular space by neuronal and extraneuronal transport mechanisms. In the past, further functional and biochemical characterisation of the corticosterone-sensitive extraneuronal transporter was hampered by the lack of highly potent inhibitors. Here we describe a new class of selective and highly potent inhibitors of the extraneuronal noradrenaline transporter.Clonal Caki-1 cells possess the human type of extraneuronal noradrenaline carrier. The effect of various steroids and steroid-like compounds on initial rates of specific ³H-noradrenaline transport in Caki-1 cells was investigated. None of these steroids had an inhibitory potency higher than that of corticosterone which hitherto was generally accepted as the most potent inhibitor of the extraneuronal noradrenaline transport. On the other hand, a variety of quinoline and isoquinoline derivatives interacted with the extraneuronal noradrenaline transporter. Several cationic quinolines that belong to the chemical class of the cyanine dyes turned out to be very potent inhibitors of ³H-noradrenaline transport in Caki-1 cells. The isocyanines, 1,1-diisopropyl-2,4-cyanine (disprocynium24) and 1-methyl-1-isopropyl-2,4-cyanine as well as the pseudoisocyanines 1,1-diethyl-2,2-cyanine (decynium22) and 1-isopropyl-l-ethyl-2,2-cyanine (iprecynium22) were most potent with IC₅₀'s of 14, 62, 16, and 18 nmol/l, respectively. The inhibitory potency on extraneuronal noradrenaline transport of 1-methyl-l-isopropyl-2,4-cyanine was determined also in isolated organs, namely the isolated incubated rabbit aorta and the isolated perfused rat heart. The IC₅₀'s were 740 and 100 nmol/l, respectively. By contrast, the desipramine-sensitive neuronal type of noradrenaline transporter in PC 12 cells was hardly affected by the cyanine-related compounds. Decynium22 (3 mol/l) inhibited the neuronal noradrenaline transporter of clonal PC12 cells by 14% only.Cyanine-related compounds potently and selectively inhibit the extraneuronal transport mechanism for noradrenaline. They are expected to facilitate the functional and biochemical characterisation of the extraneuronal noradrenaline transporter.Supported by the Deutsche Forschungsgemeinschaft (SFB 176) and the Universitätsbund Würzburg Correspondence to: H. Russ at the above address     

Effect of Coadministered Uridine on Intestinal First-Pass Metabolism of 5′-Deoxy-5-Fluorouridine in Conscious Rats—An Evaluation by Method of Portal-Systemic Concentration Difference

Purpose. The effect of uridine (UR) coadministration on the intestinal metabolism from 5-deoxy-5-fluorouridine (5-DFUR) to 5-fluorouracil (5-FU) was evaluated by a method of concentration difference between portal and systemic bloods in conscious rats (PS method). Methods. 5-DFUR (100 mg/kg) alone (Group A), or 5-DFUR + UR (100 mg/kg each) (Group B) was orally administered to conscious rats. The portal and arterial bloods were simultaneously withdrawn from two canulas at appropriate time intervals, and blood concentrations of 5-DFUR, 5-FU, UR and uracil (U) were assayed by HPLC. The concentration-time profiles of these drugs and its metabolites were analyzed by local moment analysis. Results. UR coadministration made the local absorption ratio (F_a) of 5-DFUR decrease significantly from 60.1 ± 10.5% to 38.0 ± 18.6% of dose. Though the local absorption ratios (F_a ^m) of the metabolite (5-FU) were the same between Group A and Group B (8.3 ± 1.9 and 8.7 ± 4.0% of 5-DFUR, respectively), AUC of arterial 5-FU in Group B was 5 times greater than that in Group A. UR was not detected in the portal blood, and F_a ^m of U was estimated to be 41.9 ± 26.8% of UR in Group B. Conclusions. It is predicted that a large portion of 5-FU generated from 5-DFUR is further degraded in the intestine in Group A, and U generated from UR blocks 5-FU degradation in the intestine and the systemic circulation in Group B.     

Synthesis and transformations of furan derivatives

By the reactions of 2-phenyl-4-(2-furfuryliden)-, 2-phenyl-4-(5-nitro-2-furfuryliden)-, and 2-methyl-4-(5-nitro-2-furfuryliden)-5-oxazolones with primary and secondary amines, a series of N-mono- and N,N-disubstituted amides of the corresponding-benzamido--(2-furyl)-acrylic and-benzamido- and-acetamido--(5-nitro-2-furyl)acrylic acids was synthesized. 1-Alkyl(aryl) substituted 2-phenyl-4-(5-nitro-2-furfuryliden)-5-imidazolones were synthesized from the reaction of phosphorus oxychloride and the monosubstituted amides of-benzamido--(5-nitro-2-furyl)acrylic acid.Translated from Khimiko-Farmatsevticheskii Zhurnal, No. 2, pp. 21–27, February, 1967.     

Synthesis and Study of 5′-Ester Prodrugs of N6-Cyclopentyladenosine,a Selective A1 Receptor Agonist

Purpose. A series of 5-esters of N⁶-cyclopentyladenosine (CPA) were prepared with the aim to improve stability and bioavailability of selective A₁ agonists. Log P values, stability, affinity, and activity toward human adenosine A₁ receptors were evaluated. Methods. An appropriate synthetic procedure was adopted to avoid concomitant deamination at position 6. Log P values were obtained by the Mixxor system. The stability of CPA and its 5-ester was evaluated in human plasma and whole blood and analyzed with high-performance liquid chromatography. The affinities to human A₁ receptor expressed by N⁶-cyclohexyladenosine cells were obtained by binding experiments. The activities were evaluated by measurements of the inhibition of forskolin stimulated 3-5-cyclic adenosine monophosphate, performing competitive binding assays. Results. All prodrugs were more lipophilic than CPA, and their hydrolysis, in whole blood and in plasma, was found related, respectively, to the length and hindrance of 5-substituents. Affinity and activity values indicated a very weak interaction toward adenosine A₁ receptor of the intact prodrugs. Conclusions. We propose 5-esters of CPA, characterized by suitable lipophilicity and elevated degree of stability in physiological fluids, as possible canditates for CPA prodrugs.     

Two relaxation-mediating P2-purinoceptors in guinea-pig taenia caeci

2-Methylthio ATP, noradrenaline, adenosine 5-O-(2-thiodiphosphate) (ADP\S), ,\-methylene ATP, ATP and adenosine caused relaxation of guinea-pig isolated taenia caeci precontracted by carbachol, with potency decreasing in the order indicated. 4,4-Diisothiocyanatostilbene-2,2-disulphonate (DIDS) 10, 32 and 100 M shifted the concentration-response curve of ,\-methylene ATP increasingly to the right, by the factor 141 at DIDS 100 M. Concentration-response curves of the other agonists were not shifted to the right by DIDS 100 M, except for the curve of ADP\S which was shifted by the factor 2.4. The relaxation produced by 2-methylthio ATP faded rapidly. When the fade was complete, further addition of 2-methylthio ATP or ATP did not elicit relaxation, whereas the relaxant effect of , \-methylene ATP was unchanged. The results indicate that there are at least two relaxation-mediating P₂-purinoceptors in guinea-pig taenia caeci, the P_2Y-purinoceptor which is relatively insensitive to DIDS and a distinct receptor for ,\-methylene ATP which is very sensitive to DIDS.     

Freeze-Concentration Separates Proteins and Polymer Excipients Into Different Amorphous Phases

Purpose. To study the miscibility of proteins and polymer excipients in frozen solutions and freeze-dried solids as protein formulation models. Methods. Thermal profiles of frozen solutions and freeze-dried solids containing various proteins (lysozyme, ovalbumin, BSA), nonionic polymers (Ficoll, polyvinylpyrrolidone [PVP]), and salts were analyzed by differential scanning calorimetry (DSC). The polymer miscibility was determined from the glass transition temperature of maximally freeze-concentrated solute (T_g) and the glass transition temperature of freeze-dried solid (T_g). Results. Frozen Ficoll or PVP 40k solutions showed T_g at –22°C, while protein solutions did not show an apparent T_g. All the protein and nonionic polymer combinations (5% w/w, each) were miscible in frozen solutions and presented single T_gs that rose with increases in the protein ratio. Various salts concentration-dependently lowered the single T_gs of the proteins and Ficoll combinations maintaining the mixed amorphous phase. In contrast, some salts induced the separation of the proteins and PVP combinations into protein-rich and PVP-rich phases among ice crystals. The T_gs of these polymer combinations were jump-shifted to PVP's intrinsic T_g at certain salt concentrations. Freeze-dried solids showed varied polymer miscibilities identical to those in frozen solutions. Conclusions. Freeze-concentration separates some combinations of proteins and nonionic polymers into different amorphous phases in a frozen solution. Controlling the polymer miscibility is important in designing protein formulations.     

Trennung und Bestimmung der Nucleotide des Gehirns

Ohne ZusammenfassungFolgende Abkürzungen werden in der Arbeit verwendet AMP Adenosin-5-monophosphat - ADP Adenosin-5-diphosphat - ATP Adenosin-5-triphosphat - GMP Guanosin-5-monophosphat - GDP Guanosin-5-diphosphat - GTP Guanosin-5-triphosphat - IMP Inosin-5-monophosphat - UMP Uridin-5-monophosphat - UDP Uridin-5-diphosphat - UTP Uridin-5-triphosphat - UDPAG Uridin-5-diphosphat-N-acetylglucosamin - UDPG Uridin-5-diphosphat-glucose - DPN Diphosphopyridinnucleotid - TPN Triphosphopyridinnucleotid Mit 10 TextabbildungenMit Unterstütznng der Deutschen Forschungsgemeinschaft.     

Synthesis of some aralkyldimethylhydrazine derivatives as blocking agents of adrenergic neurons

N-benzyl-N,N-dimethyl-N-acetylhydrazinium chloride, N-(o-bromobenzyl)-N,N-dimethyl-N-acetylhydrazinium bromide, and N-(o-chlorobenzyl)-N,N-dimethyl-N-acetylhydrazinium bromide, which are blocking agents for adrenergic neurones, have been synthesized. N-(o-bromobenzyl)-N,N-dimethyl-N-acetylhydrazinium bromide has the most pronounced inhibiting activity.Translated from Khimiko-Farmatsevticheskii Zhurnal, No. 6, pp. 13–15, June, 1967.