Search

Your search keyword '"Lindstrom, T. D."' showing total 42 results
Start Over Author "Lindstrom, T. D."
42 results on '"Lindstrom, T. D."'

1. The Potent BACE1 Inhibitor LY2886721 Elicits Robust Central A Pharmacodynamic Responses in Mice, Dogs, and Humans

Author

May, P. C., primary, Willis, B. A., additional, Lowe, S. L., additional, Dean, R. A., additional, Monk, S. A., additional, Cocke, P. J., additional, Audia, J. E., additional, Boggs, L. N., additional, Borders, A. R., additional, Brier, R. A., additional, Calligaro, D. O., additional, Day, T. A., additional, Ereshefsky, L., additional, Erickson, J. A., additional, Gevorkyan, H., additional, Gonzales, C. R., additional, James, D. E., additional, Jhee, S. S., additional, Komjathy, S. F., additional, Li, L., additional, Lindstrom, T. D., additional, Mathes, B. M., additional, Martenyi, F., additional, Sheehan, S. M., additional, Stout, S. L., additional, Timm, D. E., additional, Vaught, G. M., additional, Watson, B. M., additional, Winneroski, L. L., additional, Yang, Z., additional, and Mergott, D. J., additional

Published
2015
Full Text
View/download PDF

3. Robust Central Reduction of Amyloid- in Humans with an Orally Available, Non-Peptidic -Secretase Inhibitor

Author

May, P. C., primary, Dean, R. A., additional, Lowe, S. L., additional, Martenyi, F., additional, Sheehan, S. M., additional, Boggs, L. N., additional, Monk, S. A., additional, Mathes, B. M., additional, Mergott, D. J., additional, Watson, B. M., additional, Stout, S. L., additional, Timm, D. E., additional, Smith LaBell, E., additional, Gonzales, C. R., additional, Nakano, M., additional, Jhee, S. S., additional, Yen, M., additional, Ereshefsky, L., additional, Lindstrom, T. D., additional, Calligaro, D. O., additional, Cocke, P. J., additional, Greg Hall, D., additional, Friedrich, S., additional, Citron, M., additional, and Audia, J. E., additional

Published
2011
Full Text
View/download PDF

7. ChemInform Abstract: Synthesis and Biological Evaluation of a Series of Parenteral 3′‐Quaternary Ammonium Cephalosporins.

Author

BROWN, R. F., primary, KINNICK, M. D., additional, MORIN, J. M. JUN., additional, VASILEFF, R. T., additional, COUNTER, F. T., additional, DAVIDSON, E. O., additional, ENSMINGER, P. W., additional, EUDALY, J. A., additional, KASHER, J. S., additional, KATNER, A. S., additional, KOEHLER, R. E., additional, KURZ, K. D., additional, LINDSTROM, T. D., additional, LUNN, W. H. W., additional, PRESTON, D. A., additional, OTT, J. L., additional, QUAY, J. F., additional, SHADLE, J. K., additional, STEINBERG, M. I., additional, STUCKY, J. F., additional, SWARTZENDRUBER, J. K., additional, TURNER, J. R., additional, WEBBER, J. A., additional, WRIGHT, W. E., additional, and ZIMMERMAN, K. M., additional

Published
1991
Full Text
View/download PDF

10. Substituted 3-Imidazo[1,2-a]pyridin-3-yl- 4-(1,2,3,4-tetrahydro-[1,4]diazepino- [6,7,1-hi]indol-7-yl)pyrrole-2,5-diones as Highly Selective and Potent Inhibitors of Glycogen Synthase Kinase-3

Author

Engler, T. A., Henry, J. R., Malhotra, S., Cunningham, B., Furness, K., Brozinick, J., Burkholder, T. P., Clay, M. P., Clayton, J., Diefenbacher, C., Hawkins, E., Iversen, P. W., Li, Y., Lindstrom, T. D., Marquart, A. L., McLean, J., Mendel, D., Misener, E., Briere, D., O'Toole, J. C., Porter, W. J., Queener, S., Reel, J. K., Owens, R. A., Brier, R. A., Eessalu, T. E., Wagner, J. R., Campbell, R. M., and Vaughn, R.

Abstract

Glycogen synthase kinase-3 (GSK3) is involved in signaling from the insulin receptor. Inhibitors of GSK3 are expected to effect lowering of plasma glucose similar to insulin, making GSK3 an attractive target for the treatment of type 2 diabetes. Herein we report the discovery of a series of potent and selective GSK3 inhibitors. Compounds 712 show oral activity in an in vivo model of type II diabetes, and 9 and 12 have desirable PK properties.

Published
2004

11. Synthesis and Structure−Activity Relationships of Novel Arylpiperazines as Potent and Selective Agonists of the Melanocortin Subtype-4 Receptor

Author

Richardson, T. I., Ornstein, P. L., Briner, K., Fisher, M. J., Backer, R. T., Biggers, C. K., Clay, M. P., Emmerson, P. J., Hertel, L. W., Hsiung, H. M., Husain, S., Kahl, S. D., Lee, J. A., Lindstrom, T. D., Martinelli, M. J., Mayer, J. P., Mullaney, J. T., O'Brien, T. P., Pawlak, J. M., Revell, K. D., Shah, J., Zgombick, J. M., Herr, R. J., Melekhov, A., Sampson, P. B., and King, C.-H. R.

Abstract

The melanocortin receptors have been implicated as potential targets for a number of important therapeutic indications, including inflammation, sexual dysfunction, and obesity. We identified compound 1, an arylpiperazine attached to the dipeptide H-d-Tic-d-p-Cl-Phe-OH, as a novel melanocortin subtype-4 receptor (MC4R) agonist through iterative directed screening of nonpeptidyl G-protein-coupled receptor biased libraries. Structure−activity relationship (SAR) studies demonstrated that substitutions at the ortho position of the aryl ring improved binding and functional potency. For example, the o-isopropyl-substituted compound 29 (Ki = 720 nM) possessed 9-fold better binding affinity compared to the unsubstituted aryl ring (Ki = 6600 nM). Sulfonamide 39 (Ki = 220 nM) fills this space with a polar substituent, resulting in a further 2-fold improvement in binding affinity. The most potent compounds such as the diethylamine 44 (Ki = 60 nM) contain a basic group at this position. Basic heterocycles such as the imidazole 50 (Ki = 110 nM) were similarly effective. We also demonstrated good oral bioavailability for sulfonamide 39.

Published
2004

12. Fused Bicyclic Gly-Asp β-Turn Mimics with Specific Affinity for GPIIb-IIIa

Author

Fisher, M. J., Arfstan, A. E., Giese, U., Gunn, B. P., Harms, C. S., Khau, V., Kinnick, M. D., Lindstrom, T. D., Martinelli, M. J., Mest, H.-J., Mohr, M., Morin, J. M., Jr., Mullaney, J. T., Nunes, A., Paal, M., Rapp, A., Ruhter, G., Ruterbories, K. J., Sall, D. J., Scarborough, R. M., Schotten, T., Sommer, B., Stenzel, W., Towner, R. D., Um, S. L., Utterback, B. G., Vasileff, R. T., Voelkers, S., Wyss, V. L., and Jakubowski, J. A.

Abstract

Disubstituted isoquinolones 2 and 3 have affinity for GPIIb-IIIa and represent leads for further structural evaluation. Structure−activity studies centered on the bicyclic β-turn mimic contained in these molecules indicated that this moiety could accommodate a variety of modifications. Specifically, monocyclic, 6,5-bicyclic, and 6,7-bicyclic structures provide compounds with affinity for GPIIb-IIIa. Within the 6,6-series, isoquinoline, tetralin, tetralone, and benzopyran nuclei yield potent antagonists that are specific for GPIIb-IIIa. Attachment of the arginine isostere (benzamidine) to the supporting nucleus can be accomplished with an ether or amide linkage, although the latter enhances activity. Several compounds in this series provided measurable blood levels after oral dosing. Conversion of the acid moiety in these molecules to an ester generally provided compounds which gave greater systemic exposure after oral administration. Absolute bioavailabilities in the rat for the ethyl ester prodrug derivatives of the tetralin, tetralone, and benzopyran analogues of 3 were 28%, 23%, and 24%, respectively.

Published
1999

13. Effects of hepatic ischemia-reperfusion injury on the hepatic mixed function oxidase system in rats.

Author

Lindstrom, T D, Hanssen, B R, and Bendele, A M

Abstract

Hepatic ischemia induced in vivo by ligation of the left hepatic lobe of rats for up to 2 hr had no effect on cytochrome P-450, cytochrome c reductase, or lobe histology; however, cytochrome b5 increased with ischemia duration. Ethylmorphine demethylation decreased 35% after 2 hr of ischemia. Reperfusion of tissue previously made ischemic for up to 2 hr was associated with appreciable necrosis as well as decreases in cytochrome P-450, cytochrome b5, cytochrome c reductase, and ethylmorphine demethylation. Serum alanine transaminase and aspartate transaminase concentrations were increased by reperfusion of previously ischemic tissue. Reperfusion of the previously ischemic lobe for 18 hr was associated with a greater loss of cytochromes P-450 and b5, cytochrome c reductase, and ethylmorphine demethylation than reperfusion for 1 hr. The total decrease in cytochrome P-450 and b5 content was equal to the decrease in total microsomal heme content, although cytochrome P-450 decreased more than cytochrome b5. Ethoxyresorufin deethylation by hepatic microsomes from 3-methylcholanthrene-treated rats was decreased by ischemia-reperfusion; however, pentoxyresorufin dealkylation by hepatic microsomes from phenobarbital-treated rats was not, suggesting specific cytochrome P-450 isozyme loss. In vitro NADPH-dependent lipid peroxidation in hepatic microsomes from control and phenobarbital- and 3-methylcholanthrene-treated rats resulted in a selective decrease of ethoxyresorufin but not pentoxyresorufin dealkylation, similar to that observed in livers subjected to ischemia-reperfusion in vivo. These data suggest that cytochrome P-450, ethylmorphine demethylation, and ethoxyresorufin deethylation are more susceptible to ischemia-reperfusion injury than cytochrome b5 or pentoxyresorufin dealkylation.

Published
1990

14. Correlation between the disposition of [14C]clofilium and its cardiac electrophysiological effect.

Author

Lindstrom, T D, Murphy, P J, Smallwood, J K, Wiest, S A, and Steinberg, M I

Abstract

The disposition of [14C]clofilium was studied in rats and dogs and related to the electrophysiological effects observed in isolated canine Purkinje fibers. Ten percent of the dose of [14C] clofilium administered to rats and dogs i.v. was excreted in the urine within 72 hr, whereas 55% was excreted in the feces during the same period in both species. In rats, biliary excretion accounted for 35% of the dose within 48 hr. Plasma levels of radioactivity rapidly decline in rats and dogs administered 5 mg/kg of [14C]clofilium characterized by a plasma radioactivity half-life for the elimination phase of 2.5 to 3 hr. In contrast, tissue levels of radioactivity were persistent; the half-life of radioactivity in the rat heart was 5 days and 14 days in the dog heart. Twenty-four hours after an i.v. dose of clofilium (0.044-1.3 mg/kg) to dogs, the action potential duration of isolated Purkinje fibers was prolonged in a dose-dependent manner. The half-life of the effect of clofilium on action potential duration as 10 days which is in agreement with the persistence of radioactivity in tissues. The data suggest that [14C]clofilium and/or metabolites concentrate in the heart and that plasma levels of radioactivity may not be an accurate index of cardiac levels or biological response.

Published
1982

15. Correlation of anti-inflammatory activity with peak tissue rather than peak plasma levels of BF389.

Author

Bendele, A M, Ruterbories, K J, Spaethe, S M, Benslay, D N, Lindstrom, T D, Lee, S J, and Naismith, R W

Abstract

BF389 (Biofor 389) is a potent anti-inflammatory agent in various animal models including adjuvant and type II collagen arthritis in rats. In vitro assays indicate that this compound is a mixed inhibitor of arachidonic acid metabolism. The compound was evaluated for effects on the acute inflammatory response in the carrageenan paw edema assay in rats using a standard protocol in which the animals were given single or multiple (daily for 5 days) p.o. doses of the compound. Carrageenan was injected into the footpad of each animal 1 hr after dosing and volumes of both hind paws were determined 3 hr later. Basal serum prostaglandin (PG) E2 levels and PGE2 levels in arachidonate-stimulated blood from these same animals also were measured. No anti-inflammatory activity was observed in BF389-treated rats despite the occurrence of profound suppression of basal and stimulated PGE2 production. Animals treated with conventional nonsteroidal anti-inflammatory drugs in this assay had both suppressed PGE2 production and significant anti-inflammatory activity. In another study, groups of rats were given p.o. doses of 1, 10, 100 or 250 mg/kg of BF389 for 5 days in order to determine peak concentrations, T1/2s and total areas under the plasma (tissue) drug concentration curves in plasma and paws. Peak plasma concentrations occurred 2 to 4 hr postdosing and the half-life was 8 to 15 hr over the 1- to 250-mg/kg/day dose range. Peak paw concentrations occurred 6 to 12 hr postdosing and the levels were 9- to 14-fold greater in the paw than in the plasma.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1992

16. Anti-inflammatory activity of BF389, a Di-T-butylphenol, in animal models of arthritis.

Author

Bendele, A M, Benslay, D N, Hom, J T, Spaethe, S M, Ruterbories, K J, Lindstrom, T D, Lee, S J, and Naismith, R W

Abstract

Biofor 389 (BF389), dihydro-4-[[3,5-bis(1,1-dimethyl)-4-hydroxyphenyl] methylene]-2-methyl-2H-1,2-oxazin-3(4H)-one, was tested for anti-inflammatory activity in various animal models of arthritis. Initial evaluation in the lipoidalamine (LA) arthritis model in rats (5-day dosing protocol) resulted in an oral ED50 of 4.9 mg/kg for inhibition of paw swelling. No effects on splenomegaly were observed, suggesting that the compound was efficacious as a result of anti-inflammatory rather than immunomodulatory effects. BF389 was efficacious in interleukin 1 (IL-1)-enhanced type II collagen arthritis in rats (oral ED50 less than 1.0 mg/kg) as assessed by paw volume measurement and histologic evaluation of joints. Mice with IL-1-enhanced type II collagen arthritis given 30 mg/kg of BF 389 had significantly lower histological scores for joint damage than did untreated controls. Normal rats given single oral doses of BF389 had significant suppression of arachidonate-stimulated whole blood prostaglandin E2 and thromboxane B2 production 2 hr postdosing (ED50 = 0.1 mg/kg). Leukotriene B4 production in these animals was not decreased. After it became apparent that the compound was a potent inhibitor of prostaglandin production in vivo, a study was done to compare the efficacy and toxicity of BF389 with several currently marketed nonsteroidal anti-inflammatory drugs, piroxicam, naproxen and diclofenac. Lipoidalamine-injected rats were given daily oral doses of BF389 or the comparators for 21 days. Quantitation of effects on arthritis on day 21 resulted in ED50 values of 0.9 mg/kg (BF389), 3.9 mg/kg (naproxen), 4.9 mg/kg (diclofenac) and 0.6 mg/kg (piroxicam).(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1992

17. Pharmacokinetics and disposition of the KS1/4 monoclonal antibody-desacetylvinblastine hydrazide conjugate LY203725 in rats and monkeys.

Author

Lindstrom, T D, Althaus, W A, Ruterbories, K J, and Kau, D

Abstract

The plasma pharmacokinetics of the monoclonal antibody-vinca conjugate KS 1/4-desacetylvinblastine hydrazide (DAVLB-hyd; [3H]LY203725) have been evaluated in rats (17 mg/kg) and monkeys (15 mg/kg) after i.v. dosing. Plasma concentrations of radioactivity 1 hr after dosing were higher in monkeys than in rats. The biphasic elimination of radioactivity in rats was characterized by half-lives (T1/2) of 10 and 143 hr, whereas the elimination of radioactivity in monkeys was characterized by T1/2 values of 11 and 66 hr. Plasma total antibody and radioactivity concentrations were similar within 6 (rat) and 24 (monkey) hr after dosing; however, total antibody concentrations were greater than radioactivity concentrations thereafter, indicating the presence of free antibody in the plasma. Plasma elimination T1/2 values and areas under the curve of total antibody in rats and monkeys were greater than those of radioactivity. The presence of free antibody implies the presence of free DAVLB-hyd; however, plasma concentrations of free DAVLB-hyd were at least 3 orders of magnitude less than those of radioactivity in both species. The T1/2 of free DAVLB-hyd in plasma of LY203725 dosed monkeys was 16 hr. Hydrolysis of the conjugate to yield free DAVLB-hyd was observed upon incubation of conjugate with rat plasma in vitro. Administration of DAVLB-hyd to rats resulted in a rapid initial decrease in plasma DAVLB-hyd followed by a slower (T1/2 = 1.4 hr) elimination rate. Fecal excretion was the predominant mode of elimination of radioactivity in both rats and monkeys dosed with [3H]LY203725.

Published
1990

22. Fused bicyclic Gly-Asp beta-turn mimics with potent affinity for GPIIb-IIIa. Exploration of the arginine isostere.

Author

Fisher MJ, Giese U, Harms CS, Kinnick MD, Lindstrom TD, McCowan JR, Mest HJ, Morin JM Jr, Mullaney JT, Paal M, Rapp A, Rühter G, Ruterbories KJ, Sall DJ, Scarborough RM, Schotten T, Stenzel W, Towner RD, Um SL, Utterback BG, Wyss VL, and Jakubowski JA

Subjects
Adenosine Diphosphate pharmacology, Animals, Arginine chemistry, Benzamidines chemistry, Biological Availability, Drug Evaluation, Enzyme-Linked Immunosorbent Assay, Fibrinogen metabolism, Humans, Inhibitory Concentration 50, Models, Molecular, Platelet Aggregation drug effects, Platelet Glycoprotein GPIIb-IIIa Complex metabolism, Prodrugs chemical synthesis, Prodrugs chemistry, Prodrugs pharmacokinetics, Protein Binding drug effects, Protein Structure, Secondary, Rats, Stereoisomerism, Acetates metabolism, Amidines metabolism, Platelet Glycoprotein GPIIb-IIIa Complex antagonists & inhibitors, Tetralones
Abstract

6-[4-Amidinobenzoyl]amino]-tetralone-2-acetic acid is a potent antagonist of GPIIb-IIIa. Substitution in the meta position of the benzamidine, or replacement with a heteroaryl amidine was tolerated in this series. Use of an acyl-linked 4-alkyl piperidine as an arginine isostere also provided active compounds. Compounds from this series provided substantial systemic exposure in the rat following oral administration.

Published
2000
Full Text
View/download PDF

23. Fused bicyclic Gly-Asp beta-turn mimics with specific affinity for GPIIb-IIIa.

Author

Fisher MJ, Arfstan AE, Giese U, Gunn BP, Harms CS, Khau V, Kinnick MD, Lindstrom TD, Martinelli MJ, Mest HJ, Mohr M, Morin JM Jr, Mullaney JT, Nunes A, Paal M, Rapp A, Rühter G, Ruterbories KJ, Sall DJ, Scarborough RM, Schotten T, Sommer B, Stenzel W, Towner RD, and Um SL

Subjects
Administration, Oral, Animals, Benzopyrans chemistry, Benzopyrans pharmacokinetics, Benzopyrans pharmacology, Binding, Competitive, Biological Availability, Enzyme-Linked Immunosorbent Assay, Guinea Pigs, Humans, Isoquinolines chemistry, Isoquinolines pharmacokinetics, Isoquinolines pharmacology, Molecular Mimicry, Platelet Aggregation drug effects, Platelet Glycoprotein GPIIb-IIIa Complex antagonists & inhibitors, Protein Structure, Secondary, Rats, Structure-Activity Relationship, Tetrahydronaphthalenes chemistry, Tetrahydronaphthalenes pharmacokinetics, Tetrahydronaphthalenes pharmacology, Benzopyrans chemical synthesis, Isoquinolines chemical synthesis, Oligopeptides chemistry, Platelet Glycoprotein GPIIb-IIIa Complex metabolism, Tetrahydronaphthalenes chemical synthesis
Abstract

Disubstituted isoquinolones 2 and 3 have affinity for GPIIb-IIIa and represent leads for further structural evaluation. Structure-activity studies centered on the bicyclic beta-turn mimic contained in these molecules indicated that this moiety could accommodate a variety of modifications. Specifically, monocyclic, 6, 5-bicyclic, and 6,7-bicyclic structures provide compounds with affinity for GPIIb-IIIa. Within the 6,6-series, isoquinoline, tetralin, tetralone, and benzopyran nuclei yield potent antagonists that are specific for GPIIb-IIIa. Attachment of the arginine isostere (benzamidine) to the supporting nucleus can be accomplished with an ether or amide linkage, although the latter enhances activity. Several compounds in this series provided measurable blood levels after oral dosing. Conversion of the acid moiety in these molecules to an ester generally provided compounds which gave greater systemic exposure after oral administration. Absolute bioavailabilities in the rat for the ethyl ester prodrug derivatives of the tetralin, tetralone, and benzopyran analogues of 3 were 28%, 23%, and 24%, respectively.

Published
1999
Full Text
View/download PDF

24. Application of oral bioavailability surrogates in the design of orally active inhibitors of rhinovirus replication.

Author

Stratford RE Jr, Clay MP, Heinz BA, Kuhfeld MT, Osborne SJ, Phillips DL, Sweetana SA, Tebbe MJ, Vasudevan V, Zornes LL, and Lindstrom TD

Subjects
Animals, Antiviral Agents pharmacology, Benzimidazoles chemical synthesis, Benzimidazoles pharmacology, Biological Availability, Caco-2 Cells, Chemical Phenomena, Chemistry, Physical, Humans, Hydrogen-Ion Concentration, Male, Microsomes drug effects, Pharmaceutical Solutions, Rats, Rats, Inbred F344, Solubility, Antiviral Agents administration & dosage, Antiviral Agents pharmacokinetics, Benzimidazoles pharmacokinetics, Rhinovirus drug effects, Virus Replication drug effects
Abstract

Previous studies in rats and humans demonstrated poor oral bioavailability of potent in vitro 2-aminobenzimidazole inhibitors of rhinovirus replication due to significant first-pass elimination and possibly also to poor aqueous solubility. Estimations of aqueous solubility, as well as measurements of caco-2 permeability and NADPH dependent compound loss in rat liver microsomal incubations were employed alongside traditional in vivo experiments in rats to guide subsequent chemistry efforts. Retention of activity upon replacement of the metabolically labile vinyl oxime in the lead molecule with a vinyl carboxamide was a major breakthrough; however, oral bioavailability among the latter compounds was variable. Based on the ability to independently measure solubility, permeability, and metabolic stability of new compounds, variable solubility across the series (ranging from approximately 1 to 10 microg/mL) was identified as the cause of the inconsistent performance. Subsequent efforts to improve solubility led to the discovery of highly soluble (>10 mg/mL) and potent dessulfonyl vinyl carboxamide benzimidazoles. Determination of the metabolic stability of these compounds as a surrogate of the extent of their first-pass elimination supported a prediction of excellent oral bioavailability. In comparison to the sulfonyl-containing vinyl carboxamides, caco-2 permeabilities were reduced 5 to 10-fold; however, these were considered to be in the range of well-absorbed compounds based on comparison to a series of reference compounds of known percentage absorption in humans. Subsequent experiments in the rat verified the oral bioavailability of these N-alkyl compounds, with one compound (368177) having an absolute oral bioavailability of 89.4%. The application of solubility and caco-2 permeability as surrogates for oral absorption potential, in conjunction with the use of microsomal incubations as a surrogate for first-pass metabolism, was shown to augment a rational chemistry approach to discover orally bioavailable inhibitors of rhinovirus replication. Future expanded use of these surrogates is planned.

Published
1999
Full Text
View/download PDF

25. Stereoselective metabolism of tazofelone, an anti-inflammatory bowel disease agent, in rats and dogs and in human liver microsomes.

Author

Clay MP, Hanssen BR, Surapaneni SS, and Lindstrom TD

Subjects
Administration, Oral, Animals, Area Under Curve, Blood Proteins metabolism, Dogs, Female, Half-Life, Humans, In Vitro Techniques, Injections, Intravenous, Male, Phenols chemistry, Protein Binding, Rats, Rats, Inbred F344, Stereoisomerism, Sulfoxides metabolism, Thiazoles chemistry, Thiazolidines, Inflammatory Bowel Diseases drug therapy, Microsomes, Liver metabolism, Phenols metabolism, Thiazoles metabolism
Abstract

Incubation of (R)-tazofelone and (S)-tazofelone in rat, dog, and human liver microsomes demonstrated that the (R)-tazofelone enantiomer was more rapidly metabolized, with two diastereomeric sulfoxides as the major metabolites formed in all three species. The two diasteresomers epimerized at physiological pH, therefore total sulfoxide formation rates were measured. The formation of the total sulfoxide metabolites followed Michaelis-Menten kinetics. The K(m), Vmax, and intrinsic formation clearance (Vmax/K(m)) values were determined in rat, dog, and human liver microsomes. The intrinsic formation clearance of sulfoxide from (R)-tazofelone exceeded that of (S)-tazofelone in all three species. In vivo studies in rats and dogs dosed orally and intravenously confirmed the stereoselective metabolism of tazofelone observed in vitro. Plasma concentrations of (S)-tazofelone exceeded (R)-tazofelone in rats and dogs by a factor of 3 to 4. In rat portal plasma, both enantiomers were of approximately equal concentration after oral dosing, indicating similar absorption. The half-lives of tazofelone and total sulfoxides in rats were 3.5 and 2.8 h, respectively. In dogs, the half-lives of tazofelone and total sulfoxides were 2.2 and 5.5 h, respectively. Plasma clearance was 2.3 l/h in rats and 1.4 l/h in dogs, and the volumes of distribution were 12 and 4.5 l, respectively, in rats and dogs. Both enantiomers were highly bound to plasma proteins to a similar extent in both species.

Published
1999
Full Text
View/download PDF

26. In vitro biotransformation and identification of human cytochrome P450 isozyme-dependent metabolism of tazofelone.

Author

Surapaneni SS, Clay MP, Spangle LA, Paschal JW, and Lindstrom TD

Subjects
Biological Availability, Biotransformation, Humans, Inactivation, Metabolic, Isoenzymes analysis, Kinetics, Microsomes, Liver enzymology, Microsomes, Liver metabolism, Thiazolidines, Anti-Inflammatory Agents, Non-Steroidal metabolism, Cytochrome P-450 Enzyme System metabolism, Isoenzymes metabolism, Phenols metabolism, Thiazoles metabolism
Abstract

Tazofelone is a new inflammatory bowel disease agent. The biotransformation of tazofelone in human livers and the cytochrome P450 responsible for the biotransformation has been studied. Two metabolites of tazofelone were formed in vitro. A sulfoxide metabolite was identified by cochromatography with authentic standards, and a quinol metabolite of tazofelone was identified by mass spectrometry and proton NMR. Sulfoxidation was catalyzed by a single enzyme system while formation of the quinol metabolite was catalyzed by a two enzyme system. The Km and Vmax values for sulfoxidation were 12.4 microM and 0.27 nmol/min/mg protein, respectively. The high affinity Km and Vmax values for the formation of the quinol metabolite were 7.5 microM and 0.17 nmol/min/mg protein, respectively. Tazofelone was incubated at 20 microM concentration with human microsomes to determine which of the cytochrome P450 isozyme(s) is involved in the oxidation of tazofelone. A strong correlation was found between the immunoquantified concentrations of CYP3A and the rates of formation of the sulfoxide and quinol metabolites of tazofelone. Similarly, significant correlations were observed between the formation of midazolam 1'-hydroxylation and the rates of formation of both metabolites of tazofelone. Inhibition studies have indicated that triacetyloleandomycin, a CYP3A specific inhibitor, almost completely inhibited the formation of both of these tazofelone metabolites. Incubations with specific cDNA expressed microsomes indicated that the formation of both the sulfoxide and quinol metabolites was highest with CYP3A4 containing microsomes. The correlation data was confirmed by inhibition studies and cDNA expressed cytochrome P450 systems demonstrating that the biotransformation of tazofelone to its metabolites is primarily mediated by CYP3A.

Published
1997

27. Benzylamine antioxidants: relationship between structure, peroxyl radical scavenging, lipid peroxidation inhibition, and cytoprotection.

Author

Yu MJ, McCowan JR, Phebus LA, Towner RD, Ho PP, Keith PT, Luttman CA, Saunders RD, Ruterbories KJ, and Lindstrom TD

Subjects
Animals, Antioxidants pharmacology, Benzylamines pharmacology, Blood Pressure drug effects, Brain metabolism, Hippocampus drug effects, Hydrogen Peroxide pharmacology, Iron pharmacology, Male, Membrane Lipids metabolism, Neurons drug effects, Peroxides, Rabbits, Rats, Rats, Sprague-Dawley, Structure-Activity Relationship, Antioxidants chemical synthesis, Benzylamines chemical synthesis, Free Radical Scavengers, Lipid Peroxidation drug effects
Abstract

Three homologous series of 3,5-dialkoxy-4-hydroxybenzylamines were prepared and tested (1) as peroxyl radical scavengers in homogeneous aqueous solution, (2) as inhibitors of iron-dependent peroxidation of rabbit brain vesicular membrane lipids, and (3) as cytoprotective agents using primary cultures of rat hippocampal neurons exposed to hydrogen peroxide. The structural requirements for efficient radical trapping in homogeneous solution differed from those for effective lipid peroxidation inhibition: In homogeneous solution a kinetic preference existed for smaller, less sterically encumbered substituents flanking the reactive phenolic hydroxyl group. Lipid peroxidation inhibition, on the other hand, required longer more lipophilic substituents. Consequently, a lipophilic alkoxyl substituent at C3 and a small substituent at C5 appeared optimal for efficient radical scavenging activity in both lipid and homogeneous solution. Maximal cytoprotection of rat hippocampal neurons exposed to hydrogen peroxide was also associated with more lipophilic derivatives although substituent length and substituent bulk may represent independent parameters for relating structure and efficacy in this system.

Published
1993
Full Text
View/download PDF

28. Inhibition of granulocyte cAMP-phosphodiesterase by rolipram in vivo is not sufficient to protect the canine myocardium from reperfusion injury.

Author

Simpson PJ, Schelm JA, Smallwood JK, Clay MP, and Lindstrom TD

Subjects
Animals, Blood Pressure drug effects, Coronary Circulation drug effects, Dogs, Heart Rate drug effects, Leukocyte Count, Male, Myocardial Infarction physiopathology, Myocardial Reperfusion Injury physiopathology, Neutrophils drug effects, Neutrophils enzymology, Peroxidase metabolism, Pyrrolidinones blood, Rolipram, Superoxides metabolism, Ventricular Fibrillation physiopathology, 3',5'-Cyclic-AMP Phosphodiesterases antagonists & inhibitors, Granulocytes enzymology, Myocardial Reperfusion Injury prevention & control, Pyrrolidinones pharmacology
Abstract

The purpose of this study was to determine whether the selective type IV cAMP-phosphodiesterase inhibitor rolipram could reduce the reperfusion injury that occurs during myocardial infarction in the anesthetized dog. This question was tested in pentobarbital-anesthetized dogs subject to 90 min of regional myocardial ischemia and 5 h of reperfusion. Dogs were treated with 1 mg/kg of rolipram (i.v., 15 min before reperfusion) followed by a 1 mg/kg/h infusion over the duration of the 5 h of reperfusion. Rolipram was tested in vitro for efficacy in inhibition of isolated human neutrophil superoxide generation. Rolipram produced significant inhibition of superoxide production over the concentration range of 0.1-100 microM rolipram when neutrophils were stimulated with a 10(-7) M concentration of the chemotactic peptide f-Met-Leu-Phe. Rolipram significantly inhibited superoxide generation from human and canine granulocytes in whole blood stimulated by zymosan. Therapeutic concentrations of rolipram in the blood of dogs were achieved during the course of the experiments with a plasma concentration of 0.761 +/- 0.095 micrograms/ml (2.76 +/- 0.34 microM) at the time of reperfusion, and 0.574 +/- 0.098 micrograms/ml (2.08 +/- 0.36 microM) at the end of the reperfusion period. The relative severity of myocardial ischemia between the two treatment groups was similar as assessed with radiolabeled microsphere measurement of myocardial blood flow. Transmural myocardial blood flows were not significantly different between the two groups after coronary occlusion (control, 0.05 +/- 0.01 ml/min/g, n = 6, vs. rolipram, 0.18 +/- 0.07 ml/min/g, n = 6; p = 0.48).(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1992
Full Text
View/download PDF

29. Pharmacokinetics of a novel butylated hydroxytoluene-thiazolidinone CNS antiischemic agent LY256548 in rats, mice, dogs, and monkeys.

Author

Ruterbories KJ and Lindstrom TD

Subjects
Administration, Oral, Animals, Anti-Inflammatory Agents, Non-Steroidal urine, Dogs, Feces chemistry, Female, Half-Life, Infusions, Intravenous, Macaca mulatta, Male, Mice, Rats, Rats, Inbred F344, Species Specificity, Thiazoles urine, Thiazolidines, Tissue Distribution, Anti-Inflammatory Agents, Non-Steroidal pharmacokinetics, Thiazoles pharmacokinetics
Abstract

Mice, rats, dogs, and monkeys were given a single 50 mg/kg oral dose of [14C]LY256548. Plasma levels of radioactivity and LY256548 were determined, as was the excretion of radioactivity. Peak plasma levels of LY256548 occurred prior to those of radioactivity in mice, dogs, and monkeys, but were coincident in rats. The Cmax of LY256548 in rats, mice, dogs, and monkeys was 0.17, 0.30, 0.04, and 0.02 microgram/ml, respectively. However, the Cmax of radioactivity was 10-fold greater than that of LY256548 in rats and mice, 24-fold greater in dogs, and 40-fold greater in monkeys. The half-lives of LY256548 were substantially less than those of radioactivity in all four species. The oral absorption of LY256548 in rats, dogs, and monkeys was 45%, 7%, and 12%, respectively. The systemic bioavailability of LY256548 in rats, dogs, and monkeys was 6%, 0.4%, and 3%, respectively. Extensive biotransformation of LY256548 was observed in all four species. Fecal excretion of radioactivity was the primary mode of elimination, being 95% in rats, 81% in mice, 100% in dogs, and 68% in monkeys.

Published
1990

30. Alpha, beta-ketoalkene reduction. A novel reduction pathway in mammalian tissues.

Author

Lindstrom TD and Whitaker GW

Subjects
Alkenes metabolism, Animals, Cricetinae, Guinea Pigs, Hydrogen-Ion Concentration, Liver enzymology, Liver metabolism, Male, Oxidation-Reduction, Oxidoreductases analysis, Rabbits, Rats, Rats, Inbred Strains, Benzofurans metabolism, Oxidoreductases metabolism
Abstract

Reduction of an alpha, beta-unsaturated ketone to the corresponding saturated ketone in a 2-benzylidene-3-ketocoumaran derivative has been characterized with respect to subcellular and tissue distribution, species specificity, cofactor requirements, kinetic constants, and effects of inhibitors. In rats, the highest activity was found in the hepatic cytosolic (100,000g supernatant) fraction having an apparent substrate Km and Vmax of 5.6 microM and 1.3 nmol/min/mg protein, respectively. In rat hepatic cytosolic incubations, NADPH supported the reduction reaction having an apparent Km of 15 microM while NADH was 70% less effective in catalyzing the reaction than NADPH. The most effective inhibitors of the reaction were potassium cyanide and sulfhydryl reagents such as p-chloromercuribenzoic acid and iodoacetamide. Glutathione, dithiothreitol, and flavin mononucleotide were without consequential effect. Phenobarbital did not induce the activity in rats. Guinea pig hepatic cytosol was approximately 8 times more active than rat hepatic cytosol in catalyzing the reduction reaction. In rats, whole blood catalyzed the reduction of the substrate in the absence of added NADPH. Hemolysis resulted in a loss of activity which could be restored by addition of NADPH. Cinnamic acid was not reduced by the rat cytosolic fraction. The enzyme utilizes the A-side hydrogen atom at C-4 of NADPH.

Published
1984

31. Metabolism of the antiarrhythmic agent, indecainide, in rats, dogs, and monkeys.

Author

Lindstrom TD, Lacefield WB, and Whitaker GW

Subjects
Animals, Chromatography, Dogs, Female, Fluorenes blood, Fluorenes urine, Macaca mulatta, Male, Rats, Rats, Inbred Strains, Anti-Arrhythmia Agents metabolism, Fluorenes metabolism
Abstract

The biotransformation of indecainide, a potent new antiarrhythmic agent, has been studied in rats and dogs. Indecainide was excreted in the urine primarily as the unchanged compound. The major urinary metabolite was desisopropyl indecainide which accounted for approximately 5% of the urinary radioactivity in both species. This metabolite was also detected in the plasma of rats, dogs, and monkeys. Peak plasma levels of the amine metabolite were 15 and 19% of the peak plasma levels of indecainide in rats and dogs, respectively. Loss of isopropylamine resulted in the formation of an aldehyde intermediate which was stabilized as the cyclic acylaminocarbinol. An acidic metabolite presumably derived from oxidation of the aldehyde was detected as well as a cyclic imide metabolite. An additional minor metabolite corresponding to N-formyl indecainide was observed in the urine but the mechanism of its formation is unknown.

Published
1984

32. Saturation of an alpha, beta-unsaturated ketone: a novel xenobiotic biotransformation in mammals.

Author

Lindstrom TD and Whitaker GW

Subjects
Animals, Biotransformation, Cricetinae, Cytosol enzymology, Guinea Pigs, Humans, Kidney enzymology, Liver enzymology, Lung enzymology, Male, Mesocricetus, Mice, Muscles enzymology, NADP pharmacology, Oxidoreductases blood, Oxidoreductases metabolism, Rabbits, Rats, Benzofurans metabolism, Mammals metabolism
Abstract

Reduction of an alpha, beta-unsaturated ketone to the corresponding saturated ketone in a 2-benzylidene-3-ketocoumaran derivative has been investigated. Reductase activity resides in the cytosolic fraction of liver, lung and kidney. Rat and human blood also contain significant reductase activity. Hepatic reductase activity was high in guinea-pigs followed by hamsters, rabbits, rats and mice. The substrate had an apparent Km and Vmax of 5.6 microM and 1.3 nmol/min per mg protein, respectively. The reduction was dependent upon NADPH having an apparent Km of 14.8 microM and a Vmax of 1.0 nmol/min per mg protein. Only the A side hydrogen of NADPH was incorporated into the reduced product. The reaction was inhibited by cyanide, and sulphydryl reagents. Phenobarbital did not induce the activity in rats.

Published
1984
Full Text
View/download PDF

33. Determination of clofilium, a new antifibrillatory agent, in plasma by gas chromatography--mass spectrometry.

Author

Lindstrom TD and Wolen RL

Subjects
Animals, Dogs, Gas Chromatography-Mass Spectrometry, Time Factors, Anti-Arrhythmia Agents blood, Quaternary Ammonium Compounds blood
Abstract

A sensitive and selective method for the assay of the new quaternary amine antifibrillatory agent clofilium is described. Plasma samples were extracted with dichloromethane (98.5 +/- 0.2% recovery) and analyzed by gas chromatography--mass spectrometry operating in the electron-impact mode. The method involves a Hofmann elimination of an N-alkyl radical from clofilium and the internal standard in the presence of a strong nucleophile in the injector of the gas chromatograph. The resulting tertiary amines are chromatographed and detected by selective ion monitoring. The ratio of the clofilium base peak (m/z 224) to the internal standard peak (m/z 210) was linear relative to the plasma clofilium concentration over the range of 25-1000 ng/ml plasma.

Published
1982
Full Text
View/download PDF

34. Disposition and biotransformation of quinpirole, a new D-2 dopamine agonist antihypertensive agent, in mice, rats, dogs, and monkeys.

Author

Whitaker NG and Lindstrom TD

Subjects
Animals, Biotransformation, Chromatography methods, Dogs, Ergolines blood, Ergolines urine, Female, Macaca mulatta, Male, Mice, Quinpirole, Rats, Rats, Inbred Strains, Species Specificity, Ergolines metabolism
Abstract

The disposition and metabolism of quinpirole were studied in rats, mice, dogs, and monkeys. A single 2 mg/kg dose of 14C-quinpirole was administered orally to rats, mice, and monkeys. Dogs were given a single 0.2 mg/kg iv dose of 14C-quinpirole. Of the dose administered, 75-96% was recovered in the urine within 72 hr, with the majority being excreted during the first 24 hr. Peak plasma concentrations of radioactivity and quinpirole were coincident and were observed within 0.25 hr in rodents and at 2 hr in monkeys. Unchanged quinpirole accounted for 0.9%, 36%, and 69% respectively. Biotransformation of quinpirole was compared by quantitating the urinary metabolites by HPLC. The percentage of the radioactivity in urine representing unchanged drug was determined for each species: monkey (3%), dog (13%), mouse (40%), and rat (57%). The majority of 14C-quinpirole was shown to be biotransformed in rats, mice, and monkeys through common metabolic pathways but to various extents. Most metabolites resulted from structural alterations (N-dealkylation, lactam formation, omega and omega-1 hydroxylation) that centered around the piperidine ring portion of the molecule. These metabolites were less important in dogs. The major metabolic pathway in dogs involved hydroxylation of a methylene carbon adjacent to the pyrazole nucleus of quinpirole followed by O-glucuronidation. Evidence of metabolism of the pyrazole moiety was found in the isolation of an N-glucuronide conjugate of quinpirole from monkey urine.

Published
1987

35. Studies on cytochrome P-450-dependent lipid hydroperoxide reduction.

Author

Lindstrom TD and Aust SD

Subjects
Anaerobiosis, Animals, Enzyme Induction, Kinetics, Male, Microsomes, Liver drug effects, Mixed Function Oxygenases metabolism, NADPH-Ferrihemoprotein Reductase biosynthesis, Oxidation-Reduction, Phenobarbital pharmacology, Rats, Rats, Inbred Strains, Cytochrome P-450 Enzyme System metabolism, Lipid Peroxides metabolism, Microsomes, Liver metabolism, NADPH-Ferrihemoprotein Reductase isolation & purification
Abstract

A reconstituted mixed-function oxidase system containing cytochrome P-450, cytochrome P-450 reductase, phosphatidylcholine, and NADPH catalyzed the reduction of 13-hydroperoxy-9,11-octadecadienoic acid to 13-hydroxy-9,11-octadecadienoic acid. Activity was stimulated by the addition of type I substrates, while carbon monoxide and oxygen inhibited the reaction. Perfluoro-n-hexane stimulated the reduction of lipid hydroperoxide to lipid alcohol in the reconstituted system but not by cytochrome P-450 alone. Incubation of cytochrome P-450 with only lipid hydroperoxide resulted in destruction of the hemoprotein. Addition of substrates such as aminopyrine decreased cytochrome P-450 destruction. Addition of reducing equivalents from a reconstituted electron transport system also decreased cytochrome P-450 destruction.

Published
1984
Full Text
View/download PDF

36. Effect of cycloheximide and actinomycin D on carbon tetrachloride hepatotoxicity.

Author

Lindstrom TD and Anders MW

Subjects
Animals, Aspartate Aminotransferases blood, Carbon Tetrachloride Poisoning complications, Chemical and Drug Induced Liver Injury etiology, Cytochrome P-450 Enzyme System metabolism, Lipid Metabolism, Liver metabolism, Male, Microsomes, Liver metabolism, Proteins metabolism, Rats, Time Factors, Triglycerides metabolism, Carbon Tetrachloride Poisoning metabolism, Chemical and Drug Induced Liver Injury metabolism, Cycloheximide pharmacology, Dactinomycin pharmacology
Published
1977
Full Text
View/download PDF

37. Effect of agents known to alter carbon tetrachloride hepatotoxicity and cytochrome P-450 levels on carbon tetrachloride-stimulated lipid peroxidation and ethane expiration in the intact rat.

Author

Lindstrom TD and Anders MW

Subjects
1-Propanol pharmacology, Animals, Breath Tests, Cobalt pharmacology, Drug Interactions, Ethanol pharmacology, Male, Maleates pharmacology, Methylcholanthrene pharmacology, Peroxides metabolism, Phenobarbital pharmacology, Rats, Carbon Tetrachloride pharmacology, Ethane metabolism, Lipid Metabolism
Published
1978
Full Text
View/download PDF

38. The pharmacokinetics of indecainide in mice, rats, dogs, and monkeys.

Author

Lindstrom TD and Whitaker GW

Subjects
Animals, Dogs, Fluorenes blood, Fluorenes urine, Kinetics, Macaca mulatta, Mice, Rats, Rats, Inbred Strains, Anti-Arrhythmia Agents metabolism, Fluorenes metabolism
Abstract

The pharmacokinetics of indecainide, a new antiarrhythmic agent, were studied in mice, rats, dogs, and monkeys. The drug was well absorbed in all species tested resulting in peak plasma levels of drug within 2 hr. The plasma half-life of indecainide after acute oral administration was 3-5 hr in rats, dogs, and monkeys but considerably shorter in mice. The plasma half-life of indecainide was dose-dependent in dogs and increased slightly with chronic dosing. Peak plasma levels of drug were also dose-dependent in dogs and monkeys. Fecal elimination was the primary route of excretion of the drug in rats and mice after oral dosing. Fifty per cent of the dose was excreted in the bile of rats which was then subject to enterohepatic circulation. Urinary elimination was the predominant excretory route in the dog. Tissue distribution of radioactivity in rats showed that tissues which first encounter the drug have the highest levels of radioactivity. The highest concentrations were found in the stomach, intestine, liver, and kidney, whereas very low levels were observed in the fat and brain. Except for liver and kidney, only very low levels were present after 24 hr.

Published
1984

39. Disposition of the aromatase inhibitor LY56110 and associated induction and inhibition studies in rats, dogs, and monkeys.

Author

Lindstrom TD and Whitaker GW

Subjects
Animals, Body Weight drug effects, Cytochrome P-450 Enzyme System metabolism, Dogs, Enzyme Induction, Female, Half-Life, Hemoglobins metabolism, Kinetics, Liver drug effects, Macaca mulatta, Male, Microsomes, Liver metabolism, Organ Size drug effects, Rats, Rats, Inbred Strains, Species Specificity, Tissue Distribution, Aromatase Inhibitors, Pyrimidines metabolism
Abstract

Compound LY56110 was well absorbed but slowly excreted in the rat, dog, and monkey. Oral administration of 5 mg/kg of [14C]LY56110 (5-bis(4-chlorophenyl)methylpyrimidine) to the rat, monkey, and dog resulted in a total excretion of 68, 65, and 30% of the radioactivity within 5 days, respectively. Very low urinary excretion was observed in the rat and dog (2%), with fecal excretion being the predominant mode of elimination in all three species. The plasma radioactivity half-life was 49, 41, and greater than 100 hr in the rat, monkey, and dog, respectively. The plasma half-life of parent compound was 18 hr in the rat and 10 hr in the dog. LY56110 accounted for only 25, 12, and 1% of the plasma radioactivity area under the curve in the rat, dog, and monkey, respectively. High levels of radioactivity were observed in the target tissues of fat, adrenals, and ovaries of rats. LY56110 induced hepatic cytochromes b5 and P-450 and cytochrome c reductase in rats after 14 days of oral dosing at 10 mg/kg but not in monkeys after 10 days of oral dosing at 10 mg/kg. The compound was more potent than aminoglutethimide or cimetidine in inhibiting hepatic ethylmorphine and p-nitroanisole demethylase activity in vitro. LY56110 also inhibited ethinamate-induced sleeping time in rats in vivo. The compound induced a reverse type I binding spectrum with rat ovarian microsomes.

Published
1987
Full Text
View/download PDF

40. Discovery and development of a novel class of nonsteroidal aromatase inhibitors.

Author

Hirsch KS, Jones CD, Lindstrom TD, Stamm NB, Sutton GP, Taylor HM, and Weaver DE

Subjects
Animals, Body Weight drug effects, Cholesterol metabolism, Enzyme Induction, Female, Fungicides, Industrial pharmacokinetics, Fungicides, Industrial pharmacology, Humans, In Vitro Techniques, Mammary Neoplasms, Experimental enzymology, Microsomes enzymology, Microsomes, Liver enzymology, Organ Size drug effects, Pyrimidines pharmacokinetics, Pyrimidines pharmacology, Rats, Rats, Inbred F344, Rats, Inbred Strains, Tissue Distribution, Tumor Cells, Cultured drug effects, Tumor Cells, Cultured enzymology, Aromatase Inhibitors
Abstract

Efforts to develop a novel class of nonsteroidal aromatase inhibitors began with the discovery that the infertility in male rats exposed to high levels of the agricultural fungicide, fenarimol (alpha-(2-chlorophenyl)-alpha-(4-chlorophenyl)-5-pyrimidine-methanol), was attributable to the inhibition of aromatase activity within the central nervous system during the critical neonatal period. Although fenarimol was not particularly potent in inhibiting rat ovarian microsome aromatase activity in vitro (50% inhibition (IC50) = 4.1 microM). Subsequent testing of a number of analogues led to the identification of LY56110 (alpha,alpha-bis(4-chlorophenyl)-5-methylpyrimidine) which exhibited an IC50 of 29 nM. LY56110 was orally active, blocking the testosterone-induced increase of uterine weight and ovarian estrogen biosynthesis in immature female rats. In rats with established DMBA-induced mammary carcinoma, complete tumor regression was observed in 80% of the animals. Development of LY56110 was, however, stopped because of its effects on hepatic microsomal enzymes and an unacceptably long half-life. Structural modifications resulted in the development of the indenopyrimidines. LY113174 (8-chloro-5-(4-chlorophenyl)-5H-indeno less than 1, 2D greater than pyrimidine) was highly effective in vitro (IC50 = 24 nM) and in vivo but was far less potent than LY56110 with respect to induction of hepatic microsomal enzymes. LY113174 exhibited an acceptable biological half-life and had no effect on cholesterol side-chain cleavage. The indenopyrimidines appear to be a novel class of nonsteroidal aromatase inhibitors which may prove useful in the treatment of estrogen-dependent diseases.

Published
1987
Full Text
View/download PDF

41. Inhibition of microsomal biotransformation by a series of nitrogen and oxygen heterocyclic histamine H2-antagonists.

Author

Lindstrom TD, Whitaker GW, and Pioch RP

Subjects
Animals, Biotransformation drug effects, Chemical Phenomena, Chemistry, Cimetidine pharmacology, Male, Microsomes, Liver drug effects, Nitrogen, Oxygen, Rats, Rats, Inbred Strains, Structure-Activity Relationship, Ethylmorphine-N-Demethylase antagonists & inhibitors, Heterocyclic Compounds, Histamine H2 Antagonists pharmacology, Microsomes, Liver enzymology, Oxidoreductases, N-Demethylating antagonists & inhibitors
Abstract

A homologous series of potent, long-lasting thiazolo-pyrimidone-pyridine histamine H2-antagonists were examined for their inhibitory effects on rat hepatic ethylmorphine N-demethylation. Inhibitory potency increased in the order: 2-pyridinyl less than 3-pyridinyl less than 4-pyridinyl histamine H2-antagonist. Substitution ortho to the pyridine nitrogen decreased inhibitory potency. Hydroxylation of the pyridine heterocycle decreased inhibitory potency, whereas substituent electronic effects did not appreciably alter the inhibitory potency of these compounds. Antagonists containing oxygen heterocycles were moderately potent inhibitors compared to those containing unsubstituted pyridine as the heterocycle. A 3-(6-methylpyridine) histamine H2-antagonist was shown to be a slightly more potent inhibitor of ethinamate metabolism than cimetidine in rats. However, unlike cimetidine, it did not inhibit the plasma half-life of antipyrine in dogs at doses that were equally efficacious in inhibiting gastric acid secretion.

Published
1987
Full Text
View/download PDF

Catalog

Books, media, physical & digital resources
See catalog results