Your search keyword '"Reagan WJ"' showing total 45 results

1. High Resolution Electron Microscopy of Nanostructure on the Surface of commercial FCC Catalyst

Author

Tang, YL, primary, Allahverdi, M, additional, and Reagan, WJ, additional

Published

2009

2. Circulating microRNAs as promising testicular translatable safety biomarkers: current state and future perspectives.

Author

Zhang J, Campion S, Catlin N, Reagan WJ, Palyada K, Ramaiah SK, and Ramanathan R

Subjects

Male, Humans, Testis metabolism, Biomarkers metabolism, Leydig Cells metabolism, Circulating MicroRNA metabolism, MicroRNAs genetics

Abstract

Drug-induced testicular injury (DITI) is one of the often-observed and challenging safety issues seen during drug development. Semen analysis and circulating hormones currently utilized have significant gaps in their ability to detect testicular damage accurately. In addition, no biomarkers enable a mechanistic understanding of the damage to the different regions of the testis, such as seminiferous tubules, Sertoli, and Leydig cells. MicroRNAs (miRNAs) are a class of non-coding RNAs that modulate gene expression post-transcriptionally and have been indicated to regulate a wide range of biological pathways. Circulating miRNAs can be measured in the body fluids due to tissue-specific cell injury/damage or toxicant exposure. Therefore, these circulating miRNAs have become attractive and promising non-invasive biomarkers for assessing drug-induced testicular injury, with several reports on their use as safety biomarkers for monitoring testicular damage in preclinical species. Leveraging emerging tools such as 'organs-on-chips' that can emulate the human organ's physiological environment and function is starting to enable biomarker discovery, validation, and clinical translation for regulatory qualification and implementation in drug development., (© 2023. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published

2023

3. To Clot or Not to Clot: Deepening Our Understanding of Alterations in the Hemostatic System.

Author

Reagan WJ, Brooks MB, Grozovsky R, Pittman D, Vitsky A, and Brenneman K

Subjects

Humans, Hemostasis, Thrombopoietin genetics, Blood Platelets, Hemostatics, Thrombocytopenia chemically induced

Abstract

The session on the hemostatic system focused on new developments in coagulation and platelet biology as well as how therapeutic agents may affect hemostasis. The classic cascade model of coagulation was compared with the more recent models of cell-based and vascular-based coagulation, which may provide better insight on how the coagulation cascade works in vivo. A review of platelet biology highlighted that, as platelets age, desialylated platelets form and are recognized by Ashwell-Morell receptor (AMR), leading to hepatic uptake and subsequent increase in thrombopoietin (TPO) production. Administration of therapeutics that induce thrombocytopenia was also discussed, including Mylotarg, which is an antibody-drug conjugate that was shown to decrease human megakaryocyte development but had no effect on platelet aggregation. An acetyl co-A carboxylase inhibitor was shown to cause thrombocytopenia by inhibiting de novo lipogenesis, which is critical for the formation of the megakaryocyte demarcation membrane system responsible for platelet production. It was also illustrated how preclinical translation models have been very helpful in the development of adeno-associated virus (AAV) hemophilia B gene therapy and what old and new preclinical tools we have that can predict the risk of a prothrombotic state in people.

Published

2022

4. Comprehensive Nonclinical Safety Assessment of Nirmatrelvir Supporting Timely Development of the SARS-COV-2 Antiviral Therapeutic, Paxlovid™.

Author

Sathish JG, Bhatt S, DaSilva JK, Flynn D, Jenkinson S, Kalgutkar AS, Liu M, Manickam B, Pinkstaff J, Reagan WJ, Shirai N, Shoieb AM, Sirivelu M, Vispute S, Vitsky A, Walters K, Wisialowski TA, and Updyke LW

Subjects

Animals, Male, Rats, Antiviral Agents adverse effects, COVID-19 Drug Treatment

Abstract

COVID-19 is a potentially fatal infection caused by the SARS-CoV-2 virus. The SARS-CoV-2 3CL protease (Mpro) is a viral enzyme essential for replication and is the target for nirmatrelvir. Paxlovid (nirmatrelvir co-administered with the pharmacokinetic enhancer ritonavir) showed efficacy in COVID-19 patients at high risk of progressing to hospitalization and/or death. Nonclinical safety studies with nirmatrelvir are essential in informing benefit-risk of Paxlovid and were conducted to support clinical development. In vivo safety pharmacology assessments included a nervous system/pulmonary study in rats and a cardiovascular study in telemetered monkeys. Potential toxicities were assessed in repeat dose studies of up to 1 month in rats and monkeys. Nirmatrelvir administration (1,000 mg/kg, p.o.) to male rats produced transient increases in locomotor activity and respiratory rate but did not affect behavioral endpoints in the functional observational battery. Cardiovascular effects in monkeys were limited to transient increases in blood pressure and decreases in heart rate, observed only at the highest dose tested (75 mg/kg per dose b.i.d; p.o.). Nirmatrelvir did not prolong QTc-interval or induce arrhythmias. There were no adverse findings in repeat dose toxicity studies up to 1 month in rats (up to 1,000 mg/kg daily, p.o.) or monkeys (up to 600 mg/kg daily, p.o.). Nonadverse, reversible clinical pathology findings without clinical or microscopic correlates included prolonged coagulation times at ≥60 mg/kg in rats and increases in transaminases at 600 mg/kg in monkeys. The safety pharmacology and nonclinical toxicity profiles of nirmatrelvir support clinical development and use of Paxlovid for treatment of COVID-19.

Published

2022

5. The use of emerging safety biomarkers in nonclinical and clinical safety assessment - The current and future state: An IQ DruSafe industry survey.

Author

Zabka TS, Burkhardt J, Reagan WJ, Gautier JC, Glaab WE, Guffroy M, Harding J, Brees D, McDuffie E, Ramaiah L, Schultze AE, Smith JD, Wolfreys A, and Dalmas DA

Subjects

Animals, Clinical Trials as Topic methods, Drug Evaluation, Preclinical methods, Drug Evaluation, Preclinical standards, Drug Industry methods, Drug-Related Side Effects and Adverse Reactions diagnosis, Drug-Related Side Effects and Adverse Reactions prevention & control, Forecasting, Humans, Pharmaceutical Preparations metabolism, Tissue Distribution drug effects, Tissue Distribution physiology, Biomarkers, Pharmacological metabolism, Clinical Trials as Topic standards, Drug Industry standards, Drug-Related Side Effects and Adverse Reactions metabolism, Surveys and Questionnaires

Abstract

Pharmaceutical and biotechnology companies rarely disclose their use of translational emerging safety biomarkers (ESBs) during drug development, and the impact of ESB use on the speed of drug development remains unclear. A cross-industry survey of 20 companies of varying size was conducted to understand current trends in ESB use and future use prospects. The objectives were to: (1) determine current ESB use in nonclinical and clinical drug development and impact on asset advancement; (2) identify opportunities, gaps, and challenges to greater ESB implementation; and (3) benchmark perspectives on regulatory acceptance. Although ESBs were employed in only 5-50% of studies/programs, most companies used ESBs to some extent, with larger companies demonstrating greater nonclinical use. Inclusion of ESBs in investigational new drug applications (INDs) was similar across all companies; however, differences in clinical trial usage could vary among the prevailing health authority (HA). Broader implementation of ESBs requires resource support, cross-industry partnerships, and collaboration with HAs. This includes generating sufficient foundational data, demonstrating nonclinical to clinical translatability and practical utility, and clearly written criteria by HAs to enable qualification. If achieved, ESBs will play a critical role in the development of next-generation, translationally-tailored standard laboratory tests for drug development., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2021

6. De novo lipogenesis is essential for platelet production in humans.

Author

Kelly KL, Reagan WJ, Sonnenberg GE, Clasquin M, Hales K, Asano S, Amor PA, Carvajal-Gonzalez S, Shirai N, Matthews MD, Li KW, Hellerstein MK, Vera NB, Ross TT, Cappon G, Bergman A, Buckeridge C, Sun Z, Qejvanaj EZ, Schmahai T, Beebe D, Pfefferkorn JA, and Esler WP

Subjects

Acetyl-CoA Carboxylase antagonists & inhibitors, Acetyl-CoA Carboxylase metabolism, Animals, Diabetes Mellitus, Type 2 drug therapy, Dogs, Dose-Response Relationship, Drug, Double-Blind Method, Enzyme Inhibitors pharmacology, Gene Expression drug effects, Humans, Lipid Metabolism, Macaca fascicularis, Megakaryocytes physiology, Platelet Count, Rats, Blood Platelets, Lipogenesis physiology

Abstract

Acetyl-CoA carboxylase (ACC) catalyses the first step of de novo lipogenesis (DNL). Pharmacologic inhibition of ACC has been of interest for therapeutic intervention in a wide range of diseases. We demonstrate here that ACC and DNL are essential for platelet production in humans and monkeys, but in not rodents or dogs. During clinical evaluation of a systemically distributed ACC inhibitor, unexpected dose-dependent reductions in platelet count were observed. While platelet count reductions were not observed in rat and dog toxicology studies, subsequent studies in cynomolgus monkeys recapitulated these platelet count reductions with a similar concentration response to that in humans. These studies, along with ex vivo human megakaryocyte maturation studies, demonstrate that platelet lowering is a consequence of DNL inhibition likely to result in impaired megakaryocyte demarcation membrane formation. These observations demonstrate that while DNL is a minor quantitative contributor to global lipid balance in humans, DNL is essential to specific lipid pools of physiological importance.

Published

2020

7. Evaluation of Rat Acute Phase Proteins as Inflammatory Biomarkers for Vaccine Nonclinical Safety Studies.

Author

Reagan WJ, Shoieb AM, Schomaker SJ, Markiewicz VR, Clarke DW, and Sellers RS

Subjects

Acute-Phase Proteins, Animals, Biomarkers, Female, Rats, Rats, Wistar, Tetanus, Whooping Cough

Abstract

The objectives were to characterize the kinetics of acute phase proteins (APPs) α-2 macroglobulin (A2M), α-1 acid glycoprotein (A1AGP), and fibrinogen (FIB), and injection site macroscopic and microscopic findings following intramuscular administration of tetanus toxoid, reduced diphtheria toxoid, and acellular pertussis vaccine (TDaP; Adacel); adjuvants (aluminum phosphate [AlPO 4 ]; aluminum hydroxide, Al[OH] 3 ; CpG/Al[OH] 3 ; or Quillaja saponaria 21 [QS-21]); or saline to female Wistar Han rats. Intravascular lipopolysaccharide (LPS) was a positive control. Injection sites and lymph nodes were evaluated microscopically, using hematoxylin and eosin (H&E) stained sections, 48 hours postdose (HPD) and compared with APP concentrations; A2M and A1AGP were measured using Meso Scale Discovery analyzer. Fibrinogen was measured on STA Compact analyzer. In a time-course study, APP peaked at 24 or 48 HPD. In a subsequent study at 48 HPD, injection site microscopic changes included inflammation and muscle degeneration/necrosis, which was different in severity/nature between groups. The APPs were not increased in rats administered saline, Al(OH) 3 , or AlPO 4 . Fibrinogen and A1AGP increased in rats administered CpG/Al(OH) 3 , QS-21, or TDaP; and A2M increased in rats administered QS-21. Fibrinogen, A2M, and A1AGP increased after LPS administration. Acute phase proteins can be used to monitor inflammatory responses to adjuvants; however, some adjuvants may induce inflammation without higher APPs.

Published

2020

8. Confounding Factors in the Interpretation of Preclinical Studies.

Author

Morton LD, Sanders M, Reagan WJ, Crabbs TA, McVean M, and Funk KA

Subjects

Animal Experimentation, Animals, Drug Evaluation, Preclinical methods, Research Design

Abstract

A number of issues may arise during the conduct of a study which can complicate interpretation of in vitro and in vivo datasets. Speakers discussed the implications of differing interpretations and how to avoid complicating factors during study planning and execution. Consideration needs to be given to study design factors including defining objectives, consideration of expected pharmacological effects, dose selection and drug kinetics, species used, and vehicle selection. In addition, the effects of vivarium temperature effects on various endpoints, how to control variables affecting clinical pathology, and how early death animals, common background findings, and artifacts can affect histopathology interpretation all play into the final interpretation of study data.

Published

2019

9. Effects of Monoclonal Antibodies against Nerve Growth Factor on Healthy Bone and Joint Tissues in Mice, Rats, and Monkeys: Histopathologic, Biomarker, and Microcomputed Tomographic Assessments.

Author

Gropp KE, Carlson CS, Evans MG, Bagi CM, Reagan WJ, Hurst SI, Shelton DL, and Zorbas MA

Subjects

Animals, Antibodies, Monoclonal toxicity, Macaca fascicularis, Mice, Mice, Inbred C57BL, Rats, Rats, Sprague-Dawley, Tomography, X-Ray Computed, Antibodies, Monoclonal, Humanized toxicity, Bone and Bones drug effects, Joints drug effects, Nerve Growth Factor antagonists & inhibitors

Abstract

Tanezumab, an anti-nerve growth factor (NGF) antibody, is in development for management of chronic pain. During clinical trials of anti-NGF antibodies, some patients reported unexpected adverse events requiring total joint replacements, resulting in a partial clinical hold on all NGF inhibitors. Three nonclinical toxicology studies were conducted to evaluate the effects of tanezumab or the murine precursor muMab911 on selected bone and joint endpoints and biomarkers in cynomolgus monkeys, Sprague-Dawley rats, and C57BL/6 mice. Joint and bone endpoints included histology, immunohistochemistry, microcomputed tomography (mCT) imaging, and serum biomarkers of bone physiology. Responses of bone endpoints to tanezumab were evaluated in monkeys at 4 to 30 mg/kg/week for 26 weeks and in rats at 0.2 to 10 mg/kg twice weekly for 28 days. The effects of muMab911 at 10 mg/kg/week for 12 weeks on selected bone endpoints were determined in mice. Tanezumab and muMab911 had no adverse effects on any bone or joint parameter. There were no test article-related effects on bone or joint histology, immunohistochemistry, or structure. Reversible, higher osteocalcin concentrations occurred only in the rat study. No deleterious effects were observed in joints or bones in monkeys, rats, or mice administered high doses of tanezumab or muMab911.

Published

2018

10. Principles for Assessing Adversity in Toxicologic Clinical Pathology.

Author

Ramaiah L, Tomlinson L, Tripathi NK, Cregar LC, Vitsky A, Beust BV, Barlow VG, Reagan WJ, and Ennulat D

Subjects

Animals, Drug-Related Side Effects and Adverse Reactions veterinary, Humans, No-Observed-Adverse-Effect Level, Quality Control, Risk Assessment, Toxicity Tests veterinary, Biomarkers analysis, Drug-Related Side Effects and Adverse Reactions diagnosis, Guidelines as Topic, Pathology, Clinical standards, Pathology, Veterinary standards, Toxicity Tests standards

Abstract

There is limited direction in the literature or regulatory guidance on determination of adversity for clinical pathology (CP) biomarkers in preclinical safety studies. Toxicologic clinical pathologists representing the American Society for Veterinary Clinical Pathology-Regulatory Affairs Committee and Society of Toxicologic Pathology-Clinical Pathology Interest Group identified principles, overall approach, and unique considerations for assessing adversity in CP data interpretation to provide a consensus opinion. Emphasized is the need for pathophysiologic context and a weight-of-evidence approach. Most CP biomarkers do not have the potential to be adverse in isolation, regardless of magnitude of change. Rather, they quantify or describe the impact of effects, provide adjunct or supportive information regarding a process or pathogenesis, and provide translational biomarkers of effect. Most often, CP changes are part of a constellation of findings that collectively are adverse. Thus, most CP changes must be interpreted in conjunction with other study findings and require contextual and integrative interpretation. Exceptions include critical CP changes without correlates that indicate a health risk in the tested species. Overall, CP changes should not be interpreted in isolation and their adversity is best addressed with an integrated approach.

Published

2017

11. Assessment of Cardiac Troponin I Responses in Nonhuman Primates during Restraint, Blood Collection, and Dosing in Preclinical Safety Studies.

Author

Reagan WJ, Barnes R, Harris P, Summers S, Lopes S, Stubbs M, Blackwell D, and Steidl-Nichols J

Subjects

Animals, Biomarkers blood, Blood Specimen Collection standards, Blood Specimen Collection veterinary, Drug Evaluation, Preclinical standards, Drug Evaluation, Preclinical veterinary, Macaca fascicularis, Male, Restraint, Physical, Blood Specimen Collection methods, Drug Evaluation, Preclinical methods, Heart drug effects, Pharmaceutical Preparations administration & dosage, Troponin I blood

Abstract

Limited information has been published on the use of cardiac troponin I (cTnI) as a biomarker of cardiac injury in monkeys. The purpose of these studies was to characterize the cTnI response seen in cynomolgus macaques during routine dosing and blood collection procedures typically used in preclinical safety studies and to better understand the pathogenesis of this response. We measured cTnI using two different methods, the Siemens Immulite cTnI assay and the more sensitive Siemens Troponin I-Ultra assay. We were able to demonstrate that after oral, subcutaneous, or intravenous dosing of common vehicles, as well as serial chair restraint for venipuncture blood collection, that minimal to mild transient increases in cTnI could be detected in monkeys with both assays. cTnI values typically peaked at 2, 3, 4, or 6 hr after sham dosing and returned to baseline at 22 or 24 hr. In addition, marked increases in heart rate (HR) and blood pressure (BP) occurred in monkeys during the restraint procedures, which likely initiated the cTnI release in these animals. Monkeys that were very well acclimated to the chairing procedures and had vascular access ports for blood sampling did not have marked increases in HRs and BP or increases in cTnI.

Published

2017

12. Evaluation of Cardiac Toxicity Biomarkers in Rats from Different Laboratories.

Author

Kim K, Chini N, Fairchild DG, Engle SK, Reagan WJ, Summers SD, and Mirsalis JC

Subjects

Animals, Cardiotoxicity, Drug Evaluation, Preclinical, Myocardium metabolism, Myocardium pathology, Rats, Biomarkers blood, Drug Discovery standards, Drug-Related Side Effects and Adverse Reactions blood, Heart drug effects, Laboratories standards

Abstract

There is a great need for improved diagnostic and prognostic accuracy of potential cardiac toxicity in drug development. This study reports the evaluation of several commercially available biomarker kits by 3 institutions (SRI, Eli Lilly, and Pfizer) for the discrimination between myocardial degeneration/necrosis and cardiac hypertrophy as well as the assessment of the interlaboratory and interplatform variation in results. Serum concentrations of natriuretic peptides (N-terminal pro-atrial natriuretic peptide [NT-proANP] and N-terminal pro-brain natriuretic peptide [NT-proBNP]), cardiac and skeletal troponins (cTnI, cTnT, and sTnI), myosin light chain 3 (Myl3), and fatty acid binding protein 3 (FABP3) were assessed in rats treated with minoxidil (MNX) and isoproterenol (ISO). MNX caused increased heart-to-body weight ratios and prominent elevations in NT-proANP and NT-proBNP concentrations detected at 24-hr postdose without elevation in troponins, Myl3, or FABP3 and with no abnormal histopathological findings. ISO caused ventricular leukocyte infiltration, myocyte fibrosis, and necrosis with increased concentrations of the natriuretic peptides, cardiac troponins, and Myl3. These results reinforce the advantages of a multimarker strategy in elucidating the underlying cause of cardiac insult and detecting myocardial tissue damage at 24-hr posttreatment. The interlaboratory and interplatform comparison analyses also showed that the data obtained from different laboratories and platforms are highly correlated and reproducible, making these biomarkers widely applicable in preclinical studies.

Published

2016

13. Evaluation of urinary corticosterone as a biomarker of stress in rats using fenitrothion as a chemical stressor.

Author

Lapointe JM, Snyder PA, and Reagan WJ

Subjects

Animals, Body Weight, Drug-Related Side Effects and Adverse Reactions metabolism, Fenitrothion administration & dosage, Immunosuppressive Agents administration & dosage, Male, Rats, Rats, Sprague-Dawley, Spleen drug effects, Spleen pathology, Thymus Gland drug effects, Thymus Gland pathology, Adverse Drug Reaction Reporting Systems, Biomarkers urine, Corticosterone urine, Drug-Related Side Effects and Adverse Reactions diagnosis, Fenitrothion adverse effects, Immunosuppressive Agents adverse effects, Stress, Physiological physiology

Abstract

Regulatory guidelines for pharmaceutical toxicity studies recommend using one dose near the maximum tolerated. At that level significant toxicities may occur, leading to systemic stress and secondary immune suppression which can be difficult to differentiate from a primary drug effect. Therefore, there is a need for a biomarker of stress applicable to toxicity studies. This study evaluated urinary corticosterone as a biomarker, using as a pharmacologic stressor fenitrothion, which was previously shown not to cause primary immune suppression. Rats were administered fenitrothion orally at 20 and 30 mg/kg daily for 2 or 8 days, with matched vehicle controls (n = 6/group). Urine was collected for 6 and 24 h, before treatment and on Day 2 and Day 8. Urine was assayed for corticosterone, separately for the first 6 h of collection and for the whole 24 h sample. Animals were euthanized on Day 3 or Day 9 and lymphoid tissue samples were collected, weighed and examined histologically. Treated rats showed neurologic signs following treatment. Findings also included time- and dose-dependent decreases in body weight and spleen and thymus weight decreases supra-proportional to body weight on Day 9. Histologic changes were mild at a dose of 20 mg/kg, but significant at 30 mg/kg, consisting of lymphocytolysis at Day 3 and lymphoid depletion at Day 9. Urine corticosterone levels were increased on Day 2 and Day 8, in the 6-h samples, but not the 24-h ones, at both dose levels. Based on the results, urine corticosterone appears to be a sensitive biomarker of systemic stress caused by fenitrothion. Other chemical stressors should be evaluated in a similar manner in order to fully validate urine corticosterone measurement as a stress biomarker.

Published

2016

14. Cross-laboratory analytical validation of the cardiac biomarker NT-proANP in rat.

Author

Vinken P, Reagan WJ, Rodriguez LA, Buck WR, Lai-Zhang J, Goeminne N, Barbacci G, Liu R, King NM, Engle SK, and Colton H

Subjects

Animals, Biomarkers blood, Heart, Humans, Male, Myocardium metabolism, Rats, Rats, Sprague-Dawley, Atrial Natriuretic Factor blood, Protein Precursors blood

Abstract

Introduction: Natriuretic peptides, including N-terminal-proatrial natriuretic peptide (NT-proANP) are cardiac hormones that are produced in response to myocardial stretch and have been used in rats and humans as blood based functional cardiac biomarkers. There are limited validation data of these assays in rats and therefore the Predictive Safety Testing Consortium, Cardiac Hypertrophy Working Group (PSTC-CHWG) performed a cross-laboratory (5 laboratories) analytical evaluation of a commercially available NT-proANP ELISA for use with rat samples., Methods: Serum samples were collected from normal Sprague Dawley (SD) rats and were spiked with kit calibrator material or rat heart tissue extracts to provide specimens for the validation. In addition, the cardiotoxicant, isoproterenol, was used to induce elevated endogenous NT-proANP levels in a subgroup of rats for additional validation specimens. The Biomedica™ (BI-20892, Vienna, Austria) proANP (1-98) enzyme-linked immunoabsorbent assay (ELISA) kit was used to measure NT-proANP. Intra-assay and inter-assay precisions, accuracy, sample linearity, recovery, limit of detection, upper and lower limits of quantitation (ULOQ and LLOQ, respectively), sample-freeze/thaw stability and stored sample stability were assessed and compared to pre-determined acceptance criteria., Results: The majority of the experimental assessments met the established validation criteria, however there were individual results that did not meet these standards. Overall, acceptable intra- and inter-assay precisions and accuracies as well as inter-laboratory precision and accuracy were demonstrated. Linearity and recovery values fell within the pre-determined acceptance criteria, samples remained stable for up to three freeze-thaw cycles and frozen samples were stable at ~-70 °C for 12 months. The limit of detection (LOD) and LLOQ and ULOQ were similar to those specified by the manufacturer., Discussion: Overall, the assay was demonstrated to be technically adequate for the detection of NT-proANP serum levels in SD rats., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2016

15. Toxicities associated with 1-month treatment with propylthiouracil (PTU) and methimazole (MMI) in male rats.

Author

Nambiar PR, Palanisamy GS, Okerberg C, Wolford A, Walters K, Buckbinder L, and Reagan WJ

Subjects

Animals, Male, Methimazole administration & dosage, Methimazole blood, Methimazole pharmacokinetics, Propylthiouracil administration & dosage, Propylthiouracil blood, Propylthiouracil pharmacokinetics, Rats, Rats, Wistar, Testis chemistry, Testis pathology, Thyroid Gland chemistry, Thyroid Gland pathology, Toxicity Tests, Methimazole toxicity, Propylthiouracil toxicity, Testis drug effects, Thyroid Gland drug effects

Abstract

Thionamides such as propylthiouracil (PTU) and methimazole (MMI) have been used for more than 50 years to treat the more common causes of thyrotoxicosis/hyperthyroidism such as Graves' disease. Serious adverse effects associated with thionamides in humans include idiosyncratic liver damage, agranulocytosis, aplastic anemia, and vasculitis. Both prospective and retrospective clinical studies with these drugs have failed to identify predictive biomarker for these adverse effects. To assess whether rat is a good model for predicting drug-related adverse events in the liver and in the bone marrow, we conducted a comprehensive study in male rats with multiple doses of PTU and MMI. As expected, euthyroid animals became hypothyroid along with several secondary changes associated with hypothyroidism. There were slight reductions in red blood cell parameters along with some marginal effects on the bone marrow elements. However, there was no evidence of significant neutropenia and liver injury in both PTU-treated and MMI-treated cohorts. MMI-related effects were noted in the seminiferous tubules of the testes. Overall, 1-month daily treatment of euthyroid rats with PTU or MMI resulted in hypothyroidism, minor bone marrow effects, and several secondary effects associated with hypothyroidism, but without any evidence of adverse effects reported in humans including liver injury and agranulocytosis., (© 2013 by The Author(s).)

Published

2014

16. The American Society for Veterinary Clinical Pathology Regulatory Affairs Committee's clinical pathology best practices recommendations will impact the discipline of veterinary toxicologic clinical pathology.

Author

Reagan WJ

Subjects

Animals, Drug-Related Side Effects and Adverse Reactions veterinary, Practice Guidelines as Topic, Societies, Toxicology, United States, Pathology, Clinical standards, Pathology, Veterinary standards

Published

2013

17. Summary of the HESI consortium studies exploring circulating inhibin B as a potential biomarker of testis damage in the rat.

Author

Chapin R, Weinbauer G, Thibodeau MS, Sonee M, Saldutti LP, Reagan WJ, Potter D, Moffit JS, Laffan S, Kim JH, Goldstein RA, Erdos Z, Enright BP, Coulson M, and Breslin WJ

Subjects

Animals, Biomarkers blood, Male, Rats, Rats, Sprague-Dawley, Rats, Wistar, Ecology, Health, Inhibins blood, Testis metabolism, Testis pathology

Abstract

The Developmental and Reproductive Toxicity Technical Committee of the Health and Environmental Sciences Institute hosted a working consortium of companies to evaluate a new commercially available analytic assay for Inhibin B in rat serum or plasma. After demonstrating that the kit was stable and robust, the group performed a series of independent pathogenesis studies (23 different compound/investigator combinations) designed to examine the correlation between the appearance of lesions in the testis and changes in circulating levels of Inhibin B. These studies were reported individually in the previous articles in this series (this issue), and are discussed in this paper. For roughly half of these exposures, lesions appeared well before Inhibin B changed. A few of the studies showed a good correlation between seminiferous tubule damage and reduced circulating Inhibin B levels, while for seven exposures, circulating Inhibin B was reduced with no detectable alteration in testis histology. Whether this indicates a prodromal response or a false-positive signal will require further investigation. These exceptions could plausibly suggest some value of circulating Inhibin B as a useful biomarker in some circumstances. However, for roughly half of these exposures, Inhibin B appeared to be a lagging biomarker, requiring significant damage to the seminiferous tubules before a consistent and credible reduction in circulating levels of Inhibin B was observed., (© 2013 Wiley Periodicals, Inc.)

Published

2013

18. The inhibin B response in male rats treated with two drug candidates.

Author

Chapin RE, Alvey JD, Goldstein RA, Dokmanovich MG, Reagan WJ, Johnson K, and Geoly FJ

Subjects

Animals, Follicle Stimulating Hormone blood, Hormones blood, Male, Organ Size drug effects, Rats, Spermatozoa drug effects, Spermatozoa metabolism, Testis drug effects, Testis pathology, Anti-Bacterial Agents pharmacology, Antiviral Agents pharmacology, Inhibins blood

Abstract

Background: Serum Inhibin B was measured in two studies of known testis-toxic drug candidates., Methods and Results: Study 1 was for a compound for Hepatitis C, and utilized a 10-week dosing period, followed by mating and necropsy of half of each group, and then a 12-week recovery period for the remaining animals. At the postmating necropsy, 6 of 15 high-dose males had testis lesions; Inhibin B was significantly reduced in all animals in that group. The mid-dose group had no lesions but significantly reduced serum Inhibin B. At recovery, 9 of 15 high-dose males showed damage in testes; serum Inhibin B levels were not different from controls. Inhibin B appeared to both overreport and underreport testis damage in Study 1. Study 2 was an acute pathogenesis study for an antibacterial compound, using control and two dose levels and multiple time points (days 5, 8, 15, 22, and then untreated until day 71). At each time point blood was sampled from all remaining rats and five/group were killed for histologic evaluation. The low-dose group had minimal to moderate lesions, while serum Inhibin B was never changed. The high-dose animals progressed quickly from minimal lesions to being broadly and moderately affected; serum Inhibin B levels were reduced at days 8 and 15 only. In Study 2, Inhibin B appeared less sensitive than histology, except at the extremes of testis damage, when Inhibin B was routinely low., Conclusion: We conclude that in these two studies there was a poor correlation between changes in serum levels of Inhibin B and testis histopathology., (© 2013 Wiley Periodicals, Inc.)

Published

2013

19. Analytic evaluation of a human ELISA kit for measurement of inhibin B in rat samples.

Author

Coulson M, Bickerton S, Betts CJ, Jacobsen M, Stewart J, Chapin RE, Reagan WJ, Alvey J, Erdos Z, Saldutti LP, Sonee M, Bogdan N, Singer M, Vinken P, Barlow V, Czajkowski K, and Kim JH

Subjects

Animals, Biological Assay, Freezing, Humans, Male, Quality Control, Rats, Rats, Sprague-Dawley, Reference Standards, Reference Values, Serum metabolism, Enzyme-Linked Immunosorbent Assay methods, Inhibins blood

Abstract

Background: A cross-laboratory analytic evaluation of a commercially available human inhibin B ELISA for measuring inhibin B in rat serum and plasma has been undertaken., Methods: Dilution linearity, spiked recovery, intra- and inter-assay precision, functional sensitivity, matrix effects, and frozen stability were assessed across five laboratories. Reference ranges were generated for male Sprague Dawley and Han Wistar rats., Results: Acceptable performance was defined as an overall assay coefficient of variation ≤ 20% with an intraday LLOQ ≤ 20 pg/ml. Intra- and inter-assay precision and functional sensitivity (≤6.4 pg/ml) generally met these criteria, but with occasional evidence of greater variability, particularly at lower concentrations. Dilution linearity was acceptable with occasional low recovery. Acceptable recovery of kit calibrators from rat serum confirmed the absence of matrix effects. Matched serum and plasma samples gave comparable results. The signal increased on freezing, remained constant for ≥3 freeze-thaw cycles and was generally stable for at least 8 weeks. Mean inhibin B ranged from 33.5 to 140.6 pg/ml in adult rats across laboratories, with some evidence for a decline from 6 to 9 weeks of age. Power calculations using preliminary reference range data indicated 10 animals/group would generally detect a 40% decrease in inhibin B at AstraZeneca, but laboratories with lower control values would require larger groups., Conclusions: The assay meets the analytical performance criteria; however, precision at the low end of the standard curve, biological variability, and low control values observed in some laboratories indicate that the utility of the assay may be limited in some laboratories., (© 2013 Wiley Periodicals, Inc.)

Published

2013

20. Comparison of cardiac troponin I and T, including the evaluation of an ultrasensitive assay, as indicators of doxorubicin-induced cardiotoxicity.

Author

Reagan WJ, York M, Berridge B, Schultze E, Walker D, and Pettit S

Subjects

Animals, Body Weight drug effects, Clinical Chemistry Tests, Eating drug effects, Heart drug effects, Heart Diseases metabolism, Hematologic Tests, Male, Myocardium chemistry, Rats, Rats, Sprague-Dawley, Sensitivity and Specificity, Toxicity Tests, Doxorubicin toxicity, Heart Diseases blood, Heart Diseases chemically induced, Troponin I blood, Troponin T blood

Abstract

Cardiac troponin (cTn) has been utilized to assess acute myocardial injury, but the cTn response in active/ongoing chronic injury is not well documented. The purpose of this study was to characterize the cardiac troponin I (cTnI), cardiac troponin T (cTnT), high-sensitivity cTnI, hematology, and clinical chemistry responses in rats treated with doxorubicin. Rats treated with 1, 2, or 3 mg/kg/week (wk) of doxorubicin for 2, 4, or 6 wks were sacrificed after 0, 2, or 4 wks of recovery and compared to untreated controls and animals treated with doxorubicin/dexrazoxane (50 mg/kg/wk) or etoposide (1 and 3 mg/kg/wk). The incidence and mean magnitude of cTn response increased with increasing dose and/or duration of doxorubicin treatment. Conversely, dexrazoxane/doxorubicin was partially protective for cardiotoxicity, and minimal cardiotoxicity occurred with etoposide treatment. Both cTnI and cTnT effectively identified doxorubicin-induced injury as indicated by vacuolation of cardiomyocytes of the atria/ventricles. The association between the cTn responses and histological changes was greater at the higher total exposures, but the magnitude of cTn response did not match closely with histologic grade. The high-sensitivity cTnI assay was also effective in identifying cardiac injury. Alterations occurred in the hematology and clinical chemistry parameters and reflected both dose and duration of doxorubicin treatment.

Published

2013

21. Response letter from Clinical Pathology Interest Group of the Society of Toxicologic Pathology (STP) for manuscript entitled International recommendations for training future toxicologic pathologists participating in regulatory-type, nonclinical toxicity studies by Bolon et al.

Author

Tripathi NK, Schultze AE, Pearson RC, Everds NE, Elliott GS, Ramaiah L, Wells MY, Latimer KS, Walter GL, Katavolos P, Collins ND, Tarrant J, Walker DB, Topper MJ, Jordan HL, O'Rourke LG, Guilpin VB, Brockus CW, Wilcox AL, Clemo FA, Smith GS, Reagan WJ, and McCartney JE

Subjects

Animals, International Cooperation, Pathology standards, Pathology trends, Professional Competence standards, Toxicity Tests standards, Toxicology standards, Toxicology trends, Guidelines as Topic, Pathology education, Toxicity Tests methods, Toxicology education

Published

2013

22. Metabolic adaptive ALT isoenzyme response in livers of C57/BL6 mice treated with dexamethasone.

Author

Reagan WJ, Yang RZ, Park S, Goldstein R, Brees D, and Gong DW

Subjects

Alanine Transaminase genetics, Animals, Blotting, Western, Gene Expression Regulation, Enzymologic drug effects, Glycogen metabolism, Isoenzymes genetics, Liver enzymology, Mice, Mice, Inbred C57BL, RNA, Messenger metabolism, Adaptation, Biological drug effects, Alanine Transaminase metabolism, Dexamethasone toxicity, Glucocorticoids toxicity, Isoenzymes metabolism, Liver drug effects

Abstract

Alanine aminotransferase (ALT) is used as an indicator of hepatocellular injury. Since ALT consists of two isoenzymes, a better understanding of ALT isoenzyme biology in response to compounds that cause metabolic adaptive versus hepatotoxic responses will allow for a more accurate assessment of the significance of an ALT increase. The purpose of this study was to characterize the ALT isoenzyme response in mice treated with 25 or 75 mg/kg of dexamethasone, which is known to induce a progluconeogenic state, for 24 or 72 hr. Those mice treated with 75 mg/kg for 72 hr showed an increase in total liver ALT activity. Western blot showed that there was an increase in ALT2 at both doses and time points and there was a concurrent increase in ALT2 ribonucleic acid at 24 and 72 hr. The ALT isoenzyme response assessed by an activity assay showed an increase in ALT2. The increases in liver ALT were associated with an increase in liver glycogen and there was no hepatocellular necrosis. There was an increase in total serum ALT activity, although serum isoenzymes were not evaluated. Thus, the authors demonstrated that dexamethasone induced increases in hepatic and serum ALT, which reflect a hepatocellular progluconeogenic metabolic adaptive response.

Published

2012

23. Best practices for evaluation of bone marrow in nonclinical toxicity studies.

Author

Reagan WJ, Irizarry-Rovira A, Poitout-Belissent F, Bolliger AP, Ramaiah SK, Travlos G, Walker D, Bounous D, and Walter G

Abstract

This manuscript is intended to provide a best practice approach to accurately and consistently assess toxicant-induced bone marrow effects of test articles. In nonclinical toxicity studies, complete blood count data in conjunction with the histological examination of the bone marrow are recommended as the foundation for assessing the effect of test articles on the hematopoietic system. This approach alone can be used successfully in many studies. However, in some situations it may be necessary to further characterize effects on the different hematopoietic lineages, either by cytological or flow cytometric evaluation of the bone marrow. Both modalities can be used successfully, and which one is selected will depend on the expertise, preference of the facility, and the nature of the change in the bone marrow. Other specialized techniques such as clonogenic assays or electron microscopy are used rarely to further characterize hematotoxicity. The indications and techniques to successfully employ histological, cytological, or flow cytometric evaluation as well as clonogenic assays and electron microscopy are reviewed., (© 2011 by the Authors, Reprinted by Permission of SAGE Publications Inc.)

Published

2011

24. Troponin as a biomarker of cardiac toxicity: past, present, and future.

Author

Reagan WJ

Subjects

Animals, Animals, Laboratory, Biomarkers blood, Cardiomyopathies chemically induced, Drug Evaluation, Preclinical trends, Drug-Related Side Effects and Adverse Reactions, Heart drug effects, Myocardium pathology, Risk Assessment, Species Specificity, Xenobiotics adverse effects, Cardiomyopathies blood, Drug Evaluation, Preclinical methods, Myocardium metabolism, Troponin T blood

Abstract

Cardiac troponin (cTn) is a sensitive and specific biomarker for assessing cardiac damage and should be utilized in drug safety assessment. Lactate dehydrogenase and creatine kinase isoenzyme analyses have historically been used in pre-clinical toxicity testing to assess cardiac injury, but since these assays are less sensitive and specific than cTn, isoenzyme analyses, as determined by the manual electrophoretic technique, are no longer warranted. Commercial cTn assays developed for humans do not have the same immunoreactivity and functional sensitivity in the common pre-clinical testing species, so it is important to show that the assay that is chosen is appropriate for the pre-clinical species being assessed. The kinetics of the cTn response depends on the dose and frequency of test article administration as well as the mechanism of the cardiac injury induced by the test article. Cardiac troponin should be used in the assessment of classes of compound that have previously been shown to induce cardiac necrosis or if cardiac necrosis is identified histologically with a novel compound. Next generation high sensitivity cTn assays are being developed and the low levels of cTn detected with these assays may be an early sign of possibly reversible damage to the heart.

Published

2010

25. A translational approach to detecting drug-induced cardiac injury with cardiac troponins: consensus and recommendations from the Cardiac Troponins Biomarker Working Group of the Health and Environmental Sciences Institute.

Author

Berridge BR, Pettit S, Walker DB, Jaffe AS, Schultze AE, Herman E, Reagan WJ, Lipshultz SE, Apple FS, and York MJ

Subjects

Animals, Cardiomyopathies blood, Clinical Trials as Topic, Cooperative Behavior, Drug Evaluation, Preclinical, Drug-Related Side Effects and Adverse Reactions, Education, Humans, Interdisciplinary Communication, Monitoring, Physiologic, Predictive Value of Tests, Risk Assessment, Cardiomyopathies chemically induced, Cardiomyopathies diagnosis, Troponin blood

Abstract

Cardiac troponins (cTns) are established biomarkers of ischemic heart disease in humans. However, their value as biomarkers of cardiac injury from causes other than ischemic heart disease is now being explored, particularly in drug development. In a workshop sponsored by the Cardiac Troponin Biomarker Working Group of the Health and Environmental Sciences Institute, preclinical, clinical, and regulatory scientists discussed the application of cTns in their respective environments, issues in translating the preclinical application of cTn to clinical studies, and gaps in our understanding of cTn biology and pathobiology. Evidence indicates that cTns are sensitive and specific biomarkers of cardiac injury from varying causes in both animals and humans. Accordingly, monitoring cTns can help ensure patient safety during the clinical evaluation of new drugs. In addition, preclinical characterization of cardiac risk and cTns as biomarkers of that risk can guide relevant clinical application and interpretation. We summarize here the outcomes of the workshop which included consensus statements, recommendations for further research, and a proposal for a cross-disciplinary group of clinical, regulatory, and drug development scientists to collaborate in such research.

Published

2009

26. Alanine aminotransferase isoenzymes: molecular cloning and quantitative analysis of tissue expression in rats and serum elevation in liver toxicity.

Author

Yang RZ, Park S, Reagan WJ, Goldstein R, Zhong S, Lawton M, Rajamohan F, Qian K, Liu L, and Gong DW

Subjects

Alanine Transaminase blood, Amino Acid Sequence, Animals, Cloning, Molecular, Conserved Sequence, DNA, Complementary genetics, Humans, Isoenzymes blood, Liver enzymology, Male, Mice, Mitochondria, Liver enzymology, Molecular Sequence Data, Polymerase Chain Reaction, Rats, Alanine Transaminase genetics, Gene Expression Regulation, Enzymologic, Isoenzymes genetics, Liver pathology

Abstract

Unlabelled: The elevation of serum alanine aminotransferase (ALT) is regarded as an indicator of liver damage based on the presumption that ALT protein is specifically and abundantly expressed in the liver. However, ALT elevation is also observed in non-liver injury conditions (for example, muscle injury) and in apparently healthy people. Conversely, serum ALT activity is normal in many patients with confirmed liver diseases (for example, cirrhosis and hepatitis C infection). To improve the diagnostic value of the ALT assay and to understand the molecular basis for serum ALT changes in various pathophysiological conditions, we have cloned rat ALT isoenzyme ALT1 and ALT2 complementary DNAs (cDNAs), examined their tissue expressions at the messenger RNA and protein levels, and determined ALT1 and ALT 2 serum levels in response to liver damage in rodents. Quantitative real-time polymerase chain reaction (qRT-PCR) analysis shows that ALT1 messenger RNA is widely distributed and mainly expressed in intestine, liver, fat tissues, colon, muscle, and heart, in the order of high to low expression level, whereas ALT2 gene expression is more restricted, mainly in liver, muscle, brain, and white adipose tissue. The tissue distribution pattern of ALT1 and ALT2 proteins largely agrees with their messenger RNA expression. Interestingly, hepatic ALT2 protein is approximately four times higher in male rats than in female rats. In addition, ALT isoenzymes distribute differentially at the subcellular level in that ALT1 is a cytoplasmic protein and ALT2 a mitochondrial protein, supporting bioinformatic prediction of mitochondrial localization of ALT2., Conclusion: Using animal models of hepatoxicity induced by carbon tetrachloride and acetaminophen, we found that both serum ALT1 and ALT2 protein levels were significantly elevated and correlated with ALT activity, providing, for the first time, the molecular basis for the elevated total serum ALT activity.

Published

2009

27. Expression, purification, and initial characterization of human alanine aminotransferase (ALT) isoenzyme 1 and 2 in High-five insect cells.

Author

Liu L, Zhong S, Yang R, Hu H, Yu D, Zhu D, Hua Z, Shuldiner AR, Goldstein R, Reagan WJ, and Gong DW

Subjects

Alanine Transaminase chemistry, Animals, Base Sequence, Blotting, Western, DNA Primers, Genetic Vectors, Humans, Hydrogen-Ion Concentration, Isoenzymes chemistry, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Spodoptera, Temperature, Alanine Transaminase genetics, Alanine Transaminase isolation & purification, Isoenzymes genetics, Isoenzymes isolation & purification

Abstract

Alanine aminotransferase (ALT) is a key enzyme for gluconeogenesis as well as a widely used serum marker for liver injury. We have identified two ALT isoenzymes, ALT1 and ALT2, which are encoded by separate genes. In this study, we described the expression, purification and initial characterization of human ALT1 and ALT2 proteins in High-five insect cells. Human ALT1 and ALT2 were expressed as His-tagged fusion proteins by recombinant baculovirus in insect cells and purified into homogeneity in one step by using immobilized Ni2+-affinity chromatography. Tag-free ALT1 and ALT2 were obtained by cleavage of enterokinase digestion and used for initial characterization of the enzymes. The specific ALT activity of purified fusion or His-tag-removed ALT1 was about 15-fold higher than that of ALT2 and their enzymatic activities decreased quickly at 37 degrees C and -20 degrees C, but were well preserved at -80 degrees C. Nevertheless, the ALT1 and ALT2 activities remained stable in a buffer containing 25% glycerol. The pH profile was similar between hALT1 and hALT2 in that both enzymes remained fully active between pH 6.5 and 8.0. The purified ALT recombinant proteins can not only be used as a reference protein standard for the ALT assay in clinical chemistry, but also will be useful for understanding the biochemical and biological significance of the isoenzymes and for developing ALT isoform-specific assays for clinical or preclinical diagnostic use.

Published

2008

28. Optimization and validation of a flow cytometric method for immunophenotyping peripheral blood lymphocytes from cynomolgus monkeys (Macaca fascicularis).

Author

Baker DL, Finco-Kent DL, Reagan WJ, Conklyn MJ, and Kawabata TT

Subjects

Animals, Flow Cytometry methods, Immunophenotyping methods, Reproducibility of Results, Flow Cytometry veterinary, Immunophenotyping veterinary, Lymphocytes cytology, Macaca fascicularis blood

Abstract

Background: Guidelines published by the Food and Drug Administration and Center for Human Medicinal Products describe the need to assess immunotoxic effects in nonclinical studies that evaluate drug toxicity, including the use of immunophenotyping to measure immunotoxicity. We are not aware of previous studies, however, that have validated methods for immunophenotyping peripheral blood lymphocyte subsets in whole blood samples from cynomolgus monkeys., Objective: The purpose of this study was to optimize and validate a flow cytometric assay for immunophenotyping lymphocytes in the peripheral blood of cynomolgus monkeys., Methods: A series of prevalidation experiments were done to determine optimal reagents, volumes, timing, and other procedural details of the flow cytometric assay. Using the optimized method, we then determined precision, interindividual variation, laboratory-to-laboratory variability, and sample stability. Stabilized human blood was used as a positive control for staining, processing, and analysis. The percentage and number of pan-T cells (CD3+), T-helper cells (CD3+4+), T cytotoxic/suppressor cells (CD3+8+), natural killer cells (CD3-16+), and B-cells (CD3-20+) were determined in 146 male and 140 female, clinically healthy monkeys and reference intervals were calculated., Results: By doing 4-color staining with a lyse-wash method, intra- and interassay precision were <5% for all lymphocyte subsets. Variability between technicians and laboratories was minimal (CVs<3%). Samples were stable for up to 24 hours after staining and fixing., Conclusions: The validated method is extremely robust and can be performed under good laboratory practice conditions to support nonclinical studies. Reference intervals for lymphocyte subsets were similar to those previously reported.

Published

2008

29. Influence of urine pH on accurate urinary protein determination in Sprague-Dawley rats.

Author

Reagan WJ, VanderLind B, Shearer A, and Botts S

Subjects

Ammonium Chloride pharmacology, Animals, Hydrogen-Ion Concentration, Male, Proteinuria chemically induced, Rats, Rats, Sprague-Dawley, Reagent Strips, Sodium Bicarbonate pharmacology, Urinalysis instrumentation, Proteinuria veterinary, Urine chemistry

Abstract

Background: Rat urinary protein concentration is commonly measured during safety assessment studies to evaluate potential drug-induced nephrotoxicity. It has been reported that impregnated reagent test strips (dipsticks) can yield false-positive urinary protein results for alkaline urine samples., Objective: The objective of this study was to determine if urinary dipsticks accurately assess protein concentrations, especially in alkaline rat urine., Methods: Ten male Sprague-Dawley rats were treated with 2% sodium bicarbonate and 2% ammonium chloride to alkalinize and acidify the urine, respectively. Urine pH was measured in treated and control rats using a pH meter and urinary dipsticks with the Clinitek 500. Quantitative urinary protein results were compared to urinary dipstick protein evaluations obtained with the Clinitek 500 and sulfosalicylic acid precipitation test methods., Results: The urinary dipstick pH measurement had a very high correlation (r = .98) with the pH meter technique. Samples with alkaline pH (>or=7.5) analyzed for protein by dipstick analysis were in complete agreement 34.7% of the time with the quantitative technique, which was very similar to the 39.3% agreement for samples with neutral and acidic pH (

Published

2007

30. cDNA cloning, expression, purification, distribution, and characterization of biologically active canine alanine aminotransferase-1.

Author

Rajamohan F, Nelms L, Joslin DL, Lu B, Reagan WJ, and Lawton M

Subjects

Alanine Transaminase isolation & purification, Alanine Transaminase metabolism, Amino Acid Sequence, Animals, Base Sequence, Cloning, Molecular, DNA, Complementary chemistry, Dogs, Humans, Liver cytology, Liver metabolism, Mass Spectrometry, Mice, Molecular Sequence Data, Rats, Recombinant Fusion Proteins analysis, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins isolation & purification, Sequence Alignment, Alanine Transaminase genetics

Abstract

Alanine aminotransferase (ALT) is a pyridoxal enzyme found mainly in the liver and kidney, but also in small amounts in the heart, muscle, fat, and brain. Serum aminotransferase activities have been used broadly as surrogate markers for tissue injury and disease in human and veterinary clinical settings and in safety assessment of chemicals and pharmaceuticals. Because of its relative abundance in liver, increased serum ALT activity is generally considered indicative of liver damage. Two ALT isoenzymes, ALT1 and ALT2, are known and have been cloned and sequenced from human, rat, and mouse. In this study, we have cloned the complementary DNA encoding the canine orthologue of ALT1 (cALT1). The complete cDNA sequence comprised 1852 bases and contained a 1485-base open reading frame, which encodes a polypeptide of 494 amino acid residues. Canine ALT1 shares 87.7, 87.2, and 87.0% amino acid identity to its human, mouse, and rat orthologues, respectively. The cDNA was expressed in Escherichia coli, with a N-terminal His (6x) tag, and the recombinant enzyme was purified using immobilized metal-affinity chromatography. The final yield of the purified recombinant cALT1 was greater than 5mg/L culture. The alanine transaminase activity of purified cALT1 was 229.81U/mg protein, which is approximately 38-fold higher than that of total soluble recombinant E. coli cell lysate, confirming that the enzyme is a functional ALT. Evaluation of various canine tissues by RT-PCR revealed that the level of ALT1 expression is in the order of: heart>liver>fat approximately brain approximately gastrocnemius>kidney. The purified cALT1 will be helpful to develop isoenzyme-specific anti-bodies, which could further improve the diagnostic resolution of current ALT assays in drug safety studies.

Published

2006

31. Cardiac troponin I is a sensitive, specific biomarker of cardiac injury in laboratory animals.

Author

O'Brien PJ, Smith DE, Knechtel TJ, Marchak MA, Pruimboom-Brees I, Brees DJ, Spratt DP, Archer FJ, Butler P, Potter AN, Provost JP, Richard J, Snyder PA, and Reagan WJ

Subjects

Animal Diseases diagnosis, Animals, Biomarkers blood, Dogs, Female, Heart Diseases blood, Luminescent Measurements standards, Male, Mice, Myocardium chemistry, Rats, Sensitivity and Specificity, Troponin T blood, Animal Diseases blood, Animals, Laboratory blood, Heart Diseases veterinary, Luminescent Measurements veterinary, Troponin I blood

Abstract

This study directly demonstrates that cardiac troponin I (cTnI) is a sensitive, specific, and persistent biomarker in laboratory animals. Histopathological and pathophysiological cardiac changes in dogs, rats and mice correlated with increased serum cTnI with various cardiac inotropic agents, and cardiotoxic drugs and with cardiac arrhythmias, tachycardia, cardiac effusion with dyspnoea, and ageing. A comparison of six immunoassays for cTnI and cardiac troponin T (cTnT) to detect and monitor cardiac injury in a rodent model indicated that enzyme-linked immunosorbent (Life Diagnostics Inc and TriChem Resources Inc, West Chester, Philadelphia, USA) and Immulite (Diagnostic Products Corporation, Llanberis, UK) assays had low sensitivity and less than 1% of the dynamic range of Centaur (Bayer Healthcare Diagnostics, Newbury, UK) cTnI and Elecsys (Roche Diagnostics, Basel, Switzerland) and M8 (Bioveris Europe, Whitney, UK) cTnT assays. In dogs, however, the Immulite assay was effective and correlated with the Centaur. Serum concentrations were highly correlated but 10-fold lower for cTnT compared with cTnI with cardiac injury. Centaur assay also detected cTnI in myocardium from marmosets, swine, cattle, and guinea pigs, indicating it to be candidate cardiac biomarker for these species as well. Purified rat cTnI was 50% more reactive than purified human cTnI in the Centaur assay. In the rat, an age- and gender-dependent variation in serum cTnI was found. Male rats aged six and eight months had a 10-fold greater serum cTnI than age-matched females and three-month-old rats. These increases correlated with minimal histopathological change. Isoproterenol-induced serum cTnI increased up to 760-fold the minimal detectable concentration of 0.07 microg/L, within 4-6 h and decreased with a half-life of 6 h, with an expected return to baseline of 60 h. Severity of histopathological change correlated with serum cTnI during the ongoing injury.

Published

2006

32. Inoculation of two genotypes of Hemobartonella felis (California and Ohio variants) to induce infection in cats and the response to treatment with azithromycin.

Author

Westfall DS, Jensen WA, Reagan WJ, Radecki SV, and Lappin MR

Subjects

Anaplasmataceae genetics, Anaplasmataceae Infections blood, Anaplasmataceae Infections drug therapy, Anemia drug therapy, Anemia microbiology, Anemia veterinary, Animals, Cat Diseases blood, Cats, DNA, Bacterial chemistry, DNA, Bacterial genetics, Female, Hematocrit veterinary, Leukocyte Count veterinary, Lymphocyte Count veterinary, Male, Polymerase Chain Reaction, Specific Pathogen-Free Organisms, Anaplasmataceae pathogenicity, Anaplasmataceae Infections veterinary, Anti-Bacterial Agents therapeutic use, Azithromycin therapeutic use, Cat Diseases drug therapy, Cat Diseases microbiology

Abstract

Objectives: To describe clinical and laboratory findings associated with cats experimentally infected by inoculation with the 2 recognized genotypes of Hemobartonella felis (small variant, Hfsm; large variant, Hflg) and to determine the response of cats to treatment with azithromycin., Animals: 18 young adult domestic shorthair cats of both sexes., Procedures: Cats were inoculated with H felis and monitored weekly, using CBC counts and a polymerase chain reaction (PCR) designed to detect both genetic variants of H felis. Beginning 26 days after inoculation, 11 cats were administered azithromycin (15 mg/kg of body weight, PO, q 12 h, for 7 days)., Results: Inoculation resulted in coinfection with Hflg and Hfsm, and both variants were detected by PCR. Clinical abnormalities and anemia were most severe in Hflg- and dual-infected cats. Results of PCR and CBC were positive for H felis in 112/112 (100%) and 42/112 (37.5%), respectively, samples collected after inoculation. Administration of azithromycin had little effect on clinical variables, including anemia. All cats, regardless of treatment with azithromycin, had positive results for the PCR at the end of the study period., Conclusions and Clinical Relevance: In these cats, Hflg was more pathogenic than Hfsm, and coinfection with both variants was detected. Results of the PCR were superior to results of CBC for detecting infection with H felis. Azithromycin administered at the dose and duration reported here was not efficacious for the treatment of cats with hemobartonellosis.

Published

2001

33. Use of a polymerase chain reaction assay to detect and differentiate two strains of Haemobartonella felis in naturally infected cats.

Author

Jensen WA, Lappin MR, Kamkar S, and Reagan WJ

Subjects

Anaplasmataceae chemistry, Anaplasmataceae genetics, Anaplasmataceae Infections blood, Anaplasmataceae Infections microbiology, Animals, Base Sequence, Blood Cell Count veterinary, Cat Diseases blood, Cat Diseases diagnosis, Cats, DNA, Bacterial genetics, Molecular Sequence Data, Polymerase Chain Reaction methods, Sequence Alignment, Sequence Homology, Nucleic Acid, Anaplasmataceae classification, Anaplasmataceae Infections veterinary, Cat Diseases microbiology, Polymerase Chain Reaction veterinary

Abstract

Objective: To develop a polymerase chain reaction (PCR) assay that detects and differentiates the Ohio strain of Haemobartonella felis (H. felis-OH) and the California strain of H. felis (H. felis-CA) and to apply the assay to blood samples from cats with and without suspected haemobartonellosis (suspect and control cats, respectively)., Sample Population: 220 blood samples were examined; 82 were from suspect cats, and 138 were from control cats., Procedure: A PCR assay was designed to detect and differentiate H. felis-OH and H. felis-CA., Results: On the basis of PCR assay results, the overall prevalence of H. felis infection was 19.5% (43/220). Suspect cats (28.0%; 23/82) were significantly more likely than control cats (14.5%; 20/138) to be H. felis infected. Significantly greater numbers of suspect cats were H. felis-OH infected (12.2%, 9/82) or H. felis-OH and H. felis-CA infected (4.9%, 4/82) than control cats (0% [0/138] and 0.7% [1/138], respectively). Significantly more anemic cats were H. felis-OH infected (14.3%; 4/28) or H. felis-OH and H. felis-CA infected (7.1%; 2/28) than nonanemic cats (2.3% [3/128] and 0.8% [1/128], respectively). The PCR assay was more accurate than cytologic examination for detection of H. felis., Conclusions and Clinical Relevance: Haemobartonella felis infections are more common in cats than previously recognized. Haemobartonella felis-OH is apparently more pathogenic than H. felis-CA. The PCR assay is more accurate than cytologic examination for detection of H. felis infection and is an effective clinical tool for the detection and differentiation of both H. felis strains known to infect cats.

Published

2001

34. Effects of human intravenous immunoglobulin on canine monocytes and lymphocytes.

Author

Reagan WJ, Scott-Moncrieff C, Christian J, Snyder P, Kelly K, and Glickman L

Subjects

Animals, B-Lymphocytes immunology, Binding Sites, CD4-Positive T-Lymphocytes immunology, CD8-Positive T-Lymphocytes immunology, Cells, Cultured, Dogs, Erythrocytes physiology, Flow Cytometry, Fluorescent Antibody Technique, Indirect, Humans, Immunoglobulin Fab Fragments immunology, Immunoglobulin Fc Fragments immunology, Immunoglobulin G immunology, Immunoglobulins, Intravenous pharmacokinetics, Phagocytosis, Immunoglobulins, Intravenous pharmacology, Lymphocytes immunology, Monocytes immunology

Abstract

Objective: To evaluate interactions of human intravenous immunoglobulin (IVIG) with canine lymphocytes and monocytes., Sample Population: Heparinized blood samples from 4 clinically normal Beagles., Procedure: Binding ability of IVIG to canine lymphocytes and monocytes was measured by flow cytometry and an indirect immunofluorescent assay. Dual-staining fluorescent assays were done to determine lymphocyte subsets that bind IVIG. Competitive assays were done, using intact canine IgG and Fc fragments, and inhibition of binding was compared with that of F(ab)2 fragments. Ability of IVIG to inhibit phagocytosis of antibody-coated canine RBC also was determined, using a canine mononuclear cell phagocytic assay., Results: IVIG concentrations (10, 1, 0.1, and 0.01 mg/ml) bound to (mean+/-SD) 99.6+/-0.4, 92.4+/-6.1, 20.4+/-24.6 and 2.0+/-5.1 % of canine lymphocytes, respectively, Dual staining analyses with IVIG and canine lymphocyte markers indicated that IVIG bound to CD4, CD8, and B lymphocytes. The aforementioned 4 IVIG concentrations bound to 98.0+/-2.1, 85.5+/-13.5, 64.7+/-32.8, and 26.5+/-17.1 % of monocytes, respectively. Inhibition of IVIG (0.01 mg/ml) binding to monocytes was significant (P< 0.05) in the presence of 1 and 10 mg of canine IgG/ml and 1 mg of canine Fc fragments/ml. In the presence of F(ab')2 fragments of canine IgG, inhibition was not significant, suggesting that binding is Fc mediated. Co-culturing of monocytes, opsonized RBC, and the 4 concentrations of IVIG and no IVIG resulted in 11.8+/-5.1, 27.7+/-12.3, 31.8+15.1, 53.8+/-6.7, and 45 + 12% of the monocytes containing RBC, respectively. Phagocytosis inhibition was significant (P < 0.05) at an IVIG concentration of 10 mg/ml., Conclusions: IVIG binds to canine lymphocytes and monocytes; binding to the latter is Fc mediated. IVIG also inhibits Fc-mediated phagocytosis of antibody-coated RBC., Clinical Relevance: Owing to its ability to inhibit Fc-mediated phagocytosis of antibody-coated RBC, IVIG may be an effective short-term treatment for dogs with immune-mediated hemolytic anemia.

Published

1998

35. Use of laser flare-cell photometry to count anterior chamber canine leukocytes and latex beads in vitro.

Author

Krohne SG, Reagan WJ, and Welch PM

Subjects

Animals, Anterior Chamber chemistry, Anterior Chamber pathology, Dogs, In Vitro Techniques, Lasers, Leukocyte Count methods, Linear Models, Microspheres, Neutrophils cytology, Photometry methods, Photometry veterinary, Reproducibility of Results, Serum Albumin, Bovine, Uveitis, Anterior pathology, Anterior Chamber cytology, Dog Diseases pathology, Leukocyte Count veterinary, Uveitis, Anterior veterinary

Abstract

Objective: To determine whether the cell measuring function of a laser flare-cell photometer is accurate and reproducible, using an in vitro model., Sample Population: Leukocytes from 8 clinically normal Beagles., Procedure: Latex beads 11.9 and 6.4 microm in diameter were used to simulate canine WBC and RBC, respectively. Beads were diluted to known concentrations, placed in a model eye, and counted by use of the laser flare-cell photometer. A range of protein diluents from 0 to 2,000 mg/dl was used to suspend beads and simulate anterior uveitis, when cells and protein would be in the aqueous humor. A similar series of experiments were repeated, using leukocytes isolated from the blood of Beagles., Results: The laser flare-cell photometer can count 6.4-microm beads reproducibly and linearly up to a total of 510 cells/mm3, and 11.9-microm beads up to 1,300 cells/mm3 over a protein range of 0 to 2,000 mg/dl. The instrument can also count canine leukocytes reproducibly and linearly up to 1,300 cells/mms over that protein range., Conclusions and Clinical Relevance: Cell and bead sizes and concentrations and protein concentrations were chosen to mimic the range observed in dogs with uveitis. Because the laser flare-cell photometer accurately counted these cells in a range of protein concentrations in the model eye, it has the potential for use in noninvasive quantitative evaluation and monitoring of uveitis in dogs.

Published

1998

36. Human intravenous immunoglobulin therapy.

Author

Scott-Moncrieff JC and Reagan WJ

Subjects

Anemia, Hemolytic, Autoimmune immunology, Anemia, Hemolytic, Autoimmune therapy, Anemia, Hemolytic, Autoimmune veterinary, Animals, Autoimmune Diseases drug therapy, Autoimmune Diseases immunology, Dog Diseases blood, Dog Diseases immunology, Dogs, Humans, Immunization, Passive methods, Immunoglobulins, Intravenous administration & dosage, Immunoglobulins, Intravenous adverse effects, Primary Myelofibrosis immunology, Primary Myelofibrosis therapy, Primary Myelofibrosis veterinary, Thrombocytopenia immunology, Thrombocytopenia therapy, Thrombocytopenia veterinary, Autoimmune Diseases veterinary, Dog Diseases therapy, Immunization, Passive veterinary, Immunoglobulins, Intravenous therapeutic use

Abstract

Human intravenous immunoglobulin (hIVIG) is a preparation of normal polyspecific IgG obtained from the plasma of healthy blood donors. Although purified immunoglobulins were initially developed for treatment of primary immunodeficiency syndromes, they have since been documented to be effective in the treatment of some immune-mediated diseases such as immune-mediated thrombocytopenia purpura and autoimmune hemolytic anemia. Blockade of Fc receptors on mononuclear phagocytic cells has been proposed as the most likely mechanism for the rapid early response to hIVIG treatment. Human IVIG has been used to treat canine immune-mediated hemolytic anemia (IMHA), anemia with myelofibrosis, and immune-mediated thrombocytopenia. Doses from 0.5 to 1.5 g/kg may be effective, although most studies have used a dose of 1 g/kg. Human IVIG is administered as an intravenous infusion over 6 to 12 hours, and dogs should be carefully monitored for adverse reactions during administration. The possibility of a increased risk of thromboembolism should be considered when undertaking hIVIG treatment. The safety of multiple treatments of hIVIG has not been established. In most dogs with IMHA, benefit may be limited to short-term improvement in hematocrit, which may allow time for other treatment modalities to become effective. Dogs with nonregenerative anemia and associated myelofibrosis may have longer-term responses to hIVIG treatment.

Published

1997

37. Intravenous administration of human immune globulin in dogs with immune-mediated hemolytic anemia.

Author

Scott-Moncrieff JC, Reagan WJ, Snyder PW, and Glickman LT

Subjects

Anemia, Hemolytic, Autoimmune therapy, Animals, Dogs, Erythrocyte Count veterinary, Female, Hematocrit veterinary, Humans, Immunoglobulins, Intravenous administration & dosage, Immunoglobulins, Intravenous adverse effects, Immunosuppressive Agents therapeutic use, Male, Platelet Count veterinary, Prospective Studies, Pulmonary Embolism etiology, Pulmonary Embolism veterinary, Reticulocytes drug effects, Thrombocytopenia etiology, Thrombocytopenia veterinary, Treatment Outcome, Anemia, Hemolytic, Autoimmune veterinary, Dog Diseases therapy, Immunoglobulins, Intravenous therapeutic use

Abstract

Objective: To evaluate the efficacy and safety of intravenous administration of human immune globulin in the treatment of dogs with immune-mediated hemolytic anemia (IMHA)., Design: Prospective clinical trial., Animals: 10 dogs with confirmed primary IMHA that had failed to respond to conventional immunosuppressive treatment (administration of prednisone and cyclophosphamide or azathioprine)., Procedure: Diagnosis of IMHA was confirmed by detecting spherocytosis or autoagglutination in blood smears and by excluding secondary causes of IMHA. Dogs were treated with human immune globulin (1 g/kg [0.45 g/lb] of body weight, i.v.) during a 6- to 12-hour period. Prednisone treatment was continued in all dogs, and cyclophosphamide treatment was continued in 4., Results: Median duration of prior immunosuppressive treatment was 12.5 days. Short-term response could not be evaluated in 2 dogs, because they were given blood transfusions within 7 days after immune globulin treatment. However, there was a significant increase in mean Hct and hemoglobin concentration in 8 other dogs from day 0 to 28 after treatment. Five dogs had clinically meaningful responses to treatment. Three dogs were alive 12 months after treatment. There were not any adverse effects that could be definitively attributed to immune globulin treatment; however, thrombocytopenia was observed in 6 dogs after treatment, and evidence of thromboembolism was detected at necropsy in 5 of the 7 dogs that died., Clinical Implications: Human immune globulin may be useful for short-term stabilization of some dogs with IMHA; however, it did not appear to improve long-term survival.

Published

1997

38. Antibodies to canine granulocyte colony-stimulating factor induce persistent neutropenia.

Author

Reagan WJ, Murphy D, Battaglino M, Bonney P, and Boone TC

Subjects

Animals, Blotting, Western, Bone Marrow pathology, Dogs, Enzyme-Linked Immunosorbent Assay, Erythrocytes pathology, Female, Granulocytes pathology, Hyperplasia pathology, Hyperplasia veterinary, Necrosis pathology, Necrosis veterinary, Neutropenia etiology, Neutropenia immunology, Rabbits, Recombinant Proteins adverse effects, Recombinant Proteins immunology, Antibodies immunology, Granulocyte Colony-Stimulating Factor adverse effects, Granulocyte Colony-Stimulating Factor immunology, Neutropenia veterinary

Abstract

A severe persistent neutropenia developed in a rabbit that was injected intradermally with 120, 60, 60, and 120 micrograms of recombinant canine granulocyte colony-stimulating factor (cG-CSF) on days 1, 22, 31, and 44, respectively. The neutropenia was present from day 44 to day 205. The nadir of the neutropenia (60 cells/microliters) occurred in conjunction with peak antibody titer (640,000) to cG-CSF on day 58. The immune antiserum from this rabbit reacted positively for cG-CSF on Western blot analysis. The immune antiserum also neutralized the activity of cG-CSF. On day 160, examination of the bone marrow showed marked granulocytic hypoplasia and mild erythroid hyperplasia. On day 205, the rabbit was still neutropenic (430 cells/microliters), even though the last injection of cG-CSF was given 161 previously. Necropsy on day 205 showed that there was still mild granulocytic hypoplasia with mild erythroid hyperplasia. Because of the lack of any inflammatory foci found at necropsy and the granulocytic hypoplasia, it was thought that the neutropenia was most likely due to decreased production and was not a consumptive process. It is hypothesized that the antibody that was produced to cG-CSF neutralized the effect of endogenous rabbit granulocyte colony-stimulating factor and prevented the normal proliferation and maturation of the rabbit neutrophils.

Published

1995

39. Treatment of nonregenerative anemia with human gamma-globulin in dogs.

Author

Scott-Moncrieff JC, Reagan WJ, Glickman LT, DeNicola DB, and Harrington D

Subjects

Anemia, Hypochromic therapy, Anemia, Macrocytic therapy, Animals, Biopsy, Needle veterinary, Bone Marrow pathology, Dogs, Female, Humans, Infusions, Intravenous veterinary, Prednisone therapeutic use, Anemia, Hypochromic veterinary, Anemia, Macrocytic veterinary, Dog Diseases therapy, Immunization, Passive veterinary, gamma-Globulins administration & dosage

Abstract

Five dogs with nonregenerative anemia were treated with human immunoglobulin as a 12-hour IV infusion, at dosages ranging from 0.5 to 1.5 g/kg of body weight. All dogs had a rapid response to treatment, with reticulocytosis within 1 to 4 days and a substantial increase in hematocrit within 3 to 8 days of treatment. In 2 of 5 dogs, the hematocrit returned to values within reference range and remained in the reference range for 8 to 14 months after treatment, despite discontinuing or tapering prednisone treatment to a low dose. In 3 of 5 dogs, the hematocrit did not return to the reference range. In 1 of these 3 dogs, the hematocrit remained at the new, increased value (26 to 28%) for 248 days after treatment, at which time the dog was euthanatized. In the other 2 dogs, the hematocrit had decreased to pretreatment values by 52 days after treatment. Retreatment of these 2 dogs resulted in a similar, but blunted, response to human immunoglobulin. Human immunoglobulin may be an effective treatment for some dogs with immune-mediated anemia that fail to respond to conventional treatment.

Published

1995

40. Evaluation of in vitro cytotoxicity of nonsteroidal anti-inflammatory drugs against canine tumor cells.

Author

Knapp DW, Chan TC, Kuczek T, Reagan WJ, and Park B

Subjects

Animals, Aspirin toxicity, Cell Division drug effects, Cell Line, Cell Survival drug effects, Dogs, Drug Screening Assays, Antitumor veterinary, Hydroxyurea analogs & derivatives, Hydroxyurea toxicity, Indomethacin toxicity, Piroxicam toxicity, Tumor Cells, Cultured, Tumor Stem Cell Assay veterinary, Anti-Inflammatory Agents, Non-Steroidal toxicity, Antineoplastic Agents toxicity, Carcinoma, Squamous Cell veterinary, Carcinoma, Transitional Cell veterinary, Dog Diseases, Melanoma veterinary, Sarcoma veterinary

Abstract

Piroxicam and other nonsteroidal anti-inflammatory drugs (NSAID) have antitumor activity against naturally acquired cancer in dogs and human beings, and against experimentally induced tumors in rodents. We are investigating potential mechanisms of NSAID antitumor activity. The direct cytotoxicity of piroxicam indomethacin, and aspirin against 4 canine tumor cell lines (transitional cell carcinoma, squamous cell carcinoma, melanoma, and soft tissue sarcoma) was determined in short-term growth rate assays and in clonogenic assays. Piroxicam was evaluated alone and in combination with the lipoxygenase inhibitor zileuton, and in combination with the chemotherapeutic agents cisplatin and carboplatin. The 50% inhibitory concentrations (IC50) against melanoma cells in short-term growth rate assays were: 530 microM piroxicam, 180 microM indomethacin, and greater than 1 mM aspirin. These IC50 values were over 10 times greater than serum concentrations of these drugs that could safely be achieved in vivo. The IC50 of zileuton combined with piroxicam (280 microM) was not different from the IC50 of zileuton alone (230 microM; ANOVA P = 0.47) in melanoma cells. Similarly, addition of piroxicam did not alter the IC50 of either cisplatin (1.6 microM) or carboplatin (6.1 microM). These results suggest that NSAID, at serum concentrations achievable in vivo, do not have direct cytotoxicity against canine tumor cells tested. It is unlikely that the in vivo antitumor activity of NSAID is attributable to a direct cytotoxic effect.

Published

1995

41. Eccentrocytosis in equine red maple leaf toxicosis.

Author

Reagan WJ, Carter C, and Turek J

Published

1994

42. A review of myelofibrosis in dogs.

Author

Reagan WJ

Subjects

Animals, Dog Diseases blood, Dog Diseases pathology, Dogs, Primary Myelofibrosis etiology, Primary Myelofibrosis pathology, Dog Diseases etiology, Primary Myelofibrosis veterinary

Abstract

Myelofibrosis is a proliferative response of the bone marrow fibroblasts. Myelofibrosis can be classified as primary or secondary depending on the underlying etiology. Primary myelofibrosis is a myeloproliferative disorder in humans in which there is a clonal proliferation of a pluripotent stem cell. Hemopathology includes finding nucleated red blood cells and immature granulocytes in the circulation, extramedullary hematopoiesis, and myelofibrosis. The proliferation of the bone marrow fibroblasts is not clonal in origin. To the best of this author's knowledge, this type of myelofibrosis has not been reported to occur naturally in the dog. Secondary myelofibrosis has been reported in the dog associated with neoplastic conditions, irradiation, congenital hemolytic anemias, and a variety of unknown etiologies. It has been shown in some cases of myelofibrosis that there is often concurrent bone marrow necrosis. Bone marrow necrosis has been documented in dogs with Ehrlichiosis and septicemia, and associated with drug treatment, including estrogens and cephalosporins. It is though that this necrosis is due to the destruction of the bone marrow microvasculature and/or hematopoietic elements. Release of growth factors by inflammatory cells may lead to the subsequent fibroblast proliferation. Several cases of secondary myelofibrosis in female laboratory beagles have been recently observed. These dogs present with a severe nonregenerative anemia and often a mild neutropenia with varying degrees of myelofibrosis in the bone marrow. Some animals have had concurrent bone marrow necrosis. At this time, the exact etiology is unknown.

Published

1993

43. Flow cytometric analysis of feline reticulocytes.

Author

Reagan WJ, Vap LM, and Weiser MG

Subjects

Anemia blood, Animals, Benzothiazoles, Female, Fluorescent Dyes, Male, Quinolines, Reproducibility of Results, Thiazoles, Anemia veterinary, Cat Diseases blood, Cats blood, Erythrocyte Count veterinary, Flow Cytometry veterinary, Reticulocytes

Abstract

Hemolytic anemia was induced in five Domestic Shorthair cats (four adult males and one spayed female obtained from a breeding colony at Colorado State University, CO), and blood samples were analyzed from five other cats (two castrated male Domestic Shorthairs, one castrated male Domestic Longhair, one castrated male Persian, and one spayed female Siamese presented to the Veterinary Teaching Hospital at Colorado State University for miscellaneous problems). Blood samples taken from these cats had percentages of aggregate reticulocytes that ranged from 0% to 14.5% as determined by manual counting and were used to identify the best technique for staining cat reticulocytes for flow cytometric analysis. The best technique was mixing a blood sample (1/2,000 dilution) with 0.2 micrograms thiazole orange in 1 ml of diluent and incubating the mixture in the dark at room temperature for 30 to 60 minutes. The percentage of reticulocytes determined by flow cytometry correlated well (r = 0.88) with manually determined aggregate reticulocyte percentages; no significant differences were observed between the two techniques (P > 0.05). For the conditions used, punctate reticulocytes were not detected by flow cytometry. Samples with very high platelet numbers and very low packed cell volumes may show falsely elevated percentages of reticulocytes as determined by flow cytometry. The reproducibility of the flow cytometric technique was good; the coefficient of variation ranged from 4.8% to 17.9% in two samples with two different times of incubation. Staining of cat aggregate reticulocytes with thiazole orange and use of flow cytometric quantification is a reproducible technique that has a good correlation with the manual reticulocyte counting method.

Published

1992

44. Cells of chemically induced tumors differentially express major histocompatibility complex class I antigens.

Author

Reagan WJ, Pardi D, and Callahan GN

Subjects

Animals, Gene Expression Regulation, Neoplastic physiology, Genes, MHC Class I physiology, H-2 Antigens immunology, H-2 Antigens physiology, Histocompatibility Antigens Class I genetics, Methylcholanthrene, Mice, Mice, Inbred BALB C, Mice, Nude, Neoplasm Transplantation, Neoplasms, Experimental chemically induced, Neoplasms, Experimental pathology, Phenotype, Precipitin Tests, Radioimmunoassay, Tumor Cells, Cultured, Histocompatibility Antigens Class I physiology, Neoplasms, Experimental immunology

Abstract

Several recent studies have indicated that alterations in expression of major histocompatibility complex (MHC) antigens by tumor cells affects the ability of the host to mount an effective antitumor immune response. To investigate whether newly induced tumors frequently exhibit altered MHC antigen expression, we used methylcholanthrene to induce a series of tumors and elevated MHC antigen expression by these cells. The tumors exhibited a variety of MHC phenotypes in vitro. The nature of their phenotypes suggested that these cells were, in fact, capable of independent and abnormal regulation of MHC class 1 genes. However, when maintained in vivo, these same tumor cells expressed measurable levels of all of the appropriate MHC class I antigens. Thus, newly induced tumor cells are capable of abnormal MHC class I antigen expression. However, there was no obvious correlation between the phenotypes exhibited by these tumor cells in vitro and either their phenotype or their tumorigenic potential in vivo.

Published

1991

45. The clinicopathologic, light, and scanning electron microscopic features of eperythrozoonosis in four naturally infected llamas.

Author

Reagan WJ, Garry F, Thrall MA, Colgan S, Hutchison J, and Weiser MG

Subjects

Anemia veterinary, Animals, Blood Cell Count veterinary, Blood Chemical Analysis veterinary, Blood Protein Electrophoresis veterinary, Erythrocytes microbiology, Female, Iron blood, Male, Microscopy, Electron, Scanning, Mycoplasma isolation & purification, Mycoplasma ultrastructure, Mycoplasma Infections blood, Mycoplasma Infections pathology, Camelids, New World, Erythrocytes ultrastructure, Mycoplasma Infections veterinary

Abstract

The hematologic, biochemical, and light and scanning electron microscopic features of eperythrozoonosis in four llamas are described. One female and three male yearling llamas were presented for evaluation of chronic weight loss. Three of four llamas had historical evidence of chronic inflammatory conditions. On examination, multiple clinical problems were apparent, including poorly to non-regenerative anemia, inflammatory disease, and hypoproteinemia. Coccoid- and ring-shaped basophilic organisms were present on the erythrocytes of all the llamas. On scanning electron microscopy, individual, pairs, and clusters of coccoid-shaped organisms were present on the erythrocytes. The organisms measured 0.4 to 0.6 micron in diameter and caused no marked deformation of the erythrocyte membrane. A rare organism could be found that produced a slight indentation into the erythrocyte membrane. The light and scanning electron microscopic morphologic features suggested that the organism was an Eperythrozoon. Serial evaluation of serum iron concentrations of the llamas showed a decrease serum iron in all animals, with a concurrent decrease in the total iron binding capacity and percent transferrin saturation in two of the llamas. Common abnormalities seen on serum electrophoresis included a decrease in albumin and beta serum fraction in all llamas and a decrease in the gamma globulin fraction of two individuals.

Published

1990