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2. Porcine Circovirus type 2 (PCV2) causes apoptosis in experimentally inoculated BALB/c mice

Author

Galbreath Elizabeth J, Stevenson Gregory W, Kiupel Matti, North Adam, HogenEsch Harm, and Mittal Suresh K

Subjects
Veterinary medicine, SF600-1100
Abstract

Abstract Background We have previously described microscopic and electron microscopic alterations in lymphoid organs of PCV2 inoculated mice as apoptosis. In this study we wanted to investigate the molecular pathogenetic mechanism of PCV2-induced apoptosis. Eight-week old BALB/c mice were either sham inoculated (control mice) or inoculated intraperitoneally (ip) and intranasally (in) with a single (sPCV mice) or multiple (mPCV mice) doses of PCV2. Four control mice and 4 sPCV mice were sacrificed 7, 14, 28 and 42 days post inoculation (PI). All 4 mPCV mice were sacrificed 42 days PI. Following necropsy, immunohistochemistry for caspase 3 and in-situ TUNEL assay were performed on sections of spleen, lymph nodes, thymus and ileum from control, sPCV and mPCV mice. In addition, total RNA was extracted from spleens of control, sPCV and mPCV mice for simultaneous detection and semiquantitation of bcl-2 homologues and various caspase mRNAs using a multiprobe RNase protection assay system. Results PCV2 replicated and was associated with apoptosis in spleens, lymph nodes and Peyer's patches of infected BALB/c mice. Upregulation of caspase 1, 2, 3, 6, 7, 8, 11 and 12 and upregulation for the transcripts of apoptosis inhibitors bcl-2, bcl-w and bcl-X and apoptosis promoters' bax, bak and bad was detected in spleens of sPCV and mPCV mice, but not control mice. Apoptosis was further confirmed by light and electron microscopic morphology as well as by positive TUNEL assay and detection of activated caspase 3. PCV2 nucleic acid was detected by in-situ hybridization in the nuclei and cytoplasm of such apoptotic cells. Conclusion The data presented here support the hypothesis that PCV2 induces apoptosis mediated through the activation of caspases 8 and 3 in the spleens of infected mice.

Published
2005
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3. Polioencephalomyelitis in Domestic Swine Associated With Porcine Astrovirus Type 3.

Author

Matias Ferreyra, Franco S., Bradner, Laura K., Burrough, Eric R., Cooper, Vickie L., Derscheid, Rachel J., Gauger, Phillip C., Harmon, Karen M., Madson, Darin, Piñeyro, Pablo E., Schwartz, Kent J., Stevenson, Gregory W., Zeller, Michel A., and Arruda, Bailey L.

Subjects
CIRCOVIRUS diseases, REVERSE transcriptase polymerase chain reaction, SWINE, NEUROLOGICAL disorders, SWINE diseases, PATHOLOGY
Abstract

In the past decade, different members of the genus Mamastrovirus have been associated with outbreaks of neurologic disease in humans, cattle, sheep, mink, and, most recently, porcine astrovirus 3 (PoAstV3) in swine. We performed a retrospective analysis of 50 cases of porcine neurologic disease of undetermined cause but with microscopic lesions compatible with a viral encephalomyelitis to better understand the role and pathogenesis of PoAstV3 infection. Nucleic acid was extracted from formalin-fixed paraffin-embedded (FFPE) tissue for reverse transcription quantitative polymerase chain reaction (RT-qPCR) testing for PoAstV3. In addition, 3 cases with confirmed PoAstV3-associated disease were assayed by RT-qPCR to investigate PoAstV3 tissue distribution. PoAstV3 was detected in central nervous system (CNS) tissue via RT-qPCR and in situ hybridization in 13 of 50 (26%) FFPE cases assayed. PoAstV3 was rarely detected in any tissues outside the CNS. Positive cases from the retrospective study included pigs in various production categories beginning in 2010, the earliest year samples were available. Based on these results, PoAstV3 appears to be a recurring putative cause of viral encephalomyelitis in swine that is rarely detected outside of the CNS at the time of clinical neurologic disease, unlike other common viral causes of neurologic disease in swine. [ABSTRACT FROM AUTHOR]

Published
2020
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4. Outbreak of H5N2 highly pathogenic avian Influenza A virus infection in two commercial layer facilities.

Author

Arruda, Paulo H. E., Stevenson, Gregory W., Killian, Mary L., Burrough, Eric R., Gauger, Phillip C., Harmon, Karen M., Magstadt, Drew R., Yoon, Kyoung-Jin, Zhang, Jianqiang, Madson, Darin M., Piñeyro, Pablo, Derscheid, Rachel J., Schwartz, Kent J., Cooper, Vickie L., Halbur, Patrick G., Main, Rodger G., Sato, Yuko, and Arruda, Bailey L.

Subjects
INFLUENZA A virus, H3N2 subtype, VIRUS diseases, DISEASE outbreaks, BIRD diseases, POULTRY industry, IMMUNOHISTOCHEMISTRY, POLYMERASE chain reaction
Abstract

The largest outbreak of highly pathogenic avian Influenza A virus (HPAIV) infection in U.S. history began in December 2014 resulting in the euthanasia of millions of birds and collateral economic consequences to the U.S. poultry industry. We describe 2 cases of H5N2 HPAIV infection in laying hens in Iowa. Following a sharp increase in mortality with minimal clinical signs, 15 dead birds, from 2 unrelated farms, were submitted to the Iowa State University Veterinary Diagnostic Laboratory. Common lesions included diffuse edema and multifocal hemorrhage of the comb, catarrhal exudate in the oropharynx, and multifocal tracheal hemorrhage. Less common lesions included epicardial petechiae, splenic hemorrhage, and pancreatic necrosis. Influenza A virus nucleoprotein was detected by immunohistochemistry in multiple cell types including ependymal cells, the choroid plexus, neurons, respiratory epithelium and macrophages in the lung, cardiac myocytes, endothelial cells, necrotic foci in the spleen, Kupffer cells in the liver, and necrotic acinar cells in the pancreas. Real-time polymerase chain reaction and sequencing confirmed H5N2 HPAIV with molecular characteristics similar to other contemporary U.S. H5N2 HPAIVs in both cases. [ABSTRACT FROM AUTHOR]

Published
2016
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5. Emergence of Porcine epidemic diarrhea virus in the United States: clinical signs, lesions, and viral genomic sequences.

Author

Stevenson, Gregory W., Hoang, Hai, Schwartz, Kent J., Burrough, Eric R., Sun, Dong, Madson, Darin, Cooper, Vickie L., Pillatzki, Angela, Gauger, Philip, Schmitt, Beverly J., Koster, Leo G., Killian, Mary L., and Yoon, Kyoungjin J.

Subjects
DIARRHEA, DIARRHEA in animals, SWINE diseases, GENOMICS, SWINE
Abstract

During the 10 days commencing April 29, 2013, the Iowa State University Veterinary Diagnostic Laboratory received the first 4 of many submissions from swine farms experiencing explosive epidemics of diarrhea and vomiting affecting all ages, with 90–95% mortality in suckling pigs. Histology revealed severe atrophy of villi in all segments of the small intestines with occasional villus-epithelial syncytial cells, but testing for rotaviruses and Transmissible gastroenteritis virus (Alphacoronavirus 1) were negative. Negative-staining electron microscopy of feces revealed coronavirus-like particles and a pan-coronavirus polymerase chain reaction (PCR) designed to amplify a conserved region of the polymerase gene for all members in the family Coronaviridae produced expected 251-bp amplicons. Subsequent sequencing and analysis revealed 99.6–100% identity among the PCR amplicons from the 4 farms and 97–99% identity to the corresponding portion of the polymerase gene of Porcine epidemic diarrhea virus (PEDV) strains, with the highest identity (99%) to strains from China in 2012. Findings were corroborated at National Veterinary Services Laboratories using 2 nested S-gene and 1 nested N-gene PCR tests where the sequenced amplicons also had the highest identity with 2012 China strains. Whole genome sequence for the virus from 2 farms in 2 different states using next-generation sequencing technique was compared to PEDV sequences available in GenBank. The 2013 U.S. PEDV had 96.6–99.5% identity with all known PEDV strains and the highest identity (>99.0%) to some of the 2011–2012 Chinese strains. The nearly simultaneous outbreaks of disease, and high degree of homology (99.6–100%) between the PEDV strains from the 4 unrelated farms, suggests a common source of virus. [ABSTRACT FROM PUBLISHER]

Published
2013
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6. Experimental co-infection of pigs with Bovine viral diarrhea virus 1 and Porcine circovirus-2.

Author

Langohr, Ingeborg M., Stevenson, Gregory W., Nelson, Eric A., Lenz, Stephen D., Huiling Wei, and Pogranichniy, Roman M.

Subjects
CATTLE diseases, VIRAL diarrhea, CIRCOVIRUSES, VACCINATION, SWINE diseases, CATTLE, COLOSTRUM
Abstract

The article shows the function of Bovine viral diarrhea virus (BVDV) in progression of Porcine circovirus-2 (PCV-2). Two studies were performed, where the first one involved vaccination of germ-free pigs vaccinated with different PCV-2 and BVDV viruses. The second study looked at cesarian-derived, colostrum-derived pigs that were vaccinated with the viruses. Results showed that BVDV and PCV-2 hinder growth and caused death of pigs through developing acute respiratory distress.

Published
2012
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7. Genotyping of Porcine teschovirus from nervous tissue of pigs with and without polioencephalomyelitis in Indiana.

Author

Bangari, Dinesh S., Pogranichniy, Roman M., Gillespie, Tom, and Stevenson, Gregory W.

Subjects
ENTEROVIRUSES, PICORNAVIRUSES, SWINE diseases, NERVE tissue
Abstract

The article discusses the results of a study on the genotyping of Porcine teschovirus (PTV) from the nervous tissue of pigs with and without polioencephalomyelitis in Indiana. The researchers isolated PTV in cell culture and showed it through polymerase chain reaction in samples of brain and spinal cord from pigs. The study found that low-to-moderate virulence strains of PTV are endemic in swineherds in Indiana.

Published
2010
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8. Porcine Circovirus type 2 (PCV2) causes apoptosis in experimentally inoculated BALB/c mice.

Author

Kiupel, Matti, Stevenson, Gregory W., Galbreath, Elizabeth J., North, Adam, HogenEsch, Harm, and Mittal, Suresh K.

Subjects
*RIBONUCLEASES, *APOPTOSIS, *NUCLEIC acids, *MESSENGER RNA, *VIRUS diseases in swine, *LABORATORY mice, *VETERINARY medicine
Abstract

Background: We have previously described microscopic and electron microscopic alterations in lymphoid organs of PCV2 inoculated mice as apoptosis. In this study we wanted to investigate the molecular pathogenetic mechanism of PCV2-induced apoptosis. Eight-week old BALB/c mice were either sham inoculated (control mice) or inoculated intraperitoneally (ip) and intranasally (in) with a single (sPCV mice) or multiple (mPCV mice) doses of PCV2. Four control mice and 4 sPCV mice were sacrificed 7, 14, 28 and 42 days post inoculation (PI). All 4 mPCV mice were sacrificed 42 days PI. Following necropsy, immunohistochemistry for caspase 3 and in-situ TUNEL assay were performed on sections of spleen, lymph nodes, thymus and ileum from control, sPCV and mPCV mice. In addition, total RNA was extracted from spleens of control, sPCV and mPCV mice for simultaneous detection and semiquantitation of bcl-2 homologues and various caspase mRNAs using a multiprobe RNase protection assay system. Results: PCV2 replicated and was associated with apoptosis in spleens, lymph nodes and Peyer's patches of infected BALB/c mice. Upregulation of caspase 1, 2, 3, 6, 7, 8, 11 and 12 and upregulation for the transcripts of apoptosis inhibitors bcl-2, bcl-w and bcl-X and apoptosis promoters' bax, bak and bad was detected in spleens of sPCV and mPCV mice, but not control mice. Apoptosis was further confirmed by light and electron microscopic morphology as well as by positive TUNEL assay and detection of activated caspase 3. PCV2 nucleic acid was detected by in-situ hybridization in the nuclei and cytoplasm of such apoptotic cells. Conclusion: The data presented here support the hypothesis that PCV2 induces apoptosis mediated through the activation of caspases 8 and 3 in the spleens of infected mice. [ABSTRACT FROM AUTHOR]

Published
2005
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9. Rapid detection of terbufos in stomach contents using desorption electrospray ionization mass spectrometry.

Author

Wilson, Christina R., Mulligan, Christopher C., Strueh, Kurt D., Stevenson, Gregory W., and Hooser, Stephen B.

Subjects
ELECTROSPRAY ionization mass spectrometry, TERBUFOS, POISONS, CHOLINESTERASE reactivators, VETERINARY toxicology
Abstract

Desorption electrospray ionization mass spectrometry (DESI-MS) is an emerging analytical technique that permits the rapid and direct analysis of biological or environmental samples under ambient conditions. Highlighting the versatility of this technique, DESI-MS has been used for the rapid detection of illicit drugs, chemical warfare agents, agricultural chemicals, and pharmaceuticals from a variety of sample matrices. In diagnostic veterinary toxicology, analyzing samples using traditional analytical instrumentation typically includes extensive sample extraction procedures, which can be time consuming and labor intensive. Therefore, efforts to expedite sample analyses are a constant goal for diagnostic toxicology laboratories. In the current report, DESI-MS was used to directly analyze stomach contents from a dog exposed to the organophosphate insecticide terbufos. The total DESI-MS analysis time required to confirm the presence of terbufos and diagnose organophosphate poisoning in this case was approximately 5 min. This highlights the potential of this analytical technique in the field of veterinary toxicology for the rapid diagnosis and detection of toxicants in biological samples. [ABSTRACT FROM PUBLISHER]

Published
2014
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