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  1. NTU Theses and Dissertations Repository
  2. 生物資源暨農學院
  3. 獸醫專業學院
  4. 分子暨比較病理生物學研究所
請用此 Handle URI 來引用此文件: http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/57446
完整後設資料紀錄
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dc.contributor.advisor王汎熒
dc.contributor.authorChien-Chun Kuoen
dc.contributor.author郭建均zh_TW
dc.date.accessioned2021-06-16T06:46:26Z-
dc.date.available2017-07-31
dc.date.copyright2014-07-31
dc.date.issued2014
dc.date.submitted2014-07-25
dc.identifier.citation呂榮修, 蔡義雄, 鍾明華, 劉培柏, 李永林, 楊喜吟, 王金和, 王吉德, 1981. 台灣豬腸道病毒分離與抗體調查. 台灣省畜衛試研報 17, 83-90.
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Cano-Gomez, C., Garcia-Casado, M.A., Soriguer, R., Palero, F., Jimenez-Clavero, M.A., 2013. Teschoviruses and sapeloviruses in faecal samples from wild boar in Spain. Vet. Microbiol. 165, 115-122.
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Deng, M.Y., Millien, M., Jacques-Simon, R., Flanagan, J.K., Bracht, A.J., Carrillo, C., Barrette, R.W., Fabian, A., Mohamed, F., Moran, K., Rowland, J., Swenson, S.L., Jenkins-Moore, M., Koster, L., Thomsen, B.V., Mayr, G., Pyburn, D., Morales, P., Shaw, J., Burrage, T., White, W., McIntosh, M.T., Metwally, S., 2012. Diagnosis of Porcine teschovirus encephalomyelitis in the Republic of Haiti. J. Vet. Diagn. Invest. 24, 671-678.
Derbyshire, J.B., Arkell, S., 1971. The activity of some chemical disinfectants against Talfan virus and porcine adenovirus type 2. British Vet. J. 127, 137-142.
Donin, D.G., de Arruda Leme, R., Alfieri, A.F., Alberton, G.C., Alfieri, A.A., 2014. First report of Porcine teschovirus (PTV), Porcine sapelovirus (PSV) and Enterovirus G (EV-G) in pig herds of Brazil. Tropical Anim. Hlth. Produc. 46, 523-528.
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Jimenez-Clavero, M.A., Fernandez, C., Ortiz, J.A., Pro, J., Carbonell, G., Tarazona, J.V., Roblas, N., Ley, V., 2003. Teschoviruses as indicators of porcine fecal contamination of surface water. Appl. Environ. Microbiol. 69, 6311-6315.
Kaku, Y., Murakami, Y., Sarai, A., Wang, Y., Ohashi, S., Sakamoto, K., 2007. Antigenic properties of porcine teschovirus 1 (PTV-1) Talfan strain and molecular strategy for serotyping of PTVs. Arch. Virol. 152, 929-940.
Kaku, Y., Yamada, S., Murakami, Y., 1999. Sequence determination and phylogenetic analysis of RNA-dependent RNA polymerase (RdRp) of the porcine enterovirus 1 (PEV-1) Talfan strain. Arch.Virol. 144, 1845-1852.
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Krumbholz, A., 2003. Detection of porcine teschoviruses and enteroviruses by LightCycler real-time PCR. J. Virol. Methods 113, 51-63.
Lin, Y.C., 2009. Detection of porcine teschovirus in tissues of experimentally infected pigs. Master degree thesis. National Taiwan University, Taipei.
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Qiu, Z., Wang, Z., Zhang, B., Zhang, J., Cui, S., 2013. The prevalence of porcine teschovirus in the pig population in northeast of China. J. Virol. Methods 193, 209-214.
Racaniello, V.R., 2006. One hundred years of poliovirus pathogenesis. Virology 344, 9-16.
Salles, M.W., Scholes, S.F., Dauber, M., Strebelow, G., Wojnarowicz, C., Hassard, L., Acton, A.C., Bollinger, T.K., 2011. Porcine teschovirus polioencephalomyelitis in western Canada. J. Vet. Diagn. Invest. 23, 367-373.
Swindle, M.M. 2007. Urinary system and adrenal glands, In: Swine in the Laboratory: Surgery, Anesthesia, Imaging, and Experimental Techniques. Taylor & Francis Group, pp. 159.
Wang, B., Tian, Z.J., Gong, D.Q., Li, D.Y., Wang, Y., Chen, J.Z., An, T.Q., Peng, J.M., Tong, G.Z., 2010. Isolation of serotype 2 porcine teschovirus in China: evidence of natural recombination. Vet. Microbiol. 146, 138-143.
Watzinger, F., Ebner, K., Lion, T., 2006. Detection and monitoring of virus infections by real-time PCR. Mol. Asp. Med. 27, 254-298.
Yamada, M., Kozakura, R., Nakamura, K., Yamamoto, Y., Yoshii, M., Kaku, Y., Miyazaki, A., Tsunemitsu, H., Narita, M., 2009. Pathological changes in pigs experimentally infected with porcine teschovirus. J. Comp. Pathol. 141, 223-228.
Yamada, M., Miyazaki, A., Yamamoto, Y., Nakamura, K., Ito, M., Tsunemitsu, H., Narita, M., 2014. Experimental teschovirus encephalomyelitis in gnotobiotic pigs. J. Comp. Pathol. 150, 276-286.
Yang, C.L., 2013. Quantification of Porcine Teschovirus Load in Tissues of Endemically Infected Pigs. Master degree thesis. National Taiwan University,
Zell, R., Krumbholz, A., Henke, A., Birch-Hirschfeld, E., Stelzner, A., Doherty, M., Hoey, E., Dauber, M., Prager, D., Wurm, R., 2000. Detection of porcine enteroviruses by nRT-PCR: differentiation of CPE groups I-III with specific primer sets. J. Virol. Methods 88, 205-218.
dc.identifier.urihttp://tdr.lib.ntu.edu.tw/jspui/handle/123456789/57446-
dc.description.abstract豬鐵士古病毒(Porcine Teschovirus, PTV),為單股正向無封套RNA病毒。PTV目前有13種血清型,引起離乳豬的腦脊髓炎或下痢,藉由糞口傳播。在台灣曾於2000年與2004年爆發兩次疫情,現今於台灣豬場呈現普遍的地方性感染。先前研究已確認PTV會感染腎絲球體內皮細胞與腎小管上皮,推測PTV可能從尿液排毒,但仍未有數據證實。本研究目的為偵測感染豬隻糞、尿、血液及臟器的病毒量,以釐清在地方性感染下,PTV的致病機轉及排毒狀況。本研究從7個豬場採集健康及淘汰離乳豬隻臟器及體液檢體,共7隻健康豬隻及21頭淘汰離乳豬,利用即時定量反轉錄聚合酶反應(Real-Time RT-PCR)偵測檢體中的病毒量,並使用台灣常見的PTV-7毒株序列製作標準曲線,以進行絕對定量(最低可偵測到101病毒量)。實驗結果顯示所有豬隻皆可偵測到PTV,其尿液、血液、糞便、鼻腔拭子的偵測率為100%,腎臟的偵測率約38%。依照病毒量高低可將10種檢體分為3組:腸道相關(迴腸及糞便)、血液淋巴相關(扁桃腺、鼠膝淋巴結及血漿),以及臟器與泌尿相關 (脾臟、腎臟、膀胱及尿液)。 迴腸的病毒量最高,每100毫克組織的病毒量約為106.4,約為糞便的3倍,血漿的40倍。次高為糞便,每100毫克的病毒量約為105.9,此結果與糞口病毒血症的致病機轉一致。而100微升尿液中的病毒量約為104,約為糞便病毒量的百分之一,血液病毒量的六分之一,腎臟病毒量的五倍,表示PTV容易通過絲球體進入尿液中。此10種檢體的病毒量在不同豬場及不同健康狀況豬隻皆無顯著差異。淘汰豬隻的血漿病毒量略高於健康豬隻的病毒量,但在統計上無顯著差異,顯示PTV即使在健康豬隻也會造成病毒血症,與地方性感染的結論一致。本研究確認了PTV會藉由尿液排出體外,並在糞尿混合下加速了PTV的傳播。在7個豬場皆偵測到PTV,合併持續性的病毒血症,再次印證PTV在台灣已成為重要的地方性病毒性疾病。zh_TW
dc.description.abstractPorcine teschovirus (PTVs) is a non-enveloped, positive-sense, single-stranded RNA virus. At least 13 serotypes of PTVs have been identified. The PTVs can cause polioencephalomyelitis and diarrhea through fecal-oral transmission. In Taiwan, two epidemic outbreaks of PTVs occurred in years 2000 and 2004, and the endemic status of PTVs is now confirmed in herds. Previous study has demonstrated PTVs antigen and nucleic acid in glomeruli and epithelia of renal tubules, and suggested that shedding and transmission of PTVs by urine may be possible. However, this speculation remains to be verified with numerical evidence. The study aimed to clarify the shedding pathway and to further the understanding of pathogenesis in endemic infection by detecting the viral loads of urine, feces, plasma and solid tissues in naturally infected piglets. In this study, the samples were collected from 7 clinically healthy and 21 culled piglets of 7 different herds, and viral loads of each sample were quantified by means of absolute quantification in real-time RT-PCR with a detection limit of 101 copies per reaction. A standard curve was constructed by the sequence of PTV-7, which is the most common serotype in Taiwan. The results showed 100% detection rates in urine, feces, plasma and nasal swabs, and 38% in kidney. Based on the viral loads, these samples were categorized into three groups: Intestinal-related samples (feces and ileum), hematolymphoid samples (tonsil, inguinal lymph node, and plasma), visceral and fluid samples (spleen, kidney, bladder, urine and nasal swab). The viral loads of ileum were the highest, measuring 106.40 copies/100 mg tissue weight, approximately 3-times higher than those of feces (105.9 copies/100 mg), and 40-times higher than plasma (104.79 copies/100 μl). The categorization was largely consistent with the fecal-oral-viremia pathogenesis model. As speculated, PTV was present in the urine at the scale of 104 copies/100 μl fluids, which was 1% of that in feces, 17% of that in plasma but 5-times higher than in kidney. These results suggested that PTVs were easily filtered from blood to urine through glomeruli. No statistical significance was found between healthy and culled pigs, and between the 7 herds. The viral loads of plasma in culled piglets were slightly higher but no significant difference than those of healthy piglets, indicating that those outwardly healthy pigs were also infected by PTV and had viremia, consistent with the endemic situation. In conclusion, PTVs can be detected in urine, confirming the urinary shedding pathway in the naturally infected situation. The combination of urine and feces into slurry facilitate the transmission of PTVs. The detection of PTVs in different herds further confirmed the endemic situation, in which a persistent viremia was occurring. Therefore, PTVs is an important endemic disease of piglets in Taiwan.en
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Previous issue date: 2014
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dc.description.tableofcontents口試委員會審定書 i
誌謝 ii
中文摘要 iii
ABSTRACT iv
CONTENTS vi
LIST OF FIGURES ix
LIST OF TABLES x
LIST OF APPENDICES xi
Chapter 1 Introduction 1
Chapter 2 Background of Study and Literature Review 3
2.1 Porcine teschovirus 3
2.1.1 Taxonomy 3
2.1.2 Viral structure, genome and other characteristics 3
2.2 Epidemiology 4
2.2.1 Epidemiology in Taiwan 4
2.3 Clinical signs and histopathological lesions 5
2.3.1 Polioencephalomyelitis 5
2.3.2 Reproductive diseases 6
2.3.3 Diarrhea 6
2.3.4 Pneumonia, pericarditis, and myocarditis 6
2.4 Pathogenesis, cell tropism, and shedding pathway 7
2.4.1 Pathogenesis of PTVs in natural and experimental infections 7
2.4.2 Pathogenesis in endemic situation 8
2.4.3 Cell tropism of PTVs 8
2.4.4 Shedding pathways of PTVs 8
2.5 Detection and quantification of PTVs by real-time RT-PCR (quantitative RT-PCR) 9
2.5.1 Absolute quantification method by qRT-PCR 9
2.5.2 qRT-PCR assay for detecting PTVs 10
Chapter 3 Materials and Methods 11
3.1 Experimental design 11
3.2 Sample preparations 12
3.2.1 Animals 12
3.2.2 Sampling for real-time RT-PCR 12
3.2.3 Tissues for histopathological examination 12
3.3 RNA extraction 13
3.3.1 RNA extraction from solid tissues 13
3.3.2 RNA extraction from fluid samples (diluted feces, urine, plasma, and nasal swab) 13
3.3.3 RNA yield in solid tissues and fluid samples 14
3.4 Construction of the standard curve of PTV- 7 15
3.4.1 Selection of cRNA sequence 15
3.4.2 Synthesis of cRNA 15
3.4.3 Quantification of cRNA and copy number 15
3.5 Absolute quantification of PTVs by real-time RT-PCR 16
3.5.1 Real-time RT-PCR assay 16
3.5.2 Real-time RT-PCR 16
3.5.3 Construction of the standard curve 17
3.5.4 Detection of PTVs in endemically infected pigs by real-time RT-PCR 18
3.5.5 Quantification of PTVs in samples 18
3.5.6 Comparison of viral loads between solid tissues and fluid samples 18
3.5.7 Example for quantifications and data conversion of viral loads 20
3.5.8 Data analysis 21
Chapter 4 Results 23
4.1 Animals 23
4.1.1 Gross lesions 23
4.1.2 Histological lesions 23
4.2 RNA yield 24
4.3 Absolute quantification of PTVs using standard curve method in real-time RT-PCR 24
4.3.1 Sensitivity and standard curve of PTV-7 in real-time RT-PCR assay 24
4.3.2 Variability of the standard curves 25
4.3.3 Absolute quantification of PTVs in endemic infected pigs 25
4.3.4 Statistical analysis 26
Chapter 5 Discussion 27
REFERENCES 32
FIGURES 37
TABLES 44
APPENDICES 60
dc.language.isoen
dc.title在野外地方性感染現況豬鐵士古病毒經由尿液排毒之探討zh_TW
dc.titleUrinary Shedding of Porcine Teschovirus in Endemically Infected Field Situationen
dc.typeThesis
dc.date.schoolyear102-2
dc.description.degree碩士
dc.contributor.oralexamcommittee張本恆,郭鴻志,李 璠,張家宜
dc.subject.keyword豬鐵士古病毒,尿液,即時定量聚合?鏈鎖反應,zh_TW
dc.subject.keywordPorcine Teschovirus,Urine,Real-time RT-PCR,en
dc.relation.page74
dc.rights.note有償授權
dc.date.accepted2014-07-28
dc.contributor.author-college獸醫專業學院zh_TW
dc.contributor.author-dept分子暨比較病理生物學研究所zh_TW
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