Study on Perturbing Systematic Interaction Network of GPV-gosling in an Infectious Context

doi:10.7668/hbnxb.2016.02.032

Abstract

Abstract: Perturbing systematic host network for Goose parvovirus (GPV) in natural infection were still unknown.Understanding pathogenic mechanism required that protein, enzymes and isozyme from goslings infected as manifestations of network properties, rather than simply as the result of individual variations.Here blood of experimentally GPV infected goslings were examined by biochemical analysis.The results indicated that the activity of protease, Est, POD, SOD, ALP, ADH, Amy, CAT, GPT and LDH from goslings infected GPV were higher 41%/63%, 30%/53%, 50%/14%, 36%/73%, 156%/142%, 1005%/22%, 36%/26%, 13%/51%, 60%/244%, 289%/139% than that of control group respectively.The content of IgG and IgM from goslings infected GPV were lower 50%, 40% than that of control group respectively, but protein was higher 50%.The isozyme of Est, SOD, ADH and Amy appeared 2, 2, 1, 3 new enzyme band respectively, but deleted 2 slow-zone Est isozyme band in the serum of goslings infected Goose parvovirus.The isozyme of Est, POD, SOD and Amy appeared 1, 2, 1, 2 new enzyme band in the blood corpuscle of goslings infected Goose parvovirus respectively.The isozyme of CAT, LDH, GPT and ALP appeared 7, 1, 3, 3 variation band in the blood of goslings infected GPV respectively.The isozyme of CAT and ADH defected fast-zone and slow-zone, fast-zone band in the blood corpuscle of goslings infected Goose parvovirus respectively.The isozyme of ALP defected slow-zone and fast-zone band in the serum and blood corpuscle of goslings infected GPV respectively.At the same time, it also showed that the 59 kDa protein band was a common feature of IgM/G in gosling, and IgG deleted still 258, 36 kDa protein in the blood of goslings infected Goose parvovirus.The protein were increased by 131, 86, 43, 33 kDa and 144, 104, 58, 53 kDa band in the serum and blood corpuscle of goslings infected Goose parvovirus respectively.There were deleted 1 slow-zone zymoprotein band in the serum of goslings infected GPV, and increased 2 slow-zone zymoprotein band in the blood corpuscle of goslings infected GPV.Those suggested that the interaction of GPV stress and host protein/enzymes and isozyme gene expression, through unique host dynamic balance of metabolic network directly or indirectly regulated cell disturbance susceptible performance.

Key words: Gosling, Goose parvovirus, Protein/Enzymes, Isozyme, Metabolic network

CLC Number:

S852.3

ZHU Xinchan, WANG Qianwen, ZHU Fengwei, YANG Lijin. Study on Perturbing Systematic Interaction Network of GPV-gosling in an Infectious Context[J]. ACTA AGRICULTURAE BOREALI-SINICA, 2016, 31(2): 195-204. doi: 10.7668/hbnxb.2016.02.032.

/ / Recommend / Download Citations

URL: http://www.hbnxb.net/EN/10.7668/hbnxb.2016.02.032

http://www.hbnxb.net/EN/Y2016/V31/I2/195

References

[1] Shao H,Lü Y,Ye J,et al.Isolation of a goose parvovirus from swan and its molecular characteristics[J].Acta Virologica,2014,58(2):194-198.
[2] Boergeling Y,Rozhdestvensky T S,Schmolke M,et al.Evidence for a novel mechanism of influenza Virus-induced type I interferon expression by a defective RNA-encoded protein[J].PLoS Pathogens,2015,11(5):e1004924.
[3] Li B,Wang Q,Pan X,et al.Bunyamwera virus possesses a distinct nucleocapsid protein to facilitate genome encapsidation[J].Proceedings of the National Academy of Sciences of the United States of America,2013,110(22):9048-9053.
[4] Gulbahce N,Yan H,Dricot A,et al.Viral perturbations of host networks reflect disease etiology[J].PLoS Computational Biology,2012,8(6):e1002531.
[5] Wibawa H,Bingham J,Nuradji H,et al.Experimentally infected domestic ducks show efficient transmission of Indonesian H5N1 highly pathogenic avian influenza virus,but lack persistent viral shedding[J].PLoS One,2014,9(1):e83417.
[6] Rozenblatt-Rosen O,Deo R C,Padi M,et al.Interpreting cancer genomes using systematic host network perturbations by tumour virus proteins[J].Nature,2012,487(748):491-495.
[7] 赵峰,张宏福,侯水生,等.鸭空肠液中淀粉酶、胰蛋白酶、糜蛋白酶活性变异的研究[J].畜牧兽医学报,2008,39(5):601-607.
[8] 邓艳美.水牛血液与乳中LDH活力的对比研究[J].中国畜牧兽医,2008,35(4):134-135.
[9] Allison S D,Schultz J C.Differential activity of peroxidase isozymes in response to wounding,gypsy moth,and plant hormones in northern red oak (Quercus rubra L.)[J].Journal of Chemical Ecology,2004,30(7):1363-1379.
[10] 江慧芳,王雅琴,刘春国.三种脂肪酶活力测定方法的比较及改进[J].化学与生物工程,2007,24(8):72-75.
[11] 张宏,谭竹钧.四种邻苯三酚自氧化法测定超氧化物歧化酶活性方法的比较[J].内蒙古大学学报:自然科学版,2002,33(6):677-681.
[12] 刘维全.动物生物化学实验指导[M].北京:中国农业出版社,2008:90-92.
[13] 叶晓健,田纪伟,高岱峰,等.脊髓半切伤大鼠血清谷丙转氨酶和谷草转氨酶活性变化的研究[J].中国临床康复,2004,8(17):3282-3283.
[14] Shim S M,Kim J H,Jung S E,et al.Multilaboratory assessment of variations in spectrophotometry-based DNA quantity and purity indexes[J].Biopreservation and Biobanking,2010,8(4):187-192.
[15] 赵永芳.生物化学技术原理及其应用[M].武汉:武汉大学出版社,1994:287-295.
[16] 朱新产,邵艳红,朱峰伟,等.鹅细小病毒感染雏鹅的免疫球蛋白IgG/IgM变异性研究[J].华北农学报,2015,30(1):42-53.
[17] Kajihara M,Sakoda Y,Soda K,et al.The PA2,PA,HA,NP,and NS genes of a highly pathogenic avian influenza virus A/whooper swan/Mongolia/3/2005(H5N1) are responsible for pathogenicity in ducks[J].Virol J,2013,10:45.
[18] Danchenko O O,Kalytka V V.Formation of antioxidant defence system of geese in embryogenesis and early postnatal ontogenesis[J].Ukrains'kyi Biokhimichnyi Zhurnal,2004,74(4):120-124.
[19] Li F.Receptor recognition mechanisms of coronaviruses:a decade of structural studies[J].Journal of Virology,2015,89(4):1954-1964.
[20] Shah K,Nahakpam S.Heat exposure alters the expression of SOD,POD,APX and CAT isozymes and mitigates low cadmium toxicity in seedlings of sensitive and tolerant rice cultivars[J].Plant Physiol Biochem,2012,57:106-113.
[21] Surolia I,Pirnie S P,Chellappa V,et al.Functionally defective germline variants of sialic acid acetylesterase in autoimmunity[J].Nature,2010,466(733):243-247.
[22] Kumagai Y,Satoh T,Inoue A,et al.Enzymatic properties and primary structures of two α-amylase isozymes from the Pacific abalone haliotis discus hannai[J].Comparative Biochemistry and Physiology,2013,164(2):80-88.
[23] Niyomploy P,Srisomsap C,Chokchaichamnankit D,et al.Superoxide dismutase isozyme detection using two-dimensional gel electrophoresis zymograms[J].J Pharm Biomed Anal,2014,90:72-77.
[24] Guo Y,Gao M,Wang J.A novel gene encoding goose immunoglobulin λ light chain[J].Acta Biochimica et Biophysica Sinica,2012,44(9):805-806.

Please choose a citation manager

Content to export