"小鼠β-1,4-N-acetyl-galactosaminyl transferase 2
於賽特利細胞之生理功能探討"

Po-Hsun Lu; 呂柏勳

請用此 Handle URI 來引用此文件： http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/61659

完整後設資料紀錄

DC 欄位	值	語言
dc.contributor.advisor	朱善德(Sin-Tak Chu)
dc.contributor.author	Po-Hsun Lu	en
dc.contributor.author	呂柏勳	zh_TW
dc.date.accessioned	2021-06-16T13:08:45Z	-
dc.date.available	2013-08-14
dc.date.copyright	2013-08-14
dc.date.issued	2013
dc.date.submitted	2013-08-01
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Capon C, Maes E, Michalski JC, Leffler H, Kim YS (2001) Sd(a)-antigen-like structures carried on core 3 are prominent features of glycans from the mucin of normal human descending colon. Biochem J 358: 657-664. 14. Dell A, Chalabi S, Easton RL, Haslam SM, Sutton-Smith M, et al. (2003) Murine and human zona pellucida 3 derived from mouse eggs express identical O-glycans. Proc Natl Acad Sci U S A 100: 15631-15636. 15. Donald AS, Yates AD, Soh CP, Morgan WT, Watkins WM (1983) A blood group Sda-active pentasaccharide isolated from Tamm-Horsfall urinary glycoprotein. Biochem Biophys Res Commun 115: 625-631. 16. Smith PL, Lowe JB (1994) Molecular cloning of a murine N-acetylgalactosamine transferase cDNA that determines expression of the T lymphocyte-specific CT oligosaccharide differentiation antigen. J Biol Chem 269: 15162-15171. 17. Malagolini N, Dall'Olio F, Di Stefano G, Minni F, Marrano D, et al. (1989) Expression of UDP-GalNAc:NeuAc alpha 2,3Gal beta-R beta 1,4(GalNAc to Gal) N-acetylgalactosaminyltransferase involved in the synthesis of Sda antigen in human large intestine and colorectal carcinomas. Cancer Res 49: 6466-6470. 18. Wang HR, Hsieh CY, Twu YC, Yu LC (2008) Expression of the human Sd(a) beta-1,4-N-acetylgalactosaminyltransferase II gene is dependent on the promoter methylation status. Glycobiology 18: 104-113. 19. Yuki H, Hamanaka R, Shinohara T, Sakai K, Watanabe M (2005) A novel approach for N-glycosylation studies using detergent extracted microsomes. Mol Cell Biochem 278: 157-163. 20. Dohi T, Hanai N, Yamaguchi K, Oshima M (1991) Localization of UDP-GalNAc:NeuAc alpha 2,3Gal-R beta 1,4(GalNAc to Gal)N-acetylgalactosaminyltransferase in human stomach. Enzymatic synthesis of a fundic gland-specific ganglioside and GM2. J Biol Chem 266: 24038-24043. 21. Dohi T, Nakasuji M, Oshima M (1993) Induction of the fundic mucosa-specific glycolipid with dimethylformamide in gastric-cancer cell lines. Int J Cancer 53: 137-140. 22. Hakomori S (2002) Glycosylation defining cancer malignancy: new wine in an old bottle. Proc Natl Acad Sci U S A 99: 10231-10233. 23. Kawamura YI, Kawashima R, Fukunaga R, Hirai K, Toyama-Sorimachi N, et al. (2005) Introduction of Sd(a) carbohydrate antigen in gastrointestinal cancer cells eliminates selectin ligands and inhibits metastasis. Cancer Res 65: 6220-6227. 24. Kimber SJ, Spanswick C (2000) Blastocyst implantation: the adhesion cascade. Semin Cell Dev Biol 11: 77-92. 25. Klisch K, Jeanrond E, Pang PC, Pich A, Schuler G, et al. (2008) A tetraantennary glycan with bisecting N-acetylglucosamine and the Sd(a) antigen is the predominant N-glycan on bovine pregnancy-associated glycoproteins. Glycobiology 18: 42-52. 26. Li PT, Liao CJ, Wu WG, Yu LC, Chu ST (2011) Progesterone-regulated B4galnt2 expression is a requirement for embryo implantation in mice. Fertil Steril 95: 2404-2409, 2409 e2401-2403. 27. Evans SC, Lopez LC, Shur BD (1993) Dominant negative mutation in cell surface beta 1,4-galactosyltransferase inhibits cell-cell and cell-matrix interactions. J Cell Biol 120: 1045-1057. 28. Lopez LC, Maillet CM, Oleszkowicz K, Shur BD (1989) Cell surface and Golgi pools of beta-1,4-galactosyltransferase are differentially regulated during embryonal carcinoma cell differentiation. Mol Cell Biol 9: 2370-2377. 29. Roseman S (1970) The synthesis of complex carbohydrates by multiglycosyltransferase systems and their potential function in intercellular adhesion. Chem Phys Lipids 5: 270-297. 30. Roth S (1973) A molecular model for cell interactions. Q Rev Biol 48: 541-563. 31. Stewart S, Fang G (2005) Anaphase-promoting complex/cyclosome controls the stability of TPX2 during mitotic exit. Mol Cell Biol 25: 10516-10527. 32. Bullwinkel J, Baron-Luhr B, Ludemann A, Wohlenberg C, Gerdes J, et al. (2006) Ki-67 protein is associated with ribosomal RNA transcription in quiescent and proliferating cells. J Cell Physiol 206: 624-635. 33. Migrenne S, Moreau E, Pakarinen P, Dierich A, Merlet J, et al. (2012) Mouse testis development and function are differently regulated by follicle-stimulating hormone receptors signaling during fetal and prepubertal life. PLoS One 7: e53257. 34. Buzzard JJ, Wreford NG, Morrison JR (2003) Thyroid hormone, retinoic acid, and testosterone suppress proliferation and induce markers of differentiation in cultured rat sertoli cells. Endocrinology 144: 3722-3731. 35. Tarulli GA, Stanton PG, Loveland KL, Meyts ER, McLachlan RI, et al. (2013) A survey of Sertoli cell differentiation in men after gonadotropin suppression and in testicular cancer. Spermatogenesis 3: e24014. 36. Wassler MJ, Shur BD (2000) Clustering of cell surface (beta)1,4-galactosyltransferase I induces transient tyrosine phosphorylation of focal adhesion kinase and loss of stress fibers. J Cell Sci 113 Pt 2: 237-245. 37. Youakim A, Hathaway HJ, Miller DJ, Gong X, Shur BD (1994) Overexpressing sperm surface beta 1,4-galactosyltransferase in transgenic mice affects multiple aspects of sperm-egg interactions. J Cell Biol 126: 1573-1583. 38. Miller DJ, Macek MB, Shur BD (1992) Complementarity between sperm surface beta-1,4-galactosyltransferase and egg-coat ZP3 mediates sperm-egg binding. Nature 357: 589-593. 39. Shur BD (1983) Embryonal carcinoma cell adhesion: the role of surface galactosyltransferase and its 90K lactosaminoglycan substrate. Dev Biol 99: 360-372. 40. Pratt SA, Scully NF, Shur BD (1993) Cell surface beta 1,4 galactosyltransferase on primary spermatocytes facilitates their initial adhesion to Sertoli cells in vitro. Biol Reprod 49: 470-482. 41. Ziparo E, Geremia R, Russo MA, Stefanini M (1980) Surface interaction in vitro between Sertoli cells and germ cells at different stages of spermatogenesis. Am J Anat 159: 385-388.
dc.identifier.uri	http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/61659	-
dc.description.abstract	Sda β-1,4-N-acetyl-galactosaminyl transferase Ⅱ(B4galnt2)是一醣轉移酶，主要催化轉移GalNAc以β-1,4的鍵結至[Neu5Acα2-3]Galβ1-4GlcNAcβ1-3Gal之Gal上，使醣連上形成Sda結構。此一結構最早是在血球表面抗原結構所發現，實際上它廣泛存在於哺乳動物組織或體液中，包含胃、腸、腎、血清、尿液和乳汁等。近期研究發現人類胃癌和結腸癌細胞中B4GALNT2表現量會明顯下降，而使Sda抗原減少並與癌細胞轉移有密切關係；由此可知B4GALNT2的重要性與生物系統的相關性，但目前為止對其生理功能研究仍有很大的空間。2003年Dell的研究團隊首先在雌性生殖系統中發現Sda結構的存在，為了解Sda結構的生理功能，故先了解其轉化酵素B4galnt2。由實驗室成員的研究了解B4galnt2與老鼠胚胎著床及卵母細胞成熟有關，推測Sda結構在雌性生殖系統中具有其重要性，所以了解Sda轉化酶的調控，以便推測Sda角色之可能性。實驗室已發現一賽特利細胞的細胞株(TM4)會表現B4galnt2，推測B4galnt2可能在雄性生殖系統中扮演著某種角色，至於B4galnt2的功能在雄性生殖系統尚為未知。實驗中以公鼠為動物模式利用Quantitative Real-Time PCR (qRT-PCR)及免疫螢光染色法確認初級賽特利細胞與賽特利細胞株TM4在細胞膜上有B4galnt2的存在。觀察賽特利細胞不論在繁殖作用減少時或細胞株處理follicle stimulating hormone(FSH)後增強繁殖作用後，其B4galnt2基因表現量無明顯差異，推測B4galnt2和史脫力細胞之繁殖作用較無直接相關性。利用甲狀腺激素(thyroid hormone)、視黃酸(retinoic acid)、睪固酮(testosterone)此三種賀爾蒙處理賽特利細胞株，可誘導賽特利細胞進入成熟狀態，可經成熟標記基因(maturation marker gene)及成熟後生理之特性確認其賽特利細胞之成熟。在成熟過程中，B4galnt2基因表現量上升，且利用RNA interference(RNAi)抑制基因表現實驗中發現當削弱B4galnt2表現時，成熟標記基因表現量隨之下降，顯示賽特利細胞無法進入成熟階段。綜合以上各項結果推測B4galnt2與賽特利細胞之成熟作用具有相關性，此外利用初級賽特利細胞發現小鼠在靠近青春期時，B4galnt2表現量相較於出生期高，當未成熟初級賽特利細胞誘導至成熟之初級賽特利細胞，其B4galnt2基因表現量隨之升高，故B4galnt2在小鼠體內可能也和賽特利細胞之成熟作用具有正相關性。	zh_TW
dc.description.abstract	Sda β-1,4-N-acetyl-galactosaminyl transferaseⅡis a kind of carbohydrate transferases, whose main function is to catalyze and transfer GalNAc to Gal of [Neu5Acα2-3]Galβ1-4GlcNAcβ1-3Gal through β-1,4 bond, so that carbohydrate is linked to form the Sda structure. The structure was earliest found in the antigen structure on the blood corpuscle surface; in fact, however, it is widely distributed in the tissues and body fluids of the mammals, including stomach, intestine, kidney, serum, urine, and milk. Recent studies showed that the B4GALNT2 expression was obviously reduced in the gastric cancer and colon cancer cells of human being, causing decrease in the Sda antigen, and the said reduction was closely correlated with the metastasis of the cancer cells; this indicated the importance of B4GALNT2 and its correlation with the bio-system. However, very few studies have been conducted on its physiological functions. In 2003, the research team led by Dell first found the Sda structure in the female reproductive system. Before the physiological functions of the Sda structure was learned about, its invertase B4galnt2 needed to be studied. The research showed that B4galnt2 was correlated with the mouse’s embryo implantation and the maturation of its oocytes. It was presumed that the Sda structure played an important role in the female reproductive system. Therefore, to infer the role of the Sda structure, the regulation and control by the Sda invertase should be learned. The laboratory has found B4galnt2 in the cell strains (TM4) of the Sertoli cells, so it was supposed that B4galnt2 might play a certain role in the male reproductive system, but its functions in the male reproductive system remained unknown yet. In the experiment, a male mouse was taken as the subject. The Quantitative Real-Time PCR and immune fluorescent staining method were used to confirm the existence of B4galnt2 on the cell membranes of the primary Sertoli cells and Sertoli cell strains. The observation indicated that whether the proliferation of the Sertoli cells was declined or enhanced after the cell strains were treated with follicle stimulating hormone, the B4galnt2 gene expression showed no marked difference. In this way, it was presumed that B4galnt2 did not participate in the proliferation of the Sertoli cells. By using hormone to treat the Sertoli cell strains, the Sertoli cells might be induced into the state of maturity. The maturity of the Sertoli cells could be confirmed by the mature marker genes and post-maturation physiological features. In the process of maturation, the B4galnt2 gene expression was increased. The RNAi suppress gene expression experiment showed that when the B4galnt2 expression was reduced, the maturation marker gene expression decreased accordingly. This showed that the Sertoli cells could not enter the state of maturity. To sum up, it was presumed that B4galnt2 participated in the maturation of the Sertoli cells. In addition, the experiment on the primary Sertoli cells showed that the B4galnt2 expression in the mouse coming close to the puberty was higher than that when it was born. When the immature primary Sertoli cells were induced to be mature, the B4galnt2 gene expression in them was raised. Thus, it was presumed that B4galnt2 might participate in the maturation of the Sertoli cells in the mouse.	en
dc.description.provenance	Made available in DSpace on 2021-06-16T13:08:45Z (GMT). No. of bitstreams: 1 ntu-102-R00b46009-1.pdf: 1748985 bytes, checksum: 8f58d63d5434eed3f850b41ca6f9139d (MD5) Previous issue date: 2013	en
dc.description.tableofcontents	目錄中文摘要………………………………………………………………………………………………………..…………I 英文摘要……………………………………………...……………………………………………………….….......III 縮寫表………………………………………………………………………...….………………………….…….……..V 目錄…………………………………………………………………………….……………………………………….….VI 第一章緒論…………………………………………………………………………………………………………….1 一、哺乳類雄性生殖系統………………………………………………………………………..…….1 二、精子生成(spermatogenesis)……………………..………………………………………..……2 三、精子生成的關鍵角色…………………...……..………………………………………….……...4 四、賽特利細胞之功能介紹…………………..………………………..……………….……….…..4 五、Sda醣類抗原介紹…………………………………………………………………………….……...6 六、B4galnt2介紹及在腸胃道癌中的影響力………………………………………….…….7 七、B4galnt2在生殖系統中扮演的角色…….……..............…………………….………..9 八、本論文的研究動機及目的……………………………………………………………….……..9 第二章材料與方法………………………………………………………………………………………….……11 一、公鼠睪丸細胞擷取與收集………………………………………………………….…..11 二、細胞株培養………………………………………………………………………………….….13 三、藥物處理……………………………………………………………………………………….….14 四、 RNA萃取…………………………..………………………….……………………………….…14 五、反轉錄PCR(Reverse Transcription-Polymerase Chain Reaction)……...15 六、即時定量聚合酶連鎖反應(Quantitative Real-Time PCR)………...........16 七、免疫螢光染色法(Immunofluorescence)……………................................17 八、轉染(Transfection)………………..............................................................18 九、細胞移動能力分析(migration assay)………….…………………………………..18 十、增殖能力分析………………..……………………………………………………………….19 第三章結果……………………………………………………...…………………………………………………..21 I、 B4galnt2 在賽特利細胞分布位置及表現量……………………….……21 II、B4galnt2與賽特利細胞生理功能之關聯性…………….………….……22 II A 細胞繁殖…………………………………………………….…...22 II B 細胞成熟…………………………………………………….…...24 III、B4galnt2在雄性小鼠生殖系統扮演之角色........………………….……26 第四章討論…………………………………………………………………………28 第五章圖次…………………………………………………………………………31 附表…………………………………………………………………………………..48 參考文獻……………………………………………………………………………..49
dc.language.iso	zh-TW
dc.subject	Sda	zh_TW
dc.subject	B4galnt2	zh_TW
dc.subject	精子生成	zh_TW
dc.subject	史脫力細胞之成熟	zh_TW
dc.subject	史脫力細胞與生殖細胞之交互作用	zh_TW
dc.subject	Sertoli cell-Germ cell interaction	en
dc.subject	Sda	en
dc.subject	B4galnt2	en
dc.subject	Spermatogenesis	en
dc.subject	Sertoli cell maturation	en
dc.title	"小鼠β-1,4-N-acetyl-galactosaminyl transferase 2 於賽特利細胞之生理功能探討"	zh_TW
dc.title	Functional test of β-1,4-N-acetyl-galactosaminyl transferase 2 in mouse sertoli cell	en
dc.type	Thesis
dc.date.schoolyear	101-2
dc.description.degree	碩士
dc.contributor.oralexamcommittee	余榮熾(Lung-Chih Yu),張?仁(Ching-Jin Chang),曾婉芳(Wan-Fang Tzeng)
dc.subject.keyword	Sda,B4galnt2,精子生成,史脫力細胞之成熟,史脫力細胞與生殖細胞之交互作用,	zh_TW
dc.subject.keyword	Sda,B4galnt2,Spermatogenesis,Sertoli cell maturation,Sertoli cell-Germ cell interaction,	en
dc.relation.page	52
dc.rights.note	有償授權
dc.date.accepted	2013-08-01
dc.contributor.author-college	生命科學院	zh_TW
dc.contributor.author-dept	生化科學研究所	zh_TW
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