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体外培养小鼠下颌下腺细胞生长特性的实验研究 被引量:2

The Study of Submandibular Gland Cells Biology Characteristics
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摘要 目的:研究小鼠下颌下腺细胞的培养方法,探讨下颌下腺细胞培养条件及细胞生长特性,为研究干细胞转分化涎腺腺泡细胞以及涎腺再生研究奠定理论基础和技术支持。方法:取2周龄的小鼠,组织块法和消化法分别进行培养,用活细胞观察法和HE染色法记录细胞形态学特征;免疫荧光染色法鉴定;通过生长曲线和细胞倍增时间来比较两种方法对细胞增殖能力的影响。结果:组织块法和消化法均可以成功的培养下颌下腺细胞,(1)组织块法培养的细胞呈卵圆形或多边形,10天左右成铺路石样;消化法培养细胞亦为上皮样细胞,呈多边形,胞质丰富;(2)HE染色下颌下腺细胞呈多边形,胞核明显;(3)Cytokeratin13和AQP5表达阳性,Wimentin表达阴性;(4)组织块法培养细胞增殖相对较平缓,消化法培养细胞增长较迅速;(5)消化法培养倍增时间(1.3471±0.6071)天比组织块法倍增时间(2.1887±1.1503)明显缩短(P<0.05);结论:体外可以成功的培养下颌下腺细胞,但是同时证明下颌下腺细胞长期传代较困难,这为研究干细胞转分化涎腺细胞和涎腺再生体内实验提供了理论和实验基础。 Objective: To study the methods of culturing the submandibular gland cells of mouse, and discuss culture conditions and cell growth characteristics of the submandibular gland cells, and aim to laying the theoretical foundation and technical support for the research of stem cells turning to salivary gland acinar cells and salivary gland regeneration. Methods: The 2-week submandibular gland cells were cultured by the tissue block method and the digestion method separately, and then we observed the cell morphology characteristic by living cells photographic and HE dyeing. The cells were identified by immunofluorescence staining method and through the growth curve and cell multiplication time to compare the influence of cell proliferation ability between two methods. Results: Submandibular gland cells can be cultured successfully by organization block method and digestion method. (1) The cells cultured by tissue block method are ovoid or polygon, for 10 days they formed paving-stone sample, digestion culture cell are epithelical cells, polygonal and cytoplasmic rich. (2) HE dyed show the submandibular gland cells are polygonal and the nucleus is obvious. (3) The expression of Cytokeratinl3 and AQP5 are positive and Wimentin is negative. (4) The speed of cell proliferation of tissue block method is relatively gentle, while digestion method is rapid. (5) The doubling time of digestion method (1.3471 ± 0.6071 days ) is significantly shortened than organization block method (2.1887 ± 1.1503) (P〈0.05). Conclusion: It has been successful to culture submandibular gland cells in vitro, and submandibular gland cells is expected to become seed cells of salivary gland regeneration tissue engineering.
作者 邢红艳 刘彦普 刘斌 徐小方 王艳 胡翰青
机构地区 第四军医大学口腔医院颌面外科 第四军医大学口腔医院生物教研室及实验动物中心
出处 《现代生物医学进展》 CAS 2013年第28期5409-5412,共4页 Progress in Modern Biomedicine
基金 国家自然科学基金项目(31170942)
关键词 颌下腺细胞 体外培养 纯化 生长曲线 倍增时间 Submandibular gland cells Culture in vitro Purification Growth curve Multiplication time
分类号 Q95-3 [生物学—动物学] R782 [医药卫生—口腔医学]
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参考文献21

  • 1于世凤.口腔组织病理学[M].北京:人民卫生出版社,2005:198.
  • 2Wijers OB,Levendag PC,Braaksma MM,et al.Patients with headand neck cancer cured by radiation therapy:a survey of the dry mouthsyndrome in long-term survivors[J].Head Neck,2002,24(8):737-747.
  • 3Kakoei S,Haghdoost AA,Rad M,et al.Xerostomia after radiotherapyand its effect on quality of life in head and neck cancer patients[J].Arch Iran Med,2012,15(4):214-218.
  • 4Vissink A,Jansma J,Spijkervet,FK.,et al.Oral sequelae of head andneck radiotherapy[J].Crit Rev Oral Biol Med,2003,14(3):199-212.
  • 5Fang FM,Liu YT,Tang Y,et al.Quality of life as a survival predictorfor patients with advanced head and neck carcinoma treated withradiotherapy[J].Cancer,2004,100(2):425-432.
  • 6Walker MP,Wichman B,Cheng AL,et al.Impact of RadiotherapyDose on Dentition Breakdown in Head and Neck Cancer Patients[J].Pract Radiat Oncol.2011,1(3):142-148.
  • 7Sullivan CA,Haddad RI,Tishler RB,et al.Chemoradiation-inducedcell loss in human submandibular glands[J].Laryngoscope,2005,11(5):958-964.
  • 8Vermorken JB.Medical treatment in head and neck cancer[J].AnnOncol,2005,16(2):258-264.
  • 9Schliephake H,Jamil MU.Prospective evaluation of quality of lifeafter oncologic surgery for oral cancer[J].Oral Maxillofac Surg,2002,31:427-433.
  • 10周青,王玉新,王绪凯,卢利,孙长伏.肝细胞生长因子对大鼠颌下腺细胞增殖的影响[J].中华实验外科杂志,2002,19(6):538-539. 被引量:8

二级参考文献23

  • 1Matsumoto K,Nakamura T.Hepatocyte growth factor:Renotropic role and potential therapeutics for renal disease.Kidney Int,2001,59:2023-2038.
  • 2Diamond JR,Ricardo SD,Klahr S.Mechanisms of interstitial fibrosis in obstructive nephropathy.Semin Nephrol,1998,18:594-602.
  • 3Oliver C.Isolation and maintenance of differentiated exocrine gland acinar cells in vitro.In Vitro 1980;16(4):297-305.
  • 4Aframian DJ, Tran SD, Cukierman E,et al. Absence of tight junction formation in an allogeneic graft cell line used for developing an engineered artificial salivary gland. Tissue Eng 2002;8(5):871-8.
  • 5Okumura K,Nakamura K,Hisatomi Y,et al. Salivary gland progenitor cells induced by duct ligation differentiate into hepatic and pancreatic lineages.Hepatology 2003;38(1):104-13.
  • 6Takeuchi T, Aletta JM, Laychock SG, et al.Role of nerve growth factor in the regulation of parotid cell differentiation induced by rat serum.Biochem Pharmacol 2003;65(9):1507-13.
  • 7Okura M,Shirasuna K,Hiranuma T, et al. Characterization of growth and differentiation of normal human submandibular gland epithelial cells in a serum-free medium.Differentiation 1993;54(2):143-53.
  • 8Sato M, Yoshida H, Hayashi Y,et al. Expression of epidermal growth factor and transforming growth factor-beta in human salivary gland adenocarcinoma cell line. Cancer Res 1985;45(12 Pt 1):6160-7.
  • 9Donovan PJ,Gearhart J.The end of the beginning for pluripotent stem cells.Nature 2001;414(6859):92-7.
  • 10Azuma M, Tamatani T, Kasai Y, et al. Immortalization of normal human salivary gland cells with duct-, myoepithelial-, acinar-, or squamous phenotype by transfection with SV40 ori-mutant deoxyribonucleic acid. Lab Invest 1993;69(1):24-42.

共引文献10

同被引文献21

  • 1曹钰,王松灵,司徒镇强,吴军正,刘斌,李焰,李洁,李峰.小型猪腮腺细胞体外原代培养的研究[J].实用口腔医学杂志,2005,21(1):39-42. 被引量:1
  • 2薛辉,司徒镇强,吴军正.腮腺腺细胞体外极性培养及形态观察[J].实用口腔医学杂志,1995,11(2):125-127. 被引量:7
  • 3王静,吴军正,郭富平,董纪军,魏红宇.人涎腺上皮细胞体外培养及其生物学特性的初步研究[J].实用口腔医学杂志,2005,21(5):587-591. 被引量:4
  • 4张林朴,王冠华.体外连续传代培养人腮腺腺上皮细胞的观察[J].中国组织工程研究与临床康复,2007,11(3):540-541. 被引量:2
  • 5司徒镇强 吴军正.细胞培养[M].西安:世界图书版出版公司,2004.78-202.
  • 6Nagler RM. The enigmatic mechanism of irradiation-induced damage to the major salivary glands [J]. Oral Dis, 2002, 8(3): 141-146.
  • 7Stephens LC, Ang KK, Schultheiss TE, et al. Target cell and mode of radiation injury in rhesus salivary glands [J]. Radiother Oncol, 1986, 7(2): 165-174.
  • 8Dozic I,Todorovic T,dozic B.Immunohistochemical identifi- cation of cytokeratins in the rat submandibular salivary glands during ontogenesis[J].Acta veterinaria, 2009,59(1) : 69-80.
  • 9Navarro Rde L, Martins MT, de Araujo VC. Maspin expression in normal and neoplastic salivary gland [J]. J Oral Pathol Med, 2004, 33(7): 435-440.
  • 10Prasad KN, Carvalho E, Edwards-Prasad J, et al. Establishment of human parotid pleomorphic adenoma cells in culture: morphological and biochemical characterization [J].In Vitro Cell Dev Biol, 1994, 30A(5): 312-320.

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现代生物医学进展
2013年 第28期

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