大鼠下颌下腺细胞培养及其生物学特性研究

doi:10.13701/j.cnki.kqyxyj.2016.08.010

口腔医学研究 ›› 2016, Vol. 32 ›› Issue (8): 816-818.DOI: 10.13701/j.cnki.kqyxyj.2016.08.010

大鼠下颌下腺细胞培养及其生物学特性研究

柳康^1,2,王越¹,彭慧敏¹,卢浩¹,马晓周¹,杜宝霞¹,张伟^1*

1. 吉林大学口腔医学院吉林长春 130021;
2. 吉林省牙发育及颌骨重塑与再生重点实验室吉林长春 130021

收稿日期:2016-01-18 出版日期:2016-08-26 发布日期:2016-08-26
通讯作者: 张伟,E-mail:doctorzhang888@sina.com
作者简介:柳康(1990~ ),男,湖北人,硕士在读,主要从事唾液腺疾病相关研究。
基金资助:
吉林省直厅局项目(编号:5139073431)

A Study of Rat Submandibular Gland Cell Culture and Its Biological Characteristics

LIU Kang^1,2, WANG Yue¹, PENG Hui-min¹, LU Hao¹, MA Xiao-zhou¹, DU Bao-xia¹, ZHANG Wei^1*

1. School and Hospital of Stomatology, Jilin University, Changchun 130021, China;
2. Provincial Key Laboratory of Tooth Development and Jaw Remodeling and Regeneration, Changchun 130021, China.

Received:2016-01-18 Online:2016-08-26 Published:2016-08-26

摘要/Abstract

摘要： 目的:体外培养大鼠下颌下腺细胞,并对其生物学特性进行研究,为涎腺疾病的探索提供体外模型。方法:无菌条件下取7 d龄Wistar大鼠双侧下颌下腺,仔细分离脂肪、包膜、神经和血管,采用组织块培养法进行培养。运用酶消化法和差速贴壁法纯化细胞;免疫组化SP法检测Cytokeratin-8(CK-8)抗体和α-Amylase抗体的表达;PAS染色法检测细胞糖原分泌;扫描电镜(scanning electronic microscopy,SEM)观察细胞的形态学特征。结果:组织块培养法可成功获得下颌下腺细胞,免疫组化染色可见大部分细胞胞质为棕黄色,提示CK-8抗体表达阳性,α-Amylase抗体表达阳性;PAS染色可见胞质呈紫红色;SEM可见细胞伸出长短不一的伪足,胞核着色深,有些细胞可见分泌颗粒。结论:组织块培养法可以成功培养大鼠下颌下腺细胞,并且操作简便。

关键词: 下颌下腺细胞, 原代培养, 组织块培养, 扫描电镜

Abstract: Objective: To culture submandibular gland cells of rats in vitro and study its biological characteristics so as to provide a cell model for salivary gland disease research. Methods: The bilateral submandibular glands were obtained from Wistar rats of 7 days old in a sterile condition. Fat, capsule, nerve and blood vessel were carefully removed, followed by tissue-explant culturing. The cells were purified by enzymatic digestion and differential adhesion. The cell phenotype was immunohistochemically identified by cytokeratin-8 (CK-8) and α-Amylase staining, and hepatin secreting ability of the cells was tested by PAS staining. Ultramicroscopic features of the cells was observed under the scanning electronic microscopy (SEM). Results: Submandibular gland cells were successfully obtained by tissue-explant culturing. The cells gained were positively stained for both CK-8 and α-Amylase. The cytoplasm manifested as purple red in PAS staining. Under SEM, cells had different lengths of pseudopodia and the nucleues were darker-stained; in some cells secretory granules were visible. Conclusion: Rat submandibular gland cells can be successfully cultured by the uncomplicated tissue-explant technique.

Key words: Submandibular gland cell, Primary culture, Tissue-explant technique, Scanning electronic microscopy

中图分类号:

R780.2

柳康,王越,彭慧敏,卢浩,马晓周,杜宝霞,张伟. 大鼠下颌下腺细胞培养及其生物学特性研究[J]. 口腔医学研究, 2016, 32(8): 816-818.

LIU Kang, WANG Yue, PENG Hui-min, LU Hao, MA Xiao-zhou, DU Bao-xia, ZHANG Wei. A Study of Rat Submandibular Gland Cell Culture and Its Biological Characteristics[J]. Journal of Oral Science Research, 2016, 32(8): 816-818.

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大鼠下颌下腺细胞培养及其生物学特性研究

A Study of Rat Submandibular Gland Cell Culture and Its Biological Characteristics

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