腮腺主导管结扎及再通后腺泡凋亡与再生变化规律的研究

口腔医学研究 ›› 2015, Vol. 31 ›› Issue (5): 444-447.

腮腺主导管结扎及再通后腺泡凋亡与再生变化规律的研究

卢浩, 刘士维, 崔智, 吴梓齐, 孙宾, 柳康, 张伟^*

吉林大学口腔医院颌面外科吉林长春 130021

收稿日期:2014-09-28 出版日期:2015-05-28 发布日期:2016-04-29
通讯作者: 张伟,E-mail:tianbingxiaojiang@126.com
作者简介:卢浩(1990~ ),男,山东省人,硕士在读,主要从事口腔涎腺疾病的基础研究。
基金资助:
吉林省直厅局项目(编号:5139073431)

Roles of Apoptosis and Mitosis in the Regeneration of Rat Parotid Gland following Ligation-induced Atrophy.

LU Hao, LIU Shi-wei, CUI Zhi, et al.

Department of Oral and Maxillofacial Surgery, Jilin University, Changchun 130021

Received:2014-09-28 Online:2015-05-28 Published:2016-04-29

摘要/Abstract

摘要： 目的:研究大鼠腮腺主导管结扎及再通后腺泡凋亡与再生的变化规律。方法:通过对大鼠右侧腮腺主导管双重结扎14 d后再通,建立腮腺组织萎缩后再生模型。分别于主导管再通术后0、1、3、5、7、10、14和21 d获取腮腺组织标本,应用HE和AB-PAS染色观察腺体的组织学变化,免疫组织化学染色法检测腺泡中增殖细胞核抗原(PCNA)、半胱氨酸天冬氨酸蛋白水解酶3(Caspase3)的表达。结果:组织学观察见:主导管结扎14 d后腺泡萎缩、消失,导管样结构增多,酶原颗粒消失;主导管再通术后,腺泡再生,导管样结构减少,酶原颗粒数目恢复正常。免疫组织化学染色分析结果示:在主导管结扎14 d后PCNA散在表达,主导管再通1 d后表达增加,5 d后达峰值,7 d后降低并趋于平稳;主导管结扎14 d及再通后Caspase3表达水平持续较低,且平稳。各实验组间PCNA表达差异有统计学意义(P＜0.05),而Caspase3表达差异无统计学意义。结论:腮腺主导管持续结扎14 d后再通,萎缩的腺泡可再生,形态及功能均可恢复正常水平,表明主导管持续结扎14 d对腺体组织造成的损伤完全可逆。

关键词: 细胞再生, 细胞凋亡, 唾液腺

Abstract: Objective: To investigate the roles of apoptosis and mitosis in the regeneration of rat parotid gland following release from duct ligation. Methods: The excretory duct was double ligated with metal-clip unilaterally near the hilum in order to induce atrophy of the parotid gland, and after 2 weeks of ligation(day 0)the double-ligated duct was reopened from 0 to 21 days in order to enable parotid gland regeneration. The evolving gland were examined with HE-staining, AB-PAS staining technique and immunohistochemistry for proliferating cell nuclear antigen(PCNA)as a marker of proliferating cells and Caspase3 as a marker of apoptotic cells. Results: After 14days ligation, the vast majority of acinus and the zymogen granules were replaced by the ductal structure. But during the regeneration of parotid gland, many residual and newly formed acinar cells were identified by HE and AB-PAS staining accompanying increasing zymogen granules. There were occasional PCNA-positive acinar or duct cells in ligated gland, but after 3d of the release of metal-clip, many PCNA-positive cells were seen especially acinar cells between 3d to 7d, thereafter PCNA-positive cells decreased in number.During the regeneration of parotid glands, the Caspase3-positive cells were very rarely observed in 0d, but Caspase3-positive numbers decreased after that. The difference of PCNA-positive numbers were statistically significant between each group (P<0.05)and the reaction of acinar cells compared to duct cells were significantly different at each point of the experimental group(P<0.05). Conclusion: During regeneration of the parotid gland, most acinar cells regeneration from the residual acinar cells at the peripheral region of lobules and the apoptosis of did not play important roles in the regeneration of rat parotid gland after 2 weeks duct-ligation.

Key words: Regeneration , Apoptosis , Salivary glands

中图分类号:

R783.1

卢浩, 刘士维, 崔智, 吴梓齐, 孙宾, 柳康, 张伟. 腮腺主导管结扎及再通后腺泡凋亡与再生变化规律的研究[J]. 口腔医学研究, 2015, 31(5): 444-447.

LU Hao, LIU Shi-wei, CUI Zhi, et al.. Roles of Apoptosis and Mitosis in the Regeneration of Rat Parotid Gland following Ligation-induced Atrophy.[J]. Journal of Oral Science Research, 2015, 31(5): 444-447.

参考文献

[1] 周竹云,左金华,王丽芳,等.腮腺主导管结扎后腺体的组织学变化 [J].口腔医学研究,2011,27(8)∶660-663
[2] Dieckman LM,Freudenthal BD,Washington MT.PCNA structure and function: insights from structures of PCNA complexes and post-translationally modified PCNA [J]. Subcell Biochem,2012,62∶281-299
[3] Takahashi S,Gobe GC,Yoshimura Y,et al. Participation of the Fas and Fas ligand systems in apoptosis during atrophy of the rat submandibular glands [J]. Exp Pathol,2007,88(1)∶9-17
[4] Ikeno T,Ikeno K,Uno T. Relationship between serum-amylase activity and intraductal pressures in the rat parotid and submandibular salivary after administration of pilocarpine or isoprenaline [J]. Arch Oral Biol,1988,33(6)∶403-406
[5] Harrison JD,Fouad HM,Garrett JR,et al. The effects of ductal obstruction on the acinar cells of the parotid of cat [J]. Arch Oral Biol,2000,45(11)∶945-949
[6] Takahashi S,Shinzato K,Nakamura S,et al. Cell death and cell proliferation in the regeneration of atrophied rat submandibular glands after duct ligation [J]. Oral Pathol Med,2004,33(1)∶23-29
[7] Cotroneo E,Procter GB,Carpenter GH. Regeneration of acinar cells following ligation of rat submandibular gland retraces the embryonic-perinatal pathway of cytodifferentiation [J]. Differentiation,2010,79(2)∶120-130
[8] Arany S,Catalan MA,Roztocil E,et al. Ascl3 knockout and cell ablation models reveal complexity of salivary gland maintenance and regeneration [J]. Dev Biol,2011,353(2)∶186-193
[9] Takahashi S, Shinzato K, Nakamura S, et al. The roles of apoptosis and mitosis in atrophy of the rat sublingual gland [J]. Tissue and Cell, 2002, 34(5)∶297-304
[10] Taira K, Hiroyasu S, Shiraishi M, et al. Role of the Fas system in liver regeneration after a partial hepatectomy in rats [J]. European surgical research, 2002, 33(5-6)∶334-341
[11] Miyazaki T,Tatsukawa S,Kitamura H,et al. Morphological and functional changes of the rat parotid glandular cells by clipping and reopening the parotid duct, using HAM8 antibody [J]. Anat Sci Int,2008,83(2)∶89-95
[12] Osailan SM,Proctor GB,Carpenter GH,et al. Recovery of rat submandibular salivary gland function following removal of obstruction: a sialometrical and sialochemical study [J]. Exp Pathol,2006,87(6)∶411-423