Chen Zixiu, Zhao Junhong, Wang Cangyu, Liu Xiang, Chen Zihua, Zhou Jianda, Zhang Lei, Zhang Cuiping, Li Haihong
Department of Wound Repair and Dermatologic Surgery, Taihe Hospital, Hubei University of Medicine, Jinzhou Medical University Graduate Training Base, Shiyan, Hubei Province, China.
Department of Burns and Plastic Surgery, The Third Hospital of Central South University, Changsha, Hunan, China.
Acta Histochem. 2023 Oct;125(7):152093. doi: 10.1016/j.acthis.2023.152093. Epub 2023 Sep 25.
Each eccrine sweat gland (ESG) is a single-tubular structure with a central lumen, and the formation of hollow lumen in the initial solid cell mass is a key developmental process. To date, there are no reports on the mechanism of native ESG lumen formation.
To investigate the lumen morphogenesis and the lumen formation mechanisms of Sprague-Dawley (SD) rat ESGs, SD rat hind-footpads at E20.5, P1-P5, P7, P9, P12, P21, P28 and P56 were obtained. The lumen morphogenesis of ESGs was examined by HE staining and immunofluorescence staining for polarity markers. The possible mechanisms of lumen formation were detected by terminal deoxynucleotidyl transferase dUTP nick end labeling (TUNEL) apoptosis assay and autophagy marker LC3B immunofluorescence staining, and further explored by ouabain intervention experiment.
In SD rat ESGs, the microlumen was formed at P1, and the small intact lumen with apical-basal polarity appeared at P3. The expression of apical marker F-actin, basal marker Laminin, basolateral marker E-cadherin was consistent with the timing of lumen formation of SD rat ESGs. During rat ESG development, apoptosis and autophagy were not detected. However, inhibition of Na-K-ATPase (NKA) with ouabain resulted in decreased lumen size, although neither the timing of lumen formation nor the expression of polarity proteins was altered.
Epithelial polarity-driven membrane separation but not cavitation regulates lumen formation of SD rat ESGs. NKA-regulated fluid accumulation drives lumen expansion.
每个外泌汗腺(ESG)是一个具有中央管腔的单管状结构,在初始实体细胞团中形成中空管腔是一个关键的发育过程。迄今为止,尚无关于天然ESG管腔形成机制的报道。
为了研究Sprague-Dawley(SD)大鼠ESG的管腔形态发生和管腔形成机制,获取了E20.5、P1-P5、P7、P9、P12、P21、P28和P56时的SD大鼠后足垫。通过HE染色和极性标记物的免疫荧光染色检查ESG的管腔形态发生。通过末端脱氧核苷酸转移酶dUTP缺口末端标记(TUNEL)凋亡检测和自噬标记物LC3B免疫荧光染色检测管腔形成的可能机制,并通过哇巴因干预实验进一步探索。
在SD大鼠ESG中,微管腔在P1形成,具有顶端-基部极性的小完整管腔在P3出现。顶端标记物F-肌动蛋白、基部标记物层粘连蛋白、基底外侧标记物E-钙黏蛋白的表达与SD大鼠ESG管腔形成的时间一致。在大鼠ESG发育过程中,未检测到凋亡和自噬。然而,用哇巴因抑制钠钾ATP酶(NKA)导致管腔大小减小,尽管管腔形成的时间和极性蛋白的表达均未改变。
上皮极性驱动的膜分离而非空化调节SD大鼠ESG的管腔形成。NKA调节的液体积累驱动管腔扩张。
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