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小鼠睑板腺的发育

The development of meibomian glands in mice.

作者信息

Nien Chyong Jy, Massei Salina, Lin Gloria, Liu Hongshan, Paugh Jerry R, Liu Chia-Yang, Kao Winston Whei-Yang, Brown Donald J, Jester James V

机构信息

Gavin Herbert Eye Institute, University of California Irvine, Orange, CA 92868, USA.

出版信息

Mol Vis. 2010 Jun 18;16:1132-40.

Abstract

PURPOSE

The purpose of this study was to characterize the natural history of meibomian gland morphogenesis in the mouse.

METHODS

Embryonic (E) and post natal (P) C57Bl/6 mouse pups were obtained at E18.5, P0, P1, P3, P5, P8, P15, and P60. Eyelids were fixed and processed for en bloc staining with Phalloidin/DAPI to identify gland morphogenesis, or frozen for immunohistochemistry staining with Oil red O (ORO) to identify lipid and antibodies specific against peroxisome proliferator-activated receptor gamma (PPARgamma) to identify meibocyte differentiation. Samples were then evaluated using a Zeiss 510 Meta laser scanning confocal microscope or Nikon epi-fluorescent microscope. Tissues from adult mice (2 month-old) were also collected for western blotting.

RESULTS

Meibomian gland morphogenesis was first detected at E18.5 with the formation of an epithelial placode within the fused eyelid margin. Invagination of the epithelium into the eyelid was detected at P0. From P1 to P3 there was continued extension of the epithelium into the eyelid. ORO and PPARgamma staining was first detected at P3, localized to the central core of the epithelial cord thus forming the presumptive ductal lumen. Ductal branching was first detected at P5 associated with acinar differentiation identified by ORO and PPARgamma staining. Adult meibomian glands were observed by P15. Western blotting of meibomian gland proteins identified a 50 kDa and a 72 kDa band that stained with antibodies specific to PPARgamma.

CONCLUSIONS

We have demonstrated that meibomian gland development bears distinct similarities to hair development with the formation of an epithelial placode and expression of PPARgamma co-incident with lipid synthesis and meibocyte differentiation.

摘要

目的

本研究旨在描述小鼠睑板腺形态发生的自然史。

方法

获取胚胎期(E)和出生后(P)的C57Bl/6小鼠幼崽,时间点分别为E18.5、P0、P1、P3、P5、P8、P15和P60。将眼睑固定,用鬼笔环肽/4',6-二脒基-2-苯基吲哚(Phalloidin/DAPI)进行整体染色以鉴定腺体形态发生,或将其冷冻用于油红O(ORO)免疫组织化学染色以鉴定脂质,并用抗过氧化物酶体增殖物激活受体γ(PPARγ)的抗体进行免疫组织化学染色以鉴定睑板腺细胞分化。然后使用蔡司510 Meta激光扫描共聚焦显微镜或尼康落射荧光显微镜对样本进行评估。还收集了成年小鼠(2月龄)的组织用于蛋白质免疫印迹分析。

结果

在E18.5时首次检测到睑板腺形态发生,在融合的眼睑边缘形成上皮基板。在P0时检测到上皮向眼睑内陷。从P1到P3,上皮持续向眼睑内延伸。在P3时首次检测到ORO和PPARγ染色,定位于上皮索的中央核心,从而形成假定的导管腔。在P5时首次检测到导管分支,同时通过ORO和PPARγ染色鉴定出腺泡分化。在P15时观察到成年睑板腺。睑板腺蛋白的蛋白质免疫印迹分析鉴定出一条50 kDa和一条72 kDa的条带,它们与PPARγ特异性抗体发生反应。

结论

我们已经证明,睑板腺发育与毛发发育具有明显的相似性,包括上皮基板的形成以及PPARγ的表达与脂质合成和睑板腺细胞分化同时发生。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/21af/2901193/09e6cea7bb65/mv-v16-1132-f1.jpg

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