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胚胎唾液腺形态发生中N-连接糖缀合物的放射自显影分析。

An autoradiographic analysis of N-linked glycoconjugates in embryonic salivary gland morphogenesis.

作者信息

Bassett K E, Spooner B S

出版信息

J Exp Zool. 1987 Jun;242(3):317-24. doi: 10.1002/jez.1402420310.

Abstract

The synthesis, deposition, and loss of mannose-bearing glycoconjugates during branching morphogenesis of embryonic mouse salivary glands has been evaluated. Day 13 embryonic mouse salivary glands were cultured for 44 hr, pulse labeled 4 hr with [3H]mannose, then fixed after 0, 2, 4, 8, or 24 hr of chase in nonradioactive medium, and processed for autoradiography. Light microscopic autoradiograms of sectioned rudiments reveal extensive label within the epithelium, little label over the mesenchyme, and a concentration of radioactivity at the basal surface of the epithelium. Autoradiograms of "chased" rudiments reveal a) no detectable loss of label from the epithelium or the basal epithelial surface over the first 8 hr, and b) significant label loss by 24 hr of chase at the basal epithelial surface, while moderate amounts of radioactivity remain throughout the rest of the epithelium. The [3H]bound material is insensitive to chondroitinase ABC, a glycosaminoglycan degradative enzyme, but is sensitive to tunicamycin presence in the culture medium. Earlier studies showed that embryonic mouse salivary glands cultured in medium containing tunicamycin (25 ng/ml) continued normal epithelial branching while epithelial growth was inhibited. The present autoradiographic studies of [3H]mannose-labeled rudiments demonstrate that tunicamycin causes a significant decrease in radioactivity, relative to controls. Thus, our results suggest that epithelial branching activity is independent of control levels of mannose-containing/tunicamycin-sensitive, glycoconjugate deposition.

摘要

已对胚胎小鼠唾液腺分支形态发生过程中含甘露糖糖缀合物的合成、沉积和丢失进行了评估。将第13天的胚胎小鼠唾液腺培养44小时,用[3H]甘露糖脉冲标记4小时,然后在无放射性培养基中追踪0、2、4、8或24小时后固定,并进行放射自显影处理。切片原基的光学显微镜放射自显影片显示上皮内有大量标记,间充质上几乎没有标记,且放射性集中在上皮的基底表面。“追踪”原基的放射自显影片显示:a)在最初8小时内上皮或基底上皮表面未检测到标记丢失;b)追踪24小时后基底上皮表面有明显的标记丢失,而整个上皮的其余部分仍保留适量的放射性。[3H]结合物质对糖胺聚糖降解酶软骨素酶ABC不敏感,但对培养基中衣霉素的存在敏感。早期研究表明,在含有衣霉素(25 ng/ml)的培养基中培养的胚胎小鼠唾液腺,上皮分支正常进行,而上皮生长受到抑制。目前对[3H]甘露糖标记原基的放射自显影研究表明,相对于对照,衣霉素会导致放射性显著降低。因此,我们的结果表明,上皮分支活性与含甘露糖/对衣霉素敏感的糖缀合物沉积的对照水平无关。

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