首页> 美国卫生研究院文献>The Journal of Biophysical and Biochemical Cytology >Assembly of the intestinal brush border: appearance and redistribution of microvillar core proteins in developing chick enterocytes
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Assembly of the intestinal brush border: appearance and redistribution of microvillar core proteins in developing chick enterocytes

机译:肠刷缘的组装:发育中的小鸡肠上皮细胞中微绒毛核心蛋白的出现和重新分布

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摘要

The assembly of the intestinal microvillus cytoskeleton during embryogenesis in the chick was examined by immunochemical and light microscopic immunolocalization techniques. For these studies, affinity- purified antibodies reactive with three major cytoskeletal proteins of the adult intestinal microvillus, fimbrin, villin, and the 110-kD subunit of the 110K-calmodulin protein complex were prepared. Immunocytochemical staining of frozen sections of embryonic duodena revealed that all three proteins were present at detectable levels at the earliest stages examined, day 7-8 of incubation (Hamilton/Hamburger stages 25-30). Although initially all three proteins were diffusely distributed throughout the cytoplasm, there was a marked asynchrony in the accumulation of these core proteins within the apical domain of the enterocyte. Villin displayed concentrated apical staining by embryonic day 8 (stage 28), while the apical concentration of fimbrin was first observed at embryonic day 10 (stage 37). Diffuse staining of the enterocyte cytoplasm with the anti-110K was observed throughout development until a few days before hatch. By embryonic day 19-21 110K staining was concentrated at the cell periphery (apical and basolateral). The restricted apical localization characteristic of 110K in the adult brush border was not observed until the day of hatching. Immunoblot analysis of whole, solubilized embryonic duodena confirmed the presence of 110K, villin, and fimbrin throughout development and indicated substantial increases in all three proteins, particularly late in development. Immunoblot staining with anti-110K also revealed the presence of a high molecular mass (200 kD) immunoreactive species in embryonic intestine. This 200-kD form was absent from isolated embryonic enterocytes and may be a component of intestinal smooth muscle.
机译:通过免疫化学和光学显微镜免疫定位技术检查了鸡胚发生过程中肠道微绒毛细胞骨架的组装。对于这些研究,制备了与成年肠道微绒毛,纤维蛋白,villin和110K-钙调蛋白蛋白复合物的110-kD亚基的三种主要细胞骨架蛋白反应的亲和纯化抗体。胚胎十二指肠冷冻切片的免疫细胞化学染色显示,在检查的最早阶段,即孵化的第7-8天(汉密尔顿/汉堡阶段25-30),所有三种蛋白质均以可检测的水平存在。尽管最初所有三种蛋白质均分散在整个细胞质中,但这些核心蛋白质在肠上皮细胞顶端结构域内的积累却存在明显的异步性。 Villin在胚胎第8天(第28阶段)显示出浓厚的根尖染色,而在胚胎第10天(第37阶段)首先观察到了纤维蛋白的根尖浓度。在整个发育过程中直至孵化前几天,均观察到用抗110K对肠上皮细胞质进行了弥漫性染色。到胚胎第19-21天时,110K染色集中在细胞外围(顶端和基底外侧)。直到孵化之日,才观察到在成年刷缘的110K的根尖局限性特征。完整的可溶性胚胎十二指肠的免疫印迹分析证实了在整个发育过程中均存在110K,villin和fimbrin,并表明所有这三种蛋白质(特别是在发育后期)均大量增加。用抗110K进行的免疫印迹染色还揭示了胚胎小肠中存在高分子量(200 kD)免疫反应物种。分离的胚胎肠上皮细胞不存在这种200 kD的形式,可能是肠平滑肌的组成部分。

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