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鸡脊索上皮细胞在体外形成含脯氨酸的细胞外结缔组织纤维的过程。

The development of proline-containing extracellular connective tissue fibrils by chick notochordal epithelium in vitro.

作者信息

Lauscher C K, Carlson E C

出版信息

Anat Rec. 1975 Jun;182(2):151-67. doi: 10.1002/ar.1091820203.

Abstract

Notochords were isolated from Hamburger-Hamilton stages 13-15 chick embryos by trypsinization and microdissection. These were shown by electron microscopy to be completely devoid of extracellular materials or mesenchymal contaminants. Cultivation of notochordal isolates was carried out on a non-collagenous (Falcon Plastic) substratum for 0 to 48 hours. At 12 hours of in vitro incubation, a discontinuous basal lamina could be demonstrated on the surface of notochordal cells. This was followed by the appearance of microfibrils of various sizes and other components of the extracellular matrix. By 48 hours of in vitro incubation, the same extracellular materials which surround the notochord in vivo (notochord sheath) could be demonstrated in vitro. Autoradiographic studies show that tritiated proline is taken up by notochordal cells and secreted to the extracellular space where label is associated with basal lamina, microfibrils and ground substance. When cis-hydroxyproline, a known collagen-specific inhibitor is added to the system, tritiated proline label is located primarily intracellularly and fewer areas of active fibrillogenesis are noted. This suggests that ultrastructurally recognizable materials produced by notochordal cells in vitro may be at least partially collagenous. Significantly, these materials are produced in vivo at the same time (following stage 10) that notochordal tissues actively induce somite differentiation and cartilage formation. It seems reasonable that a biochemically or ultrastructurally identifiable component of the extracellular matrix may possibly mediate such induction.

摘要

通过胰蛋白酶消化和显微解剖从汉伯格-汉密尔顿13-15期鸡胚中分离出脊索。电子显微镜显示这些脊索完全没有细胞外物质或间充质污染物。将分离的脊索在非胶原(Falcon塑料)基质上培养0至48小时。在体外培养12小时时,可在脊索细胞表面显示出不连续的基膜。随后出现各种大小的微原纤维和细胞外基质的其他成分。在体外培养48小时时,可在体外显示出与体内围绕脊索的相同细胞外物质(脊索鞘)。放射自显影研究表明,氚标记的脯氨酸被脊索细胞摄取并分泌到细胞外空间,在那里标记物与基膜、微原纤维和基质相关。当向系统中加入顺式羟脯氨酸(一种已知的胶原特异性抑制剂)时,氚标记的脯氨酸标记主要位于细胞内,且观察到的活跃纤维形成区域较少。这表明脊索细胞在体外产生的超微结构可识别物质可能至少部分是胶原性的。重要的是,这些物质在体内产生的时间(在第10阶段之后)与脊索组织积极诱导体节分化和软骨形成的时间相同。细胞外基质中一种在生化或超微结构上可识别的成分可能介导这种诱导作用,这似乎是合理的。

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