Cinemicrographic study of the cell movement in the primitive-streak-stage mouse embryo.

N Nakatsuji, M H Snow, C C Wylie
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Abstract

Migration of the mesoderm cells in the primitive-streak-stage mouse embryo was directly studied by cinemicrography using whole embryo culture and Nomarski differential interference contrast optics. Relative transparency and small size of the early mouse embryos enabled direct observation of the individual cells and their cell processes. Seven-day-old mouse embryos were isolated and cultured in a small chamber in a medium consisting of 50% rat serum and 50% Dulbecco's modified minimum essential medium. The mesoderm cells move away from the primitive streak in both anterior and antimesometrial (distal) directions at a mean velocity of 46 micron h-1. They extend cell processes and constantly change cell shape. They do not translocate extensively as isolated single cells, but usually maintain attachment to other mesoderm cells. They show frequent cell division preceded by rounding up of the cell bodies, and accompanied by vigorous blebbing before and after cytokinesis. This study shows that it is possible to examine the motility of embryonic cells inside the mammalian embryo by direct observation if the embryo is small and transparent enough for the use of the Nomarski optics.

原始条纹期小鼠胚胎细胞运动的电影显微摄影研究。
采用全胚培养和诺玛斯基差差干涉对比光学技术,用显微摄影技术直接研究了原始条纹期小鼠胚胎中胚层细胞的迁移。相对透明和小尺寸的早期小鼠胚胎可以直接观察单个细胞及其细胞过程。7天大的小鼠胚胎被分离并在一个小室中培养,培养基由50%的大鼠血清和50%的Dulbecco改良的最低基本培养基组成。中胚层细胞以46微米/小时的平均速度从原始条纹的前、反中胚层(远端)方向移动。它们延长细胞过程,不断改变细胞形状。它们不作为孤立的单个细胞广泛地移位,但通常与其他中胚层细胞保持附着。它们表现为频繁的细胞分裂,在细胞体聚集之前,伴随着细胞质分裂前后剧烈的气泡。这项研究表明,如果胚胎足够小,足够透明,可以使用诺马尔斯基光学,那么通过直接观察来检查哺乳动物胚胎内胚胎细胞的运动是可能的。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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