Vanroelen C, Vakaet L, Andries L
Anat Embryol (Berl). 1980;159(3):361-7. doi: 10.1007/BF00317656.
Primitive streak stage chick blastoderms were cultured for 30 min on a medium containing tritiated glucosamine. Light microscope autoradiography revealed extracellular labeling, and pretreatment of the sections with testicular hyaluronidase suggested the glycosaminoglycan nature of the labeled products. After incorporation of the tritiated precursor, some blastoderms were transferred to a chase medium, and cultured for 30, 90, 210 min. The changes is distribution of the labeled testicular hyaluronidase-sensitive macromolecules during the chase experiment illustrated the ingression of cells in the primitive streak stage chick blastoderm. Grain density differences, resulting from the various chase periods, suggested the renewal of the testicular hyaluronidase-sensitive fraction.
将原肠胚期鸡胚盘在含有氚标记葡糖胺的培养基上培养30分钟。光学显微镜放射自显影显示细胞外标记,用睾丸透明质酸酶预处理切片表明标记产物具有糖胺聚糖性质。掺入氚标记前体后,将一些胚盘转移至追踪培养基中,再培养30、90、210分钟。追踪实验期间标记的对睾丸透明质酸酶敏感的大分子分布变化说明了原肠胚期鸡胚盘中细胞的内迁。不同追踪期导致的颗粒密度差异表明对睾丸透明质酸酶敏感部分的更新。