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生肌细胞从发育中小鼠胚胎的体节迁移至前肢芽。

Migration of myogenic cells from the somites to the fore-limb buds of developing mouse embryos.

作者信息

Sze L Y, Lee K K, Webb S E, Li Z, Paulin D

机构信息

Department of Anatomy, Faculty of Medicine, Chinese University of Hong Kong, Shatin.

出版信息

Dev Dyn. 1995 Jul;203(3):324-36. doi: 10.1002/aja.1002030305.

Abstract

In this study, we have isolated newly formed somites from the caudal regions of 8.5 day mouse embryos and transplanted them orthotopically into correspondingly staged hosts at the level of the prospective limb-forming region. The experimental embryos were then cultured intact for 32-36 hr. The donor somites used were pre-labelled with DiI, a fluorescent lipophilic dye, or were obtained from transgenic embryos that carried a 1 kb 5' regulatory sequence of the desmin gene linked to the gene encoding Escherichia coli beta-galactosidase. The transgene is specifically expressed in skeletal muscles (Li et al. [1993] Development 117:947-959). The aim of these experiments was to show definitively that the musculature of the mammalian limb is derived from the somites. The results demonstrated that DiI-labelled cells from the implanted somites were able to invade the proximal region of the fore-limb bud during the course of development. The use of transgenic somites as grafts confirmed that some of the somitic cells found in the limbs were myogenic cells. To determine whether the displacement of somitic cells is an active or passive process, somatopleure obtained from the prospective limb-forming regions of day 8.5 day embryos was implanted into 8.5 day hosts. We did not detect the presence of DiI-labelled somatopleural cells in the fore-limb after 32-36 hr of culture. This suggests that somitic cells reached the limb bud via active locomotion rather than as a result of being passively dragged there, as the limb elongates during development. In addition, we injected latex beads into the somites, as probes, to determine whether extracellular matrix-driven translocation plays a role in driving the somitic cells to the limb bud. In a majority of the specimens examined, we could not detect the presence of these beads in the limb bud. However, in the trunk of these embryos, the beads were found dispersed throughout the ventral neural crest pathway.

摘要

在本研究中,我们从8.5天龄小鼠胚胎的尾部区域分离出新形成的体节,并将其原位移植到处于相应发育阶段的宿主的预期肢体形成区域水平。然后将实验胚胎完整培养32 - 36小时。所使用的供体体节预先用亲脂性荧光染料DiI标记,或者取自携带与大肠杆菌β - 半乳糖苷酶编码基因相连的结蛋白基因1 kb 5'调控序列的转基因胚胎。该转基因在骨骼肌中特异性表达(Li等人,[1993]《发育》117:947 - 959)。这些实验的目的是明确证明哺乳动物肢体的肌肉组织源自体节。结果表明,植入体节的DiI标记细胞在发育过程中能够侵入前肢芽的近端区域。使用转基因体节作为移植物证实,在肢体中发现的一些体节细胞是成肌细胞。为了确定体节细胞的移位是一个主动还是被动过程,将从8.5天龄胚胎的预期肢体形成区域获得的体壁植入8.5天龄的宿主中。培养32 - 36小时后,我们在前肢中未检测到DiI标记的体壁细胞的存在。这表明体节细胞是通过主动运动到达肢体芽,而不是由于在发育过程中肢体伸长而被被动拖到那里的。此外,我们将乳胶珠作为探针注入体节,以确定细胞外基质驱动的转运是否在将体节细胞驱动到肢体芽中起作用。在大多数检查的标本中,我们在肢体芽中未检测到这些珠子的存在。然而,在这些胚胎的躯干中,发现珠子分散在整个腹侧神经嵴路径中。

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