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钙黏蛋白对非洲爪蟾胚胎中细胞定向迁移和组织发生的作用。

Contribution of cadherins to directional cell migration and histogenesis in Xenopus embryos.

作者信息

Broders F, Thiery J P

机构信息

UMR 144 Compartimentation et Dynamique Cellulaires, Institut Curie et CNRS 26, Paris, France.

出版信息

Cell Adhes Commun. 1995 Dec;3(5):419-40. doi: 10.3109/15419069509081296.

Abstract

Perturbation of adhesion mediated by cadherins was achieved by over-expressing truncated forms of E- and EP-cadherins (in which the extracellular domain was deleted) in different blastomeres of stage 6 Xenopus laevis embryos. Injections of mRNA encoding truncated E- and EP-cadherins into A1A2 blastomeres resulted in inhibition of cell adhesion and, at later stages, in morphogenetic defects in the anterior neural tissues to which they mainly contribute. In addition, truncated EP-cadherin mRNA produced a duplication of the dorso-posterior axis in a significant number of cases. The expression of truncated E- and EP-cadherins in blastomeres involved in gastrulation and neural induction (B1B2 and C1), led to the duplication of the dorso-posterior axis as well as to defects in anterior structures. Morphogenetic defects obtained with truncated EP-cadherin were more severe than those induced with truncated E-cadherin. Cells derived from blastomeres injected with truncated EP-cadherin mRNA, dispersed more readily at the blastula and gastrula stages than the cells derived from the blastomeres expressing truncated E-cadherin. Presumptive mesodermal cells expressing truncated cadherins did not engage in coherent directional migration. The alteration of cadherin-mediated cell adhesion led directly to the perturbation of the convergent-extension movements during gastrulation as shown in the animal cap assays and indirectly to perturbation of neural induction. Although the cytoplasmic domains of type I cadherins share a high degree of sequence identity, the over-expression of their cytoplasmic domains induces a distinct pattern of perturbations, strongly suggesting that in vivo, each cadherin may transduce a specific adhesive signal. These graded perturbations may in part result from the relative ability of each cadherin cytoplasmic domain to titer the beta-catenin.

摘要

通过在非洲爪蟾胚胎6期的不同卵裂球中过表达截短形式的E-钙黏蛋白和EP-钙黏蛋白(其中细胞外结构域被删除),实现了对钙黏蛋白介导的黏附的扰动。将编码截短的E-钙黏蛋白和EP-钙黏蛋白的mRNA注射到A1A2卵裂球中,导致细胞黏附受到抑制,并且在后期,它们主要贡献的前神经组织出现形态发生缺陷。此外,在大量情况下,截短的EP-钙黏蛋白mRNA导致背-后轴重复。在参与原肠胚形成和神经诱导的卵裂球(B1B2和C1)中表达截短的E-钙黏蛋白和EP-钙黏蛋白,导致背-后轴重复以及前结构缺陷。用截短的EP-钙黏蛋白获得的形态发生缺陷比用截短的E-钙黏蛋白诱导的更严重。注射截短的EP-钙黏蛋白mRNA的卵裂球衍生的细胞,在囊胚期和原肠胚期比表达截短的E-钙黏蛋白的卵裂球衍生的细胞更容易分散。表达截短钙黏蛋白的预定中胚层细胞没有进行连贯的定向迁移。如动物帽实验所示,钙黏蛋白介导的细胞黏附改变直接导致原肠胚形成期间汇聚延伸运动的扰动,并间接导致神经诱导的扰动。尽管I型钙黏蛋白的细胞质结构域具有高度的序列同一性,但它们细胞质结构域的过表达诱导了不同的扰动模式,强烈表明在体内,每种钙黏蛋白可能转导特定的黏附信号。这些分级扰动可能部分源于每种钙黏蛋白细胞质结构域滴定β-连环蛋白的相对能力。

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