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施佩曼组织者基因“鹅膏蕈氨酸”促进神经母细胞从耳泡中分层。

Spemann organizer gene Goosecoid promotes delamination of neuroblasts from the otic vesicle.

作者信息

Kantarci Husniye, Gerberding Andrea, Riley Bruce B

机构信息

Biology Department, Texas A&M University, College Station, TX 77843-3258.

Biology Department, Texas A&M University, College Station, TX 77843-3258

出版信息

Proc Natl Acad Sci U S A. 2016 Nov 1;113(44):E6840-E6848. doi: 10.1073/pnas.1609146113. Epub 2016 Oct 19.

Abstract

Neurons of the Statoacoustic Ganglion (SAG), which innervate the inner ear, originate as neuroblasts in the floor of the otic vesicle and subsequently delaminate and migrate toward the hindbrain before completing differentiation. In all vertebrates, locally expressed Fgf initiates SAG development by inducing expression of Neurogenin1 (Ngn1) in the floor of the otic vesicle. However, not all Ngn1-positive cells undergo delamination, nor has the mechanism controlling SAG delamination been elucidated. Here we report that Goosecoid (Gsc), best known for regulating cellular dynamics in the Spemann organizer, regulates delamination of neuroblasts in the otic vesicle. In zebrafish, Fgf coregulates expression of Gsc and Ngn1 in partially overlapping domains, with delamination occurring primarily in the zone of overlap. Loss of Gsc severely inhibits delamination, whereas overexpression of Gsc greatly increases delamination. Comisexpression of Ngn1 and Gsc induces ectopic delamination of some cells from the medial wall of the otic vesicle but with a low incidence, suggesting the action of a local inhibitor. The medial marker Pax2a is required to restrict the domain of gsc expression, and misexpression of Pax2a is sufficient to block delamination and fully suppress the effects of Gsc The opposing activities of Gsc and Pax2a correlate with repression or up-regulation, respectively, of E-cadherin (cdh1). These data resolve a genetic mechanism controlling delamination of otic neuroblasts. The data also elucidate a developmental role for Gsc consistent with a general function in promoting epithelial-to-mesenchymal transition (EMT).

摘要

支配内耳的 statoacoustic 神经节(SAG)神经元起源于耳泡底部的神经母细胞,随后脱层并向后脑迁移,然后完成分化。在所有脊椎动物中,局部表达的 Fgf 通过诱导神经泡底部的 Neurogenin1(Ngn1)表达来启动 SAG 发育。然而,并非所有 Ngn1 阳性细胞都会发生脱层,且控制 SAG 脱层的机制尚未阐明。在此我们报告,以调节 Spemann 组织者中的细胞动态而闻名的 Goosecoid(Gsc),调节耳泡中神经母细胞的脱层。在斑马鱼中,Fgf 在部分重叠区域共同调节 Gsc 和 Ngn1 的表达,脱层主要发生在重叠区域。Gsc 的缺失严重抑制脱层,而 Gsc 的过表达则大大增加脱层。Ngn1 和 Gsc 的共表达诱导耳泡内侧壁的一些细胞异位脱层,但发生率较低,这表明存在局部抑制剂的作用。内侧标记物 Pax2a 是限制 gsc 表达域所必需的,Pax2a 的错误表达足以阻断脱层并完全抑制 Gsc 的作用。Gsc 和 Pax2a 的相反活性分别与 E-钙黏蛋白(cdh1)的抑制或上调相关。这些数据解析了控制耳神经母细胞脱层的遗传机制。这些数据还阐明了 Gsc 在促进上皮-间充质转化(EMT)的一般功能中所具有的发育作用。

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