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干细胞生长因子配体对小鼠原始生殖细胞的化学引诱作用及分子信号通路

Chemoattractant action and molecular signaling pathways of Kit ligand on mouse primordial germ cells.

作者信息

Farini Donatella, La Sala Gina, Tedesco Marianna, De Felici Massimo

机构信息

Department of Public Health and Cell Biology, Section of Histology and Embryology, University of Rome Tor Vergata, Via Montpellier 1, 00173 Rome, Italy.

出版信息

Dev Biol. 2007 Jun 15;306(2):572-83. doi: 10.1016/j.ydbio.2007.03.031. Epub 2007 Mar 28.

DOI:10.1016/j.ydbio.2007.03.031
PMID:17467686
Abstract

Using a Transwell chamber as migration assay for mouse primordial germ cells (PGCs), we show here that these cells posses directional migration in the absence of somatic cell and defined matrix support and in response to a Kit ligand (KL) gradient or medium conditioned by Aorta/Gonad/Mesonephros and gonadal ridges. Other putative PGC chemoattractants such as SDF1 and TGFbeta did not exert any attractive action on PGCs. The chemoattractant activity of KL and conditioned medium was also evidenced by their ability to stimulate actin reorganization in PGCs. In the aim to identify downstream signaling pathways governing KL chemoattraction on PGCs, we demonstrated that in such cells KL rapidly (5 min) increased autophosphorylation of its receptor c-Kit and caused phosphorylation of the serine-threonine kinase AKT through the action of PI3K. 740Y-P peptide, a direct activator of PI3 kinase, stimulated PGC migration at levels similar to those elicited by KL. LY294002 (a specific inhibitor of PI3K) abolished KL-dependent PGC migration or the chemoattractant activity of the conditioned medium and inhibited AKT phosphorylation; Src kinase inhibitors PP2 and SU6656, caused significant reduction of the KL-dependent PGC migration and AKT phosphorylation, while U0126, a selective inhibitor of the MEK/ERK protein kinase cascade, reduced PGC migration and AKT phosphorylation at lesser extent. SU6656 completely abolished the chemoattractant activity of the conditioned medium. Finally, SB202190 (a p38 inhibitor) and rapamycin (mTOR inhibitor) did not affect PGC migration. In addition, to demonstrate that somatic cells are not essential for PGC motility and directional migration, we evidenced a novel role for KL as PGC chemoattractant and for PI3K/AKT and Src kinase, as players involved in the activation of the PGC migratory machinery and likely important for their directional movement towards the gonadal ridges.

摘要

利用Transwell小室对小鼠原始生殖细胞(PGCs)进行迁移分析,我们在此表明,这些细胞在没有体细胞和特定基质支持的情况下,能够响应Kit配体(KL)梯度或由主动脉/性腺/中肾及性腺嵴条件培养基的作用进行定向迁移。其他假定的PGC趋化因子,如SDF1和TGFβ,对PGCs没有任何吸引作用。KL和条件培养基的趋化活性还通过它们刺激PGCs中肌动蛋白重组的能力得到证明。为了确定控制KL对PGCs趋化作用的下游信号通路,我们证明在这些细胞中,KL迅速(5分钟)增加其受体c-Kit的自磷酸化,并通过PI3K的作用导致丝氨酸-苏氨酸激酶AKT的磷酸化。740Y-P肽是PI3激酶的直接激活剂,其刺激PGC迁移的水平与KL引起的水平相似。LY294002(PI3K的特异性抑制剂)消除了KL依赖的PGC迁移或条件培养基的趋化活性,并抑制了AKT磷酸化;Src激酶抑制剂PP2和SU6656显著降低了KL依赖的PGC迁移和AKT磷酸化,而U0126(MEK/ERK蛋白激酶级联的选择性抑制剂)在较小程度上降低了PGC迁移和AKT磷酸化。SU6656完全消除了条件培养基的趋化活性。最后,SB202190(一种p38抑制剂)和雷帕霉素(mTOR抑制剂)不影响PGC迁移。此外,为了证明体细胞对PGC运动性和定向迁移不是必需的,我们证明了KL作为PGC趋化因子以及PI3K/AKT和Src激酶的新作用,它们是参与激活PGC迁移机制的参与者,可能对它们向性腺嵴的定向移动很重要。

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