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Tartan 是细胞表面受体,也是受体酪氨酸磷酸酶 Ptp52F 的潜在体内底物。

The cell surface receptor Tartan is a potential in vivo substrate for the receptor tyrosine phosphatase Ptp52F.

机构信息

Division of Biology, California Institute of Technology, Pasadena, CA 91125, USA.

出版信息

Mol Cell Biol. 2009 Jun;29(12):3390-400. doi: 10.1128/MCB.01764-08. Epub 2009 Mar 30.

Abstract

Receptor-linked protein-tyrosine phosphatases (RPTPs) are essential regulators of axon guidance and synaptogenesis in Drosophila, but the signaling pathways in which they function are poorly defined. We identified the cell surface receptor Tartan (Trn) as a candidate substrate for the neuronal RPTP Ptp52F by using a modified two-hybrid screen with a substrate-trapping mutant of Ptp52F as "bait." Trn can bind to the Ptp52F substrate-trapping mutant in transfected Drosophila S2 cells if v-Src kinase, which phosphorylates Trn, is also expressed. Coexpression of wild-type Ptp52F causes dephosphorylation of v-Src-phosphorylated Trn. To examine the specificity of the interaction in vitro, we incubated Ptp52F-glutathione S-transferase (GST) fusion proteins with pervanadate-treated S2 cell lysates. Wild-type Ptp52F dephosphorylated Trn, as well as most other bands in the lysate. GST "pulldown" experiments demonstrated that the Ptp52F substrate-trapping mutant binds exclusively to phospho-Trn. Wild-type Ptp52F pulled down dephosphorylated Trn, suggesting that it forms a stable Ptp52F-Trn complex that persists after substrate dephosphorylation. To evaluate whether Trn and Ptp52F are part of the same pathway in vivo, we examined motor axon guidance in mutant embryos. trn and Ptp52F mutations produce identical phenotypes affecting the SNa motor nerve. The genes also display dosage-dependent interactions, suggesting that Ptp52F regulates Trn signaling in SNa motor neurons.

摘要

受体连接的蛋白酪氨酸磷酸酶(RPTPs)是果蝇轴突导向和突触发生的重要调节因子,但它们发挥作用的信号通路尚未得到明确界定。我们通过使用带有 Ptp52F 底物捕获突变体的改良双杂交筛选,将细胞表面受体 Tartan(Trn)鉴定为神经元 RPTP Ptp52F 的候选底物。如果表达 v-Src 激酶(该激酶可使 Trn 磷酸化),则 Trn 可以与 Ptp52F 底物捕获突变体在转染的果蝇 S2 细胞中结合。野生型 Ptp52F 的共表达导致 v-Src 磷酸化的 Trn 去磷酸化。为了在体外检查相互作用的特异性,我们将 Ptp52F-谷胱甘肽 S-转移酶(GST)融合蛋白与过钒酸盐处理的 S2 细胞裂解物孵育。野生型 Ptp52F 使 Trn 以及裂解物中的大多数其他条带去磷酸化。GST“下拉”实验表明,Ptp52F 底物捕获突变体仅与磷酸化的 Trn 结合。野生型 Ptp52F 下拉去磷酸化的 Trn,表明它形成了一个稳定的 Ptp52F-Trn 复合物,在底物去磷酸化后仍然存在。为了评估 Trn 和 Ptp52F 是否在体内是同一途径的一部分,我们在突变体胚胎中检查了运动轴突导向。trn 和 Ptp52F 突变产生相同的表型,影响 SNa 运动神经。这些基因还显示出剂量依赖性相互作用,表明 Ptp52F 调节 SNa 运动神经元中的 Trn 信号。

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