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GROMACS 4:  Algorithms for Highly Efficient, Load-Balanced, and Scalable Molecular Simulation.GROMACS 4:高效、负载均衡和可扩展的分子模拟算法。
J Chem Theory Comput. 2008 Mar;4(3):435-47. doi: 10.1021/ct700301q.
2
Distribution of the glycine receptor β-subunit in the mouse CNS as revealed by a novel monoclonal antibody.新型单克隆抗体揭示的小鼠中枢神经系统甘氨酸受体β亚单位的分布。
J Comp Neurol. 2012 Dec 1;520(17):3962-81. doi: 10.1002/cne.23139.
3
Proper synaptic vesicle formation and neuronal network activity critically rely on syndapin I.适当的突触囊泡形成和神经元网络活动依赖于突触联蛋白 I。
EMBO J. 2011 Sep 16;30(24):4955-69. doi: 10.1038/emboj.2011.339.
4
Let's go bananas: revisiting the endocytic BAR code.让我们疯狂一下:重新审视内吞 BAR 码。
EMBO J. 2011 Aug 31;30(17):3501-15. doi: 10.1038/emboj.2011.266.
5
The trafficking proteins Vacuolar Protein Sorting 35 and Neurobeachin interact with the glycine receptor β-subunit.液泡蛋白分选 35 和神经沙滩蛋白与甘氨酸受体β亚基相互作用。
Biochem Biophys Res Commun. 2011 Sep 2;412(3):435-40. doi: 10.1016/j.bbrc.2011.07.110. Epub 2011 Jul 29.
6
The functions of the actin nucleator Cobl in cellular morphogenesis critically depend on syndapin I.肌动蛋白成核因子 Cobl 在细胞形态发生中的功能严重依赖于衔接蛋白 I。
EMBO J. 2011 Jul 1;30(15):3147-59. doi: 10.1038/emboj.2011.207.
7
Molecular basis for SH3 domain regulation of F-BAR-mediated membrane deformation.SH3 结构域调控 F-BAR 介导的膜变形的分子基础。
Proc Natl Acad Sci U S A. 2010 May 4;107(18):8213-8. doi: 10.1073/pnas.1003478107. Epub 2010 Apr 19.
8
PH-domain-driven targeting of collybistin but not Cdc42 activation is required for synaptic gephyrin clustering.PH 结构域驱动的 collybistin 靶向而非 Cdc42 活化对于突触 gephyrin 簇集是必需的。
Eur J Neurosci. 2010 Apr;31(7):1173-84. doi: 10.1111/j.1460-9568.2010.07149.x. Epub 2010 Mar 19.
9
F-BAR proteins of the syndapin family shape the plasma membrane and are crucial for neuromorphogenesis.Syndapin家族的F-BAR蛋白塑造质膜,对神经形态发生至关重要。
J Neurosci. 2009 Oct 21;29(42):13315-27. doi: 10.1523/JNEUROSCI.3973-09.2009.
10
Synaptic activation modifies microtubules underlying transport of postsynaptic cargo.突触激活会改变突触后货物运输所依赖的微管。
Proc Natl Acad Sci U S A. 2009 May 26;106(21):8731-6. doi: 10.1073/pnas.0812391106. Epub 2009 May 13.

糖蛋白受体β亚基(GlyRβ)相互作用蛋白的蛋白质组学分析:衔接蛋白 I 调节突触糖蛋白受体的证据。

Proteomic analysis of glycine receptor β subunit (GlyRβ)-interacting proteins: evidence for syndapin I regulating synaptic glycine receptors.

机构信息

Department of Neurochemistry, Max-Planck-Institute for Brain Research, D-60438 Frankfurt/Main.

Institute for Biochemistry I, Jena University Hospital, Friedrich Schiller University Jena, D-07743 Jena.

出版信息

J Biol Chem. 2014 Apr 18;289(16):11396-11409. doi: 10.1074/jbc.M113.504860. Epub 2014 Feb 7.

DOI:10.1074/jbc.M113.504860
PMID:24509844
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4036276/
Abstract

Glycine receptors (GlyRs) mediate inhibitory neurotransmission in spinal cord and brainstem. They are clustered at inhibitory postsynapses via a tight interaction of their β subunits (GlyRβ) with the scaffolding protein gephyrin. In an attempt to isolate additional proteins interacting with GlyRβ, we performed pulldown experiments with rat brain extracts using a glutathione S-transferase fusion protein encompassing amino acids 378-455 of the large intracellular loop of GlyRβ as bait. This identified syndapin I (SdpI) as a novel interaction partner of GlyRβ that coimmunoprecipitates with native GlyRs from brainstem extracts. Both SdpI and SdpII bound efficiently to the intracellular loop of GlyRβ in vitro and colocalized with GlyRβ upon coexpression in COS-7 cells. The SdpI-binding site was mapped to a proline-rich sequence of 22 amino acids within the intracellular loop of GlyRβ. Deletion and point mutation analysis disclosed that SdpI binding to GlyRβ is Src homology 3 domain-dependent. In cultured rat spinal cord neurons, SdpI immunoreactivity was found to partially colocalize with marker proteins of inhibitory and excitatory synapses. When SdpI was acutely knocked down in cultured spinal cord neurons by viral miRNA expression, postsynaptic GlyR clusters were significantly reduced in both size and number. Similar changes in GlyR cluster properties were found in spinal cultures from SdpI-deficient mice. Our results are consistent with a role of SdpI in the trafficking and/or cytoskeletal anchoring of synaptic GlyRs.

摘要

甘氨酸受体 (GlyRs) 在脊髓和脑干中介导抑制性神经传递。它们通过其β亚基 (GlyRβ) 与支架蛋白神经胶质蛋白的紧密相互作用聚集在抑制性突触后。为了分离与 GlyRβ 相互作用的其他蛋白质,我们使用谷胱甘肽 S-转移酶融合蛋白进行了大鼠脑提取物的下拉实验,该融合蛋白包含 GlyRβ 大细胞内环的氨基酸 378-455 作为诱饵。这鉴定出衔接蛋白 I (SdpI) 是 GlyRβ 的一种新的相互作用伙伴,它与脑提取物中的天然 GlyRs 共免疫沉淀。SdpI 和 SdpII 都能有效地与 GlyRβ 的细胞内环结合,并且在 COS-7 细胞中共表达时会共定位。SdpI 结合位点被映射到 GlyRβ 细胞内环内的一个富含脯氨酸的 22 个氨基酸序列上。缺失和点突变分析表明,SdpI 与 GlyRβ 的结合依赖于 Src 同源性 3 结构域。在培养的大鼠脊髓神经元中,SdpI 免疫反应性部分与抑制性和兴奋性突触的标记蛋白共定位。当 SdpI 通过病毒 miRNA 表达在培养的脊髓神经元中被急性敲低时,突触后 GlyR 簇在大小和数量上都显著减少。在 SdpI 缺陷小鼠的脊髓培养物中也发现了 GlyR 簇特性的类似变化。我们的结果与 SdpI 在突触 GlyR 的运输和/或细胞骨架锚定中的作用一致。