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本文引用的文献

1
Cooperative and independent roles of the Drp1 adaptors Mff, MiD49 and MiD51 in mitochondrial fission.动力相关蛋白1(Drp1)衔接蛋白Mff、MiD49和MiD51在线粒体分裂中的协同与独立作用
J Cell Sci. 2016 Jun 1;129(11):2170-81. doi: 10.1242/jcs.185165. Epub 2016 Apr 12.
2
Dynamin-related Protein 1 Oligomerization in Solution Impairs Functional Interactions with Membrane-anchored Mitochondrial Fission Factor.溶液中动力相关蛋白1的寡聚化会损害与膜锚定线粒体分裂因子的功能相互作用。
J Biol Chem. 2016 Jan 1;291(1):478-92. doi: 10.1074/jbc.M115.680025. Epub 2015 Nov 17.
3
Distinct Splice Variants of Dynamin-related Protein 1 Differentially Utilize Mitochondrial Fission Factor as an Effector of Cooperative GTPase Activity.动力相关蛋白1的不同剪接变体以不同方式利用线粒体分裂因子作为协同GTP酶活性的效应器。
J Biol Chem. 2016 Jan 1;291(1):493-507. doi: 10.1074/jbc.M115.680181. Epub 2015 Nov 17.
4
The mechanoenzymatic core of dynamin-related protein 1 comprises the minimal machinery required for membrane constriction.动力相关蛋白1的机械酶核心包含膜收缩所需的最小机制。
J Biol Chem. 2015 May 1;290(18):11692-703. doi: 10.1074/jbc.M114.610881. Epub 2015 Mar 13.
5
Preparation of ready-to-use small unilamellar phospholipid vesicles by ultrasonication with a beaker resonator.使用烧杯谐振器通过超声处理制备即用型小单层磷脂囊泡。
Anal Biochem. 2015 May 15;477:10-2. doi: 10.1016/j.ab.2015.02.015. Epub 2015 Feb 21.
6
Specific interaction with cardiolipin triggers functional activation of Dynamin-Related Protein 1.与心磷脂的特异性相互作用触发动力相关蛋白1的功能激活。
PLoS One. 2014 Jul 18;9(7):e102738. doi: 10.1371/journal.pone.0102738. eCollection 2014.
7
A dimeric equilibrium intermediate nucleates Drp1 reassembly on mitochondrial membranes for fission.一种二聚体平衡中间体促使动力相关蛋白1(Drp1)在线粒体膜上重新组装以进行裂变。
Mol Biol Cell. 2014 Jun 15;25(12):1905-15. doi: 10.1091/mbc.E14-02-0728. Epub 2014 Apr 30.
8
Dynamin assembly strategies and adaptor proteins in mitochondrial fission.线粒体分裂中的动力蛋白组装策略和衔接蛋白
Curr Biol. 2013 Oct 7;23(19):R891-9. doi: 10.1016/j.cub.2013.08.040.
9
Structural insights into oligomerization and mitochondrial remodelling of dynamin 1-like protein.结构洞察解旋酶 1 样蛋白寡聚化和线粒体重排。
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10
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利用支架脂质体在体外重建脂质近端蛋白质-蛋白质相互作用

Using Scaffold Liposomes to Reconstitute Lipid-proximal Protein-protein Interactions In Vitro.

作者信息

Clinton Ryan W, Mears Jason A

机构信息

Department of Pharmacology, Center for Mitochondrial Diseases, The Cleveland Center for Membrane and Structural Biology, Case Western Reserve University School of Medicine.

Department of Pharmacology, Center for Mitochondrial Diseases, The Cleveland Center for Membrane and Structural Biology, Case Western Reserve University School of Medicine;

出版信息

J Vis Exp. 2017 Jan 11(119):54971. doi: 10.3791/54971.

DOI:10.3791/54971
PMID:28117823
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5409191/
Abstract

Studies of integral membrane proteins in vitro are frequently complicated by the presence of a hydrophobic transmembrane domain. Further complicating these studies, reincorporation of detergent-solubilized membrane proteins into liposomes is a stochastic process where protein topology is impossible to enforce. This paper offers an alternative method to these challenging techniques that utilizes a liposome-based scaffold. Protein solubility is enhanced by deletion of the transmembrane domain, and these amino acids are replaced with a tethering moiety, such as a His-tag. This tether interacts with an anchoring group (Ni coordinated by nitrilotriacetic acid (NTA(Ni)) for His-tagged proteins), which enforces a uniform protein topology at the surface of the liposome. An example is presented wherein the interaction between Dynamin-related protein 1 (Drp1) with an integral membrane protein, Mitochondrial Fission Factor (Mff), was investigated using this scaffold liposome method. In this work, we have demonstrated the ability of Mff to efficiently recruit soluble Drp1 to the surface of liposomes, which stimulated its GTPase activity. Moreover, Drp1 was able to tubulate the Mff-decorated lipid template in the presence of specific lipids. This example demonstrates the effectiveness of scaffold liposomes using structural and functional assays and highlights the role of Mff in regulating Drp1 activity.

摘要

体外对整合膜蛋白的研究常常因疏水跨膜结构域的存在而变得复杂。这些研究进一步复杂化的是,将去污剂溶解的膜蛋白重新整合到脂质体中是一个随机过程,其中蛋白质拓扑结构无法强制形成。本文提供了一种替代这些具有挑战性技术的方法,该方法利用基于脂质体的支架。通过删除跨膜结构域来提高蛋白质的溶解度,并用诸如His标签等连接部分取代这些氨基酸。该连接物与锚定基团相互作用(对于带有His标签的蛋白质,由次氮基三乙酸(NTA(Ni))配位的Ni),从而在脂质体表面强制形成统一的蛋白质拓扑结构。给出了一个例子,其中使用这种支架脂质体方法研究了动力相关蛋白1(Drp1)与整合膜蛋白线粒体裂变因子(Mff)之间的相互作用。在这项工作中,我们证明了Mff能够有效地将可溶性Drp1募集到脂质体表面,从而刺激其GTP酶活性。此外,在特定脂质存在的情况下,Drp1能够使Mff修饰的脂质模板形成微管。这个例子通过结构和功能分析证明了支架脂质体的有效性,并突出了Mff在调节Drp1活性中的作用。