Abstract

The control of membrane shape and curvature is essential for many vital cellular functions, including cell division and cell motility, as well as vesicle budding and fusion. Recent work has shown that these processes are regulated by proteins that can sense, stabilize or induce membrane curvature. Not surprisingly, aberrations in the control of membrane curvature have been linked to a number of diseases, including mental retardation, cancer and muscular dystrophy. The underlying molecular mechanisms, however, are poorly understood since little structural information exists for the biologically relevant membrane-bound forms of the curvature-sensing or inducing proteins. The central goal of this proposal is to provide such detailed structural and mechanistic information.
Aim 1 investigates the molecular mechanisms by which annexins can sense membrane curvature. This remarkable process causes a major inside-out refolding of annexins and brings buried hydrophobic residues of the solution structure into direct contact with the acyl chains of the membranes. Using a combination of continuous wave and pulsed EPR spectroscopy, the proposed work will define the three-dimensional structure of this membrane-bound form and test the hypothesis that N-terminal phosphorylation modulates curvature- dependent membrane interaction in vivo. Furthermore, it will be tested, whether the structure of the curvature- dependent membrane bound forms is related to that of the interfacial, pH-dependent membrane-bound form.
Aim 2 investigates the membrane-bound forms of the curvature-inducing N-BAR proteins endophilin and amphiphysin, while aim 3 addresses the structure of the membrane-bound form of the F-BAR protein FCHo2. The detailed structural studies proposed in both aims are designed to test the hypothesis that BAR domain proteins induce membrane curvature using a combination of three different mechanisms: (1) by acting as scaffolds that mold a specific membrane curvature;(2) by """"""""wedging"""""""" amphipathic helices into the membrane;and (3) by forming specifically aligned oligomeric structures. In particular it will be tested whether N-BAR and F-BAR proteins induce curvature by using the aforementioned mechanisms to different extents. All structural data obtained from the EPR analysis will be refined further using the recently developed PRONOX algorithm which will be employed to generate three-dimensional structural models that contain the proteins as well as the lipid membranes. These models will provide direct insight into the molecular mechanisms by which BAR domain-containing proteins induce membrane curvature. Structural analysis will further be used to test the mechanism by which amphiphysin-2 mutants (K35N and D151N) have reduced curvature-inducing properties and misfunction in familial forms of centronuclear myopathy.

Public Health Relevance

All cells need to be able to control the shapes and curvatures of their membranes. When this process is not working properly, it can lead to diseases such as cancer, muscular dystrophy and mental retardation. The present proposal seeks to establish the mechanism by which proteins involved in this process can sense and induce the appropriate curvature of cellular membranes. The results will have implications for our understanding and treatment of the aforementioned diseases.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM063915-07
Application #
7789583
Study Section
Biochemistry and Biophysics of Membranes Study Section (BBM)
Program Officer
Ainsztein, Alexandra M
Project Start
2001-07-01
Project End
2013-01-31
Budget Start
2010-02-01
Budget End
2011-01-31
Support Year
7
Fiscal Year
2010
Total Cost
$335,910
Indirect Cost

  Institution

Name
University of Southern California
Department
Neurosciences
Type
Schools of Medicine
DUNS #
072933393
City
Los Angeles
State
CA
Country
United States
Zip Code
90089

  Publications

Marotta, Nicholas P; Lin, Yu Hsuan; Lewis, Yuka E et al. (2015) O-GlcNAc modification blocks the aggregation and toxicity of the protein ?-synuclein associated with Parkinson's disease. Nat Chem 7:913-20
Ambroso, Mark R; Haworth, Ian S; Langen, Ralf (2015) Structural Characterization of Membrane-Curving Proteins: Site-Directed Spin Labeling, EPR, and Computational Refinement. Methods Enzymol 564:259-88
Kegulian, Natalie C; Sankhagowit, Shalene; Apostolidou, Melania et al. (2015) Membrane Curvature-sensing and Curvature-inducing Activity of Islet Amyloid Polypeptide and Its Implications for Membrane Disruption. J Biol Chem 290:25782-93
Isas, J Mario; Ambroso, Mark R; Hegde, Prabhavati B et al. (2015) Tubulation by amphiphysin requires concentration-dependent switching from wedging to scaffolding. Structure 23:873-881
Lai, Ying; Kim, Sunae; Varkey, Jobin et al. (2014) Nonaggregated ?-synuclein influences SNARE-dependent vesicle docking via membrane binding. Biochemistry 53:3889-96
Ambroso, Mark R; Hegde, Balachandra G; Langen, Ralf (2014) Endophilin A1 induces different membrane shapes using a conformational switch that is regulated by phosphorylation. Proc Natl Acad Sci U S A 111:6982-7
Shah, Claudio; Hegde, Balachandra G; Morén, Björn et al. (2014) Structural insights into membrane interaction and caveolar targeting of dynamin-like EHD2. Structure 22:409-420
Cheng, Chi-Yuan; Varkey, Jobin; Ambroso, Mark R et al. (2013) Hydration dynamics as an intrinsic ruler for refining protein structure at lipid membrane interfaces. Proc Natl Acad Sci U S A 110:16838-43
Moaven, Hormoz; Koike, Yukihiro; Jao, Christine C et al. (2013) Visual arrestin interaction with clathrin adaptor AP-2 regulates photoreceptor survival in the vertebrate retina. Proc Natl Acad Sci U S A 110:9463-8
Ruggiero, Linda; Connor, Mark P; Chen, Jeannie et al. (2012) Diurnal, localized exposure of phosphatidylserine by rod outer segment tips in wild-type but not Itgb5-/- or Mfge8-/- mouse retina. Proc Natl Acad Sci U S A 109:8145-8

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