Postdoctoral Position Available

Elizabeth Luna, Ph.D.

Academic Role: Professor

Faculty Appointment(s) In:
   Cell Biology

Other Affiliation(s):
   Cancer Center
   Cell Dynamics Group
   Interdisciplinary Graduate Program
   Program in Immunology and Virology

Membrane Skeleton Dynamics, Motility, Adhesion, Signal Transduction

As cells move, internal movements caused by their actin and microtubule cytoskeletons must be coordinated with events at their plasma membranes.  During the cycle of events associated with cell translocation, the cells extend surface protrusions at their leading edges, make contact with the substratum at focal adhesions, and then disassemble the focal adhesions in the rear of the cell as the cell retracts its posterior to provide material for another round of surface protrusion.  A lot is known about individual steps in this cycle, but much less is known about how the different steps are coordinated at the interface between the membrane and the cytoskeleton, a region of the cell known as the "membrane skeleton". 

Our laboratory is interested in how the membrane skeleton controls the component events during very rapid cell movement, how it regulates cellular processes, such as chemotaxis and matrix invasion, and how these proteins are involved in organism-scale motile phenomena, including wound healing and immune function.  Most of the same or similar proteins that we found in membrane skeletons from neutrophils (a type of white blood cell) also exist in human cervical and breast carcinoma cell lines and in smooth and striated muscle membranes.  These proteins include cytoskeletal proteins (spectrin, actin, myosins I and II, a -actinin, supervillin), signaling proteins (Src family kinases, heterotrimeric G proteins), and proteins that organize cholesterol-enriched membrane domains (stomatin, flotillins).

Of these membrane skeleton proteins, supervillin is of special interest to us.  Supervillin binds tightly to the neutrophil plasma membrane and also binds directly to at least six different cytoskeletal proteins, including actin- and microtubule-associated motors.  Additional candidate supervillin interaction partners include a large number of oncogenes, tumor suppressors, and other proteins implicated in motile processes. Over- and under-expression of supervillin affects each step of the motility cycle. The gene encoding supervillin maps to a region of human chromosome 10p implicated in tumor cell motility and susceptibility to obesity and diabetes.  Taken together, the working hypothesis is that supervillin is a membrane-associated adapter protein that works with a group of interacting proteins to regulate rapid motility and associated signaling processes in many cell types.

The supervillin-associated membrane skeleton localizes to specialized membrane structures, called podosomes in tissue culture cells and costameres in striated muscle.  Targeting of supervillin structures to cell-substrate contact sites called focal adhesions results in focal adhesion disassembly.  Reduced levels of supervillin disrupt the stimulus-mediated activation of the ERK1/2 family of mitogen-activated kinases, suggesting an important signaling role at either the plasma membrane or at internal sites of ERK1/2 activation.  Live cell imaging of EGFP-tagged supervillin is consistent with associations with internal trafficking membranes, as well as at the plasma membrane.

Current projects include exploring the biochemical basis for supervillin-mediated activation of myosin contractility, identifying the mechanism(s) by which supervillin promotes reorganization of the actin cytoskeleton during invasion of extracellular matrices, and characterization of the role of the supervillin cytoskeleton during endosomal trafficking.  We also have generated a supervillin-deficient mouse for studies of organ function; initial experiments on muscle contractility, immune function, and wound healing are in progress.  The overall working hypothesis is that the supervillin-associated membrane skeleton coordinates cell motility and matrix invasion by promoting protein activation and trafficking at several steps in the motility cycle.  The long-term goal is to understand how this coordination works during the motility and invasion associated with immune function, cancer metastasis, embryogenesis, and the formation of new blood vessels.

  

Figure 1: The intracellular localization of supervillin in MDBK cells is a function of cell density and adherence state. In subconfluent cells (left), supervillin (red) is found in the nucleus, in the cytoplasm, and in spots along the plasma membrane with the cell adhesion protein, E-cadherin (green). In confluent cells (right), supervillin and E-cadherin co-localize almost completely (yellow) at sites of lateral cell-cell contact.

Figure 2: Working model of the neutrophil membrane skeleton.  Supervillin is the most cytoskeletal protein that is the most proximal to the membrane bilayer, followed by myosins I and II (Nebl et al., 2002).

Movie: EGFP-supervillin in COS7 cells localizes with dynamic structures at and near the cell periphery.  Some of these structures are peripheral bundles of membrane-associated actin and myosin II; other EGFP-supervillin localizations appear to be trafficking endosomal membranes.

Recent Publications

Crowley  , J.L., Takizawa, N., Smith, T.C., and Luna, E.J.  Supervillin: A membrane skeleton protein at invadopodia and Src-induced podosomes.  In preparation.

Takizawa N., Ikebe R., Ikebe M, and Luna, E.J. (2007) Supervillin slows cell spreading by facilitating myosin II activation at the cell periphery.  J. Cell Sci. 120, 3792-3803.

Takizawa, N., Smith, T.C., Nebl, T., Crowley, J.L., Palmieri, S.J., Lifshitz, L.M., Ehrhardt, A.G., Hoffman, L.M., Beckerle, M.C. and Luna, E.J. (2006) Supervillin modulation of focal adhesions involving TRIP6/ZRP-1.  J. Cell Biol. 174, 447-458.

Gangopadhyay, S.S., Takizawa, N., Gallant, C., Barber, A.L., Je, H.D., Smith, T.C., Luna, E.J. and Morgan, K.G. (2004)  Smooth muscle archvillin:  A novel regulator of contractility in vascular smooth muscle.  J. Cell Sci.  117, 5043-5057.

Chen, Y., Takizawa, N., Crowley, J.L., Oh, S.W., Gatto, C., Li, X., Kambara, T., Sato, O., Ikebe, M. and Luna, E.J. (2003) F-actin and myosin II binding domains in supervillin. J. Biol. Chem. 278:  46094-46106.

Oh, S.W., Pope, R.K., Smith, K.P., Crowley, J.L., Nebl, T., Lawrence, J.B., and Luna, E.J. (2003) Archvillin, a muscle-specific isoform of supervillin, is an early-expressed component of the costameric membrane skeleton.  J. Cell Sci.  116, 2261-2275.

Nebl, T., Pestonjamasp, K.N., Leszyk, J.D., Crowley, J.L., Oh, S.W. and Luna, E.J. (2002) Proteomic analysis of a detergent-resistant membrane skeleton from neutrophil plasma membranes.  J. Biol. Chem. 277: 43399-43409.

Potential Rotation Projects

Rotation projects involving biochemical, molecular genetic, and/or cell-based techniques can be tailored to the interests of the students.  Questions associated with ongoing projects described above in the Research section are available for students who want to learn a specific technique.  Questions relevant to the laboratory’s interests that could be developed into independent thesis projects include:

1. Medium throughput functional screens of supervillin-associated proteins to determine which influence motility, adhesion, contractility, or the formation and function of matrix-invading structures called invadopodia;
2. Analysis of motile and signaling dysfunctions in cells and tissues from mice deficient in expression of supervillin isoforms; and
3. Function of these membrane skeleton proteins during ‘nongenomic’, plasma membrane-based, responses to steroid receptors in breast or prostate cancer cells.

Laboratory Personnel

Norio Takizawa, Ph.D., Instructor

Zhiyou Fang, Ph.D., Postdoctoral Fellow

Jessica Crowley, Graduate Student

Tara Smith, Research Technician

Academic Background

B.A., Chemistry, Southern Illinois University at Carbondale. 1972
Ph.D., Physical Chemistry, Stanford University, 1977.
NIH postdoctoral fellow, Cell and Molecular Biology, The Biological Laboratories, Harvard University, 1977-81
Princeton University, Biology Department, 1981-88
The Worcester Foundation for Experimental Biology, 1988-97
University of Massachusetts Medical School,1989-present

Office: Biotech 4 Suite 306
Phone: 508-856-8661
E-mail: Elizabeth.Luna@umassmed.edu
Keywords: Nuclear Receptors, Cell Dynamics, Cell Biology, Muscle Membrane Biochemistry, Metastasis

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Postdoctoral Position Available A postdoctoral position is available to study in this laboratory. Contact Dr. Luna for additional details.