Author
Listed:
- Pontus Nordenfelt
(Marine Biological Laboratory
Marine Biological Laboratory
Children’s Hospital, and Department of Biological Chemistry and Molecular Pharmacology and Medicine, Harvard Medical School
Lund University)
- Travis I. Moore
(Marine Biological Laboratory
Children’s Hospital, and Department of Biological Chemistry and Molecular Pharmacology and Medicine, Harvard Medical School)
- Shalin B. Mehta
(Marine Biological Laboratory
Chan Zuckerberg Biohub)
- Joseph Mathew Kalappurakkal
(Marine Biological Laboratory
Marine Biological Laboratory
National Center for Biological Sciences)
- Vinay Swaminathan
(Marine Biological Laboratory
Marine Biological Laboratory
NHLBI, NIH)
- Nobuyasu Koga
(University of Washington
Institute for Molecular Science)
- Talley J. Lambert
(Harvard Medical School)
- David Baker
(University of Washington)
- Jennifer C. Waters
(Harvard Medical School)
- Rudolf Oldenbourg
(Marine Biological Laboratory)
- Tomomi Tani
(Marine Biological Laboratory)
- Satyajit Mayor
(Marine Biological Laboratory
Marine Biological Laboratory
National Center for Biological Sciences)
- Clare M. Waterman
(Marine Biological Laboratory
Marine Biological Laboratory
NHLBI, NIH)
- Timothy A. Springer
(Marine Biological Laboratory
Marine Biological Laboratory
Children’s Hospital, and Department of Biological Chemistry and Molecular Pharmacology and Medicine, Harvard Medical School)
Abstract
Integrin αβ heterodimer cell surface receptors mediate adhesive interactions that provide traction for cell migration. Here, we test whether the integrin, when engaged to an extracellular ligand and the cytoskeleton, adopts a specific orientation dictated by the direction of actin flow on the surface of migrating cells. We insert GFP into the rigid, ligand-binding head of the integrin, model with Rosetta the orientation of GFP and its transition dipole relative to the integrin head, and measure orientation with fluorescence polarization microscopy. Cytoskeleton and ligand-bound integrins orient in the same direction as retrograde actin flow with their cytoskeleton-binding β-subunits tilted by applied force. The measurements demonstrate that intracellular forces can orient cell surface integrins and support a molecular model of integrin activation by cytoskeletal force. Our results place atomic, Å-scale structures of cell surface receptors in the context of functional and cellular, μm-scale measurements.
Suggested Citation
Pontus Nordenfelt & Travis I. Moore & Shalin B. Mehta & Joseph Mathew Kalappurakkal & Vinay Swaminathan & Nobuyasu Koga & Talley J. Lambert & David Baker & Jennifer C. Waters & Rudolf Oldenbourg & Tom, 2017.
"Direction of actin flow dictates integrin LFA-1 orientation during leukocyte migration,"
Nature Communications, Nature, vol. 8(1), pages 1-16, December.
Handle:
RePEc:nat:natcom:v:8:y:2017:i:1:d:10.1038_s41467-017-01848-y
DOI: 10.1038/s41467-017-01848-y
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