4.8 Article

Luminal signalling links cell communication to tissue architecture during organogenesis

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NATURE
卷 515, 期 7525, 页码 120-+

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NATURE PUBLISHING GROUP
DOI: 10.1038/nature13852

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  1. European Molecular Biology Organization
  2. EMBL Interdisciplinary Postdocs (EIPOD)
  3. Deutsche Forschungsgemeinschaft [SFB 488]

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Morphogenesis is the process whereby cell collectives are shaped into differentiated tissues and organs(1). The self-organizing nature of morphogenesis has been recently demonstrated by studies showing that stem cells in three-dimensional culture can generate complex organoids, such as mini-guts(2), optic-cups(3) and even mini-brains(4). To achieve this, cell collectives must regulate the activity of secreted signalling molecules that control cell differentiation, presumably through the self-assembly of microenvironments or niches. However, mechanisms that allow changes in tissue architecture to feedback directly on the activity of extracellular signals have not been described. Here we investigate how the process of tissue assembly controls signalling activity during organogenesis in vivo, using the migrating zebrafish lateral line primordium(5). We show that fibroblast growth factor (FGF) activity within the tissue controls the frequency at which it deposits rosette-like mechanosensory organs. Live imaging reveals that FGF becomes specifically concentrated in microluminal structures that assemble at the centre of these organs and spatially constrain its signalling activity. Genetic inhibition of microlumen assembly and laser micropuncture experiments demonstrate that microlumina increase signalling responses in participating cells, thus allowing FGF to coordinate the migratory behaviour of cell groups at the tissue rear. As the formation of a central lumen is a self-organizing property of many cell types, such as epithelia(6) and embryonic stem cells(7), luminal signalling provides a potentially general mechanism to locally restrict, coordinate and enhance cell communication within tissues.

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