Abstract
AbstractModeling has proposed that the amount of neural tissue folding is set by the level of differential-expansion between tissue layers and that the wavelength is set by the thickness of the outer layer. Here we used inbred mouse strains with distinct amounts of cerebellar folding to investigate these predictions. We identified a critical period where the folding amount diverges between the strains. In this period, regional changes in the level of differential-expansion between the external granule layer (EGL) and underlying core correlate with the folding amount in each strain. Additionally, the thickness of the EGL is regionally adjusted during the critical period alongside corresponding changes in wavelength. While the number of SHH-expressing Purkinje cells predicts the folding amount, the proliferation rate in the EGL is the same between the strains. However, regional changes in the cell division angle within the EGL predicts both the tangential-expansion and thickness of the EGL. Cell division angle is likely a tunable mechanism whereby both the level of differential-expansion and thickness of the EGL are regionally tuned to set the amount and wavelength of folding.
Publisher
Cold Spring Harbor Laboratory
Reference38 articles.
1. Retinal degeneration in the rd mouse is caused by a defect in the β subunit of rod cGMP-phosphodiesterase
2. The level of sonic hedgehog signaling regulates the complexity of cerebellar foliation;Dev. Camb. Engl,2006
3. Buckling without Bending: A New Paradigm in Morphogenesis;Phys. Rev. X,2018
4. [Clinical variability of polymicrogiria: report of 35 new cases and review of the literature];Rev. Neurol,2012
5. Mechanical Instabilities of Biological Tubes;Phys. Rev. Lett,2012