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In vivo cell biological screening identifies an endocytic capture mechanism for T-tubule formation

Thomas E. Hall, Nick Martel, Nicholas Ariotti, Zherui Xiong, Harriet P. Lo, Charles Ferguson, James Rae, Ye‐Wheen Lim, Robert G. Parton

2020Nature Communications53 citationsDOIOpen Access PDF

Abstract

The skeletal muscle T-tubule is a specialized membrane domain essential for coordinated muscle contraction. However, in the absence of genetically tractable systems the mechanisms involved in T-tubule formation are unknown. Here, we use the optically transparent and genetically tractable zebrafish system to probe T-tubule development in vivo. By combining live imaging of transgenic markers with three-dimensional electron microscopy, we derive a four-dimensional quantitative model for T-tubule formation. To elucidate the mechanisms involved in T-tubule formation in vivo, we develop a quantitative screen for proteins that associate with and modulate early T-tubule formation, including an overexpression screen of the entire zebrafish Rab protein family. We propose an endocytic capture model involving firstly, formation of dynamic endocytic tubules at transient nucleation sites on the sarcolemma, secondly, stabilization by myofibrils/sarcoplasmic reticulum and finally, delivery of membrane from the recycling endosome and Golgi complex.

Topics & Concepts

Cell biologyEndocytic cycleTubuleZebrafishChemistryEndoplasmic reticulumBiologyBiophysicsCellEndocytosisBiochemistryKidneyGeneEndocrinologyCellular transport and secretionCardiomyopathy and Myosin StudiesAdvanced Fluorescence Microscopy Techniques
In vivo cell biological screening identifies an endocytic capture mechanism for T-tubule formation | Litcius