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Endothelial cell secreted metalloproteinase‐2 enhances neural stem cell N‐cadherin expression, clustering, and migration
Author(s) -
Matta Rita,
Yousafzai Muhammad Sulaiman,
Murrell Michael,
Gonzalez Anjelica L.
Publication year - 2021
Publication title -
the faseb journal
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.709
H-Index - 277
eISSN - 1530-6860
pISSN - 0892-6638
DOI - 10.1096/fj.202002302rr
Subject(s) - metalloproteinase , microbiology and biotechnology , cadherin , endothelial stem cell , chemistry , neural stem cell , cluster analysis , stem cell , cell , ve cadherin , matrix metalloproteinase , biology , biochemistry , computer science , artificial intelligence , in vitro
Abstract Neuroblasts have a clustered phenotype critical for their unidirectional migration, which in part is dependent on signaling from microvascular endothelial cells (EC) and pericytes (PC). Diffusible signals secreted by vascular cells have been demonstrated to increase survival, proliferation, and differentiation of subventricular zone resident neural stem cells (NSC); however, the signals that promote the necessary initiating step of NSC clustering are undefined. To investigate the role of vascular cells in promoting NSC clustering and directing migration, we created a 3‐D hydrogel that mimics the biomechanics, biochemistry, and architectural complexity of brain tissue. We demonstrate that EC, and not PC, have a crucial role in NSC clustering and migration, further verified through microfluidic chamber systems and traction force microscopy. Ablation of the extended NSC aggregate arm halts aggregate movement, suggesting that clustering is a prerequisite for migration. When cultured with EC, NSC clustering occurs and NSC coincidentally increase their expression of N‐cadherin, as compared to NSC cultured alone. NSC‐presented N‐cadherin expression was increased following exposure to EC secreted metalloproteinase‐2 (MMP2). We demonstrate that inhibition of MMP2 prevented NSC N‐cadherin surface expression and subsequent NSC clustering, even when NSC were in direct contact with EC. Furthermore, with exogenous activation of EGFR, which serves as a downstream activator of N‐cadherin cleavage, NSC form clusters. Our results suggest that EC secretion of MMP2 promotes NSC clustering through N‐cadherin expression. The insight gained about the mechanisms by which EC promote NSC migration may enhance NSC therapeutic response to sites of injury.