Tracking the Cartoon mouse phenotype: Hemopexin domain– dependent regulation of MT1-MMP pericellular collagenolytic activity

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Abstract

Following ENU mutagenesis, a phenodeviant line was generated, termed the “Cartoon mouse,” that exhibits profound defects in growth and development. Cartoon mice harbor a single S466P point mutation in the MT1-MMP hemopexin domain, a 200-amino acid segment that is thought to play a critical role in regulating MT1-MMP collagenolytic activity. Herein, we demonstrate that the MT1-MMPS466P mutation replicates the phenotypic status of Mt1-mmp–null animals as well as the functional characteristics of MT1-MMP/ cells. However, rather than a loss-of-function mutation acquired as a consequence of defects in MT1-MMP proteolytic activity, the S466P substitution generates a misfolded, temperature-sensitive mutant that is abnormally retained in the endoplasmic reticulum (ER). By contrast, the WT hemopexin domain does not play a required role in regulating MT1-MMP trafficking, as a hemopexin domain-deletion mutant is successfully mobilized to the cell surface and displays nearly normal collagenolytic activity. Alternatively, when MT1-MMPS466P– expressing cells are cultured at a permissive temperature of 25 °C that depresses misfolding, the mutant successfully traffics from the ER to the trans-Golgi network (ER 3 trans-Golgi network), where it undergoes processing to its mature form, mobilizes to the cell surface, and expresses type I collagenolytic activity. Together, these analyses define the Cartoon mouse as an unexpected gain-of-abnormal function mutation, wherein the temperature-sensitive mutant phenocopies MT1-MMP/ mice as a consequence of eliciting a specific ER 3 trans-Golgi network trafficking defect.

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APA

Sakr, M., Li, X. Y., Sabeh, F., Feinberg, T. Y., Tesmer, J. J. G., Tang, Y., & Weiss, S. J. (2018). Tracking the Cartoon mouse phenotype: Hemopexin domain– dependent regulation of MT1-MMP pericellular collagenolytic activity. Journal of Biological Chemistry, 293(21), 8113–8127. https://doi.org/10.1074/jbc.RA117.001503

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