Literature DB >> 22491404

Integrin-linked kinase deletion in the developing lens leads to capsule rupture, impaired fiber migration and non-apoptotic epithelial cell death.

Laura Cammas1, Jordan Wolfe, Sue-Yeon Choi, Shoukat Dedhar, Hilary E Beggs.   

Abstract

PURPOSE: The lens is a powerful model system to study integrin-mediated cell-matrix interaction in an in vivo context, as it is surrounded by a true basement membrane, the lens capsule. To characterize better the function of integrin-linked kinase (ILK), we examined the phenotypic consequences of its deletion in the developing mouse lens.
METHODS: ILK was deleted from the embryonic lens either at the time of placode invagination using the Le-Cre line or after initial lens formation using the Nestin-Cre line.
RESULTS: Early deletion of ILK leads to defects in extracellular matrix deposition that result in lens capsule rupture at the lens vesicle stage (E13.5). If ILK was deleted at a later time-point after initial establishment of the lens capsule, rupture was prevented. Instead, ILK deletion resulted in secondary fiber migration defects and, most notably, in cell death of the anterior epithelium (E18.5-P0). Remarkably, dying cells did not stain positively for terminal deoxynucleotidyl transferase dUTP nick end labeling (TUNEL) or activated-caspase 3, suggesting that they were dying from a non-apoptotic mechanism. Moreover, cross to a Bax(fl/fl)/Bak⁻/⁻ mouse line that is resistant to most forms of apoptosis failed to promote cell survival in the ILK-deleted lens epithelium. Electron microscopy revealed the presence of numerous membranous vacuoles containing degrading cellular material. CONCLUSIONS. Our study reveals a role for ILK in extracellular matrix organization, fiber migration, and cell survival. Furthermore, to our knowledge we show for the first time that ILK disruption results in non-apoptotic cell death in vivo.

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Year:  2012        PMID: 22491404      PMCID: PMC3378089          DOI: 10.1167/iovs.11-9128

Source DB:  PubMed          Journal:  Invest Ophthalmol Vis Sci        ISSN: 0146-0404            Impact factor:   4.799


  81 in total

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4.  Deletion of DDB1 in mouse brain and lens leads to p53-dependent elimination of proliferating cells.

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10.  Regulation of fibronectin matrix deposition and cell proliferation by the PINCH-ILK-CH-ILKBP complex.

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2.  Beta-1 integrin is important for the structural maintenance and homeostasis of differentiating fiber cells.

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7.  Crim1 regulates integrin signaling in murine lens development.

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8.  Induction of Immune Surveillance of the Dysmorphogenic Lens.

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9.  Considerations for the use of Cre recombinase for conditional gene deletion in the mouse lens.

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10.  β1-Integrin Deletion From the Lens Activates Cellular Stress Responses Leading to Apoptosis and Fibrosis.

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Journal:  Invest Ophthalmol Vis Sci       Date:  2017-08-01       Impact factor: 4.799

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