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Ewing sarcoma gene EWS is essential for meiosis and B lymphocyte development
Hongjie Li, … , John O’Shea, Sean Bong Lee
Hongjie Li, … , John O’Shea, Sean Bong Lee
Published May 1, 2007
Citation Information: J Clin Invest. 2007;117(5):1314-1323. https://doi.org/10.1172/JCI31222.
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Research Article Development

Ewing sarcoma gene EWS is essential for meiosis and B lymphocyte development

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Abstract

Ewing sarcoma gene EWS encodes a putative RNA-binding protein with proposed roles in transcription and splicing, but its physiological role in vivo remains undefined. Here, we have generated Ews-deficient mice and demonstrated that EWS is required for the completion of B cell development and meiosis. Analysis of Ews–/– lymphocytes revealed a cell-autonomous defect in precursor B lymphocyte (pre–B lymphocyte) development. During meiosis, Ews-null spermatocytes were deficient in XY bivalent formation and showed reduced meiotic recombination, resulting in massive apoptosis and complete arrest in gamete maturation. Inactivation of Ews in mouse embryonic fibroblasts resulted in premature cellular senescence, and the mutant animals showed hypersensitivity to ionizing radiation. Finally, we showed that EWS interacts with lamin A/C and that loss of EWS results in a reduced lamin A/C expression. Our findings reveal essential functions for EWS in pre–B cell development and meiosis, with proposed roles in DNA pairing and recombination/repair mechanisms. Furthermore, we demonstrate a novel role of EWS in cellular senescence, possibly through its interaction and modulation of lamin A/C.

Authors

Hongjie Li, Wendy Watford, Cuiling Li, Alissa Parmelee, Mark A. Bryant, Chuxia Deng, John O’Shea, Sean Bong Lee

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Figure 1

Inactivation of Ews by gene targeting.

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Inactivation of Ews by gene targeting.
               
(A) Scheme for Ew...
(A) Scheme for Ews targeting strategy. The triangles indicate loxP sequences flanking the stop cassette. WT1, WT1 cDNA; PA, poly(A) sequence. The probe used for Southern blot analysis is indicated. (B) Southern blot analysis of AseI-digested tail DNA. Wild-type (9.4-kb) and targeted (6.9-kb) alleles are marked. (C) Western blot analysis of EWS and TLS using whole-cell extracts isolated from MEFs. Ews genotype and the molecular weight markers (kDa) are indicated.

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