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A unique stylopod patterning mechanism by Shox2 controlled osteogenesis
Author(s) -
Wenduo Ye,
Yingnan Song,
Zhen Huang,
Marco Osterwalder,
Anja Ljubojevic,
Jue Xu,
Brent E. Bobick,
Samuel AbassahOppong,
Ningsheng Ruan,
Ross Shamby,
Diankun Yu,
Lu Zhang,
Chen-Leng Cai,
Axel Visel,
Yanding Zhang,
John Cobb,
Yiping Chen
Publication year - 2016
Publication title -
development
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.15
H-Index - 36
eISSN - 1477-9129
pISSN - 0950-1991
DOI - 10.1242/dev.138750
Subject(s) - hox gene , biology , enhancer , repressor , genetics , regulator , regulation of gene expression , lineage (genetic) , transcription factor , transcriptional regulation , loss function , microbiology and biotechnology , homeobox , gene , computational biology , phenotype
Vertebrate appendage patterning is programmed by Hox-TALE factor-bound regulatory elements. However, it remains unclear which cell lineages are commissioned by Hox-TALE factors to generate regional specific patterns and whether other Hox-TALE co-factors exist. In this study, we investigated the transcriptional mechanisms controlled by the Shox2 transcriptional regulator in limb patterning. Harnessing an osteogenic lineage-specific Shox2 inactivation approach we show that despite widespread Shox2 expression in multiple cell lineages, lack of the stylopod observed upon Shox2 deficiency is a specific result of Shox2 loss of function in the osteogenic lineage. ChIP-Seq revealed robust interaction of Shox2 with cis-regulatory enhancers clustering around skeletogenic genes that are also bound by Hox-TALE factors, supporting a lineage autonomous function of Shox2 in osteogenic lineage fate determination and skeleton patterning. Pbx ChIP-Seq further allowed the genome-wide identification of cis-regulatory modules exhibiting co-occupancy of Pbx, Meis and Shox2 transcriptional regulators. Integrative analysis of ChIP-Seq and RNA-Seq data and transgenic enhancer assays indicate that Shox2 patterns the stylopod as a repressor via interaction with enhancers active in the proximal limb mesenchyme and antagonizes the repressive function of TALE factors in osteogenesis.

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