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The adipogenic transcriptional cofactor ZNF638 interacts with splicing regulators and influences alternative splicing. | LitMetric

The adipogenic transcriptional cofactor ZNF638 interacts with splicing regulators and influences alternative splicing.

J Lipid Res

Genetics of Development and Disease Branch of the National Institute of Diabetes and Digestive and Kidney Diseases, National Institutes of Health, Bethesda, MD 20892.

Published: September 2014

AI Article Synopsis

  • There is growing evidence that transcription (the process of copying genes into RNA) and alternative splicing (modifying RNA to produce different proteins) are interconnected, but specific factors in adipocyte differentiation (fat cell development) are not well understood.
  • The zinc finger protein ZNF638 has been identified as a key player in this process, helping to regulate adipocyte differentiation by enhancing the activity of PPARγ and working with C/EBP proteins.
  • New findings show that ZNF638 is associated with nuclear bodies that contain splicing factors, indicating that it can influence alternative splicing, particularly of genes important for fat cell function, which ultimately affects how fat cells develop.

Article Abstract

Increasing evidence indicates that transcription and alternative splicing are coordinated processes; however, our knowledge of specific factors implicated in both functions during the process of adipocyte differentiation is limited. We have previously demonstrated that the zinc finger protein ZNF638 plays a role as a transcriptional coregulator of adipocyte differentiation via induction of PPARγ in cooperation with CCAAT/enhancer binding proteins (C/EBPs). Here we provide new evidence that ZNF638 is localized in nuclear bodies enriched with splicing factors, and through biochemical purification of ZNF638's interacting proteins in adipocytes and mass spectrometry analysis, we show that ZNF638 interacts with splicing regulators. Functional analysis of the effects of ectopic ZNF638 expression on a minigene reporter demonstrated that ZNF638 is sufficient to promote alternative splicing, a function enhanced through its recruitment to the minigene promoter at C/EBP responsive elements via C/EBP proteins. Structure-function analysis revealed that the arginine/serine-rich motif and the C-terminal zinc finger domain required for speckle localization are necessary for the adipocyte differentiation function of ZNF638 and for the regulation of the levels of alternatively spliced isoforms of lipin1 and nuclear receptor co-repressor 1. Overall, our data demonstrate that ZNF638 participates in splicing decisions and that it may control adipogenesis through regulation of the relative amounts of differentiation-specific isoforms.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC4617354PMC
http://dx.doi.org/10.1194/jlr.M047555DOI Listing

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