Multivalency regulates activity in an intrinsically disordered transcription factor.
Sarah ClarkJanette B MyersAshleigh KingRadovan FialaJiri NovacekFrederick Grant PearceJörg HeierhorstSteve L ReichowElisar J BarbarPublished in: eLife (2018)
The transcription factor ASCIZ (ATMIN, ZNF822) has an unusually high number of recognition motifs for the product of its main target gene, the hub protein LC8 (DYNLL1). Using a combination of biophysical methods, structural analysis by NMR and electron microscopy, and cellular transcription assays, we developed a model that proposes a concerted role of intrinsic disorder and multiple LC8 binding events in regulating LC8 transcription. We demonstrate that the long intrinsically disordered C-terminal domain of ASCIZ binds LC8 to form a dynamic ensemble of complexes with a gradient of transcriptional activity that is inversely proportional to LC8 occupancy. The preference for low occupancy complexes at saturating LC8 concentrations with both human and Drosophila ASCIZ indicates that negative cooperativity is an important feature of ASCIZ-LC8 interactions. The prevalence of intrinsic disorder and multivalency among transcription factors suggests that formation of heterogeneous, dynamic complexes is a widespread mechanism for tuning transcriptional regulation.
Keyphrases
- transcription factor
- simultaneous determination
- dna binding
- mass spectrometry
- liquid chromatography
- genome wide identification
- endothelial cells
- tandem mass spectrometry
- machine learning
- electron microscopy
- gene expression
- oxidative stress
- binding protein
- dna methylation
- high resolution
- copy number
- genome wide
- deep learning
- small molecule
- convolutional neural network
- gas chromatography