Regulation of gene expression during development and stress response requires the concerted action of transcription factors and chromatin-binding proteins. Because this process is cell-type specific and varies with cellular conditions, mapping of chromatin factors at individual regulatory loci is crucial for understanding cis-regulatory control. Previous methods only characterize static protein binding. We present "TurboCas," a method combining a proximity-labeling (PL) enzyme, miniTurbo, with CRISPR-dCas9 that allows for efficient and site-specific labeling of chromatin factors in mammalian cells. Validating TurboCas at the FOS promoter, we identify proteins recruited upon heat shock, cross-validated via RNA polymerase II and P-TEFb immunoprecipitation. These methodologies reveal canonical and uncharacterized factors that function to activate expression of heat-shock-responsive genes. Applying TurboCas to the MYC promoter, we identify two P-TEFb coactivators, the super elongation complex (SEC) and BRD4, as MYC co-regulators. TurboCas provides a genome-specific targeting PL, with the potential to deepen our molecular understanding of transcriptional regulatory pathways in development and stress response.
TurboCas: A method for locus-specific labeling of genomic regions and isolating their associated protein interactome.
TurboCas:一种对基因组区域进行位点特异性标记并分离其相关蛋白质相互作用组的方法
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作者:Cenik Bercin K, Aoi Yuki, Iwanaszko Marta, Howard Benjamin C, Morgan Marc A, Andersen Grant D, Bartom Elizabeth T, Shilatifard Ali
| 期刊: | Molecular Cell | 影响因子: | 16.600 |
| 时间: | 2024 | 起止号: | 2024 Dec 19; 84(24):4929-4944 |
| doi: | 10.1016/j.molcel.2024.11.007 | 研究方向: | 其它 |
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