Op-hmgj160187 106..114
نویسندگان
چکیده
High-resolution mass spectrometry (MS)-based proteomics is a powerful method for the identification of soluble protein complexes and large-scale affinity purification screens can decode entire protein interaction networks. In contrast, protein complexes residing on chromatin have been much more challenging, because they are difficult to purify and often of very low abundance. However, this is changing due to recent methodological and technological advances in proteomics. Proteins interacting with chromatin marks can directly be identified by pulldowns with synthesized histone tails containing posttranslational modifications (PTMs). Similarly, pulldowns with DNA baits harbouring single nucleotide polymorphisms or DNA modifications reveal the impact of those DNA alterations on the recruitment of transcription factors. Accurate quantitation – either isotope-based or label free – unambiguously pinpoints proteins that are significantly enriched over control pulldowns. In addition, protocols that combine classical chromatin immunoprecipitation (ChIP) methods with mass spectrometry (ChIP-MS) target gene regulatory complexes in their in-vivo context. Similar to classical ChIP, cells are crosslinked with formaldehyde and chromatin sheared by sonication or nuclease digested. ChIP-MS baits can be proteins in tagged or endogenous form, histone PTMs, or lncRNAs. Locus-specific ChIP-MS methods would allow direct purification of a single genomic locus and the proteins associated with it. There, loci can be targeted either by artificial DNA-binding sites and corresponding binding proteins or via proteins with sequence specificity such as TAL or nuclease deficient Cas9 in combination with a specific guide RNA. We predict that advances in MS technology will soon make such approaches generally applicable tools in epigenetics.
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A polymerase chain reaction-restriction fragment length polymorphism method for screening ZNF804A gene polymorphism (rs1344706) in patients with schizophrenia: a significant association.
The original ZNF804A rs1344706 risk variant was identified through genome-wide association studies as a risk factor for schizophrenia. Follow-up studies involving meta-analysis have confirmed that rs1344706 is a risk factor for schizophrenia as well as bipolar disorders. We describe here a polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) method to genotype ZNF804A r...
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22 Fettke, C. R., op. cit., 231; Koeberlin, F. R., "The Brewster Iron-Bearing District of New York," Econ. Geol., 4, 737 (1909). 23 Fettke, C. R., op. cit., 234. 24 Schuchert, C., and Longwell, C. R., op. cit., 321-324. 26 Schuchert, C., and Longwell, C. R., op. cit., 321. 26 Emerson, B. K., U. S. G. S. Bull., 597, 48-49 (1917); Emerson, B. K., U. S. G. S. Mon., 29, 252-299 (1898). 27 White, D....
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1Department of Information and Computer Education, College of Education, National Taiwan Normal University, Taipei 106, Taiwan 2Department of Information Technology, Takming College, Taipei 114, Taiwan 3Graduate Institute of Networking and Multimedia, College of Electrical Engineering and Computer Science, National Taiwan University, Taipei 106, Taiwan 4Department of Computer Science and Inform...
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1Graduate Institute of Information and Computer Education, College of Education, National Taiwan Normal University, Taipei 106, Taiwan 2Department of Information Technology, Takming College, Taipei 114, Taiwan 3Department of Computer Science and Information Engineering, College of Electrical Engineering and Computer Science, National Taiwan University, Taipei 106, Taiwan 4Graduate Institute of ...
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