Heterochromatin is implicated in the regulation of diverse biological processes including recombination, chromosome segregation, transposon repression, and gene expression. As such, mutations in heterochromatin associated proteins are recurrently found in a variety of diseases, including Huntington's disease and numerous cancers. However, the role of these mutations in the progression of disease is poorly understood. A deeper understanding of heterochromatin regulation and the consequences of altered heterochromatin environments will be essential for understanding potential connections to disease. One potential mechanism of heterochromatin regulation is post-translational modification (PTM) of histones, including methylation of lysine nine on histone H3 (H3K9me). Several labs have attempted to study the role of H3K9me by mutating the enzymes that establish this modification. However, conclusions from their studies are limited because these enzymes have several non-histone substrates in addition to H3K9. Unfortunately, directly testing the role of H3K9 by mutating this residue to a non-modifiable amino acid has been unfeasible in higher eukaryotes due to the difficulty of engineering replacement histone genes. For this reason, although modification of H3K9 has been considered an important regulator of heterochromatin for more than a decade, the function of H3K9 in animals has never been directly tested. By using a Drosophila histone replacement platform recently established by our lab and collaborators, we will analyze the contribution of H3K9 to heterochromatin regulation by replacing endogenous histones with H3K9 mutant histones.
The first aim of this study seeks to determine if mutating H3K9 results in altered heterochromatin structure by assessing recruitment of heterochromatin associated proteins and chromatin compaction. Given the ability of H3K9me to recruit heterochromatin factors we expect some genomic locations to lose heterochromatic proteins and consequently form a more open chromatin environment. We will test this idea by examining localization of Heterochromatin Protein 1 and heterochromatin associated histone PTMs via ChIP-seq and polytene chromosome cytology. Moreover, we will genetically assess heterochromatin formation using Position-Effect Variegation assays and explore genome-wide open chromatin profiles using FAIRE-seq to interrogate chromatin structure in H3K9 mutants.
The second aim of this proposal will address the functional importance of H3K9 for two heterochromatin regulated processes, transposon repression and chromosome segregation. We hypothesize that a compromised heterochromatic environment will lead to de-repression of transposable elements and defects in chromosome segregation. We will test these hypotheses by performing quantitative PCR to analyze transposon expression and confocal microscopy to investigate chromosome segregation. Ultimately, we expect analysis of H3K9's role in regulating heterochromatin to augment our understanding of how altered chromatin structure may lead to disease.

Public Health Relevance

Mutations in heterochromatin associated proteins are correlated with several types of diseases including a variety of cancers; however, we do not understand if these mutations are responsible for the progression of disease. Further investigation of the mechanisms that control heterochromatin formation is necessary to understand how breakdowns in this process may lead to disease. We aim to determine if post-translational modification of lysine nine on histone three influences heterochromatin formation and ultimately how deficiencies in this process may be corrected with novel anticancer therapeutics.

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Predoctoral Individual National Research Service Award (F31)
Project #
1F31GM115194-01A1
Application #
8981245
Study Section
Special Emphasis Panel (ZRG1)
Program Officer
Sledjeski, Darren D
Project Start
2015-07-01
Project End
2018-06-30
Budget Start
2015-07-01
Budget End
2016-06-30
Support Year
1
Fiscal Year
2015
Total Cost
Indirect Cost
Name
University of North Carolina Chapel Hill
Department
Genetics
Type
Schools of Medicine
DUNS #
608195277
City
Chapel Hill
State
NC
Country
United States
Zip Code
27599
Armstrong, Robin L; Penke, Taylor J R; Strahl, Brian D et al. (2018) Chromatin conformation and transcriptional activity are permissive regulators of DNA replication initiation in Drosophila. Genome Res 28:1688-1700
Penke, Taylor J R; McKay, Daniel J; Strahl, Brian D et al. (2018) Functional Redundancy of Variant and Canonical Histone H3 Lysine 9 Modification in Drosophila. Genetics 208:229-244
Penke, Taylor J R; McKay, Daniel J; Strahl, Brian D et al. (2016) Direct interrogation of the role of H3K9 in metazoan heterochromatin function. Genes Dev 30:1866-80