Wang Jiachen, Dixon Stacy E, Ting Li-Min, Liu Ting-Kai, Jeffers Victoria, Croken Matthew M, Calloway Myrasol, Cannella Dominique, Hakimi Mohamed Ali, Kim Kami, Sullivan William J
Department of Pharmacology & Toxicology, Indiana University School of Medicine, Indianapolis, Indiana, United States of America.
Department of Medicine, Albert Einstein College of Medicine, Bronx, New York, New York, United States of America ; Department of Microbiology & Immunology, Albert Einstein College of Medicine, Bronx, New York, New York, United States of America.
PLoS Pathog. 2014 Jan;10(1):e1003830. doi: 10.1371/journal.ppat.1003830. Epub 2014 Jan 2.
Histone acetylation has been linked to developmental changes in gene expression and is a validated drug target of apicomplexan parasites, but little is known about the roles of individual histone modifying enzymes and how they are recruited to target genes. The protozoan parasite Toxoplasma gondii (phylum Apicomplexa) is unusual among invertebrates in possessing two GCN5-family lysine acetyltransferases (KATs). While GCN5a is required for gene expression in response to alkaline stress, this KAT is dispensable for parasite proliferation in normal culture conditions. In contrast, GCN5b cannot be disrupted, suggesting it is essential for Toxoplasma viability. To further explore the function of GCN5b, we generated clonal parasites expressing an inducible HA-tagged dominant-negative form of GCN5b containing a point mutation that ablates enzymatic activity (E703G). Stabilization of this dominant-negative GCN5b was mediated through ligand-binding to a destabilization domain (dd) fused to the protein. Induced accumulation of the ddHAGCN5b(E703G) protein led to a rapid arrest in parasite replication. Growth arrest was accompanied by a decrease in histone H3 acetylation at specific lysine residues as well as reduced expression of GCN5b target genes in GCN5b(E703G) parasites, which were identified using chromatin immunoprecipitation coupled with microarray hybridization (ChIP-chip). Proteomics studies revealed that GCN5b interacts with AP2-domain proteins, apicomplexan plant-like transcription factors, as well as a "core complex" that includes the co-activator ADA2-A, TFIID subunits, LEO1 polymerase-associated factor (Paf1) subunit, and RRM proteins. The dominant-negative phenotype of ddHAGCN5b(E703G) parasites, considered with the proteomics and ChIP-chip data, indicate that GCN5b plays a central role in transcriptional and chromatin remodeling complexes. We conclude that GCN5b has a non-redundant and indispensable role in regulating gene expression required during the Toxoplasma lytic cycle.
组蛋白乙酰化与基因表达的发育变化有关,并且是顶复门寄生虫的一个经过验证的药物靶点,但对于单个组蛋白修饰酶的作用以及它们如何被招募到靶基因上,我们所知甚少。原生动物寄生虫刚地弓形虫(顶复门)在无脊椎动物中很不寻常,它拥有两种GCN5家族赖氨酸乙酰转移酶(KATs)。虽然GCN5a是响应碱性应激时基因表达所必需的,但这种KAT在正常培养条件下对寄生虫增殖是可有可无的。相比之下,GCN5b无法被破坏,这表明它对弓形虫的生存能力至关重要。为了进一步探索GCN5b的功能,我们构建了表达可诱导的HA标签显性负性形式GCN5b的克隆寄生虫,该GCN5b含有一个消除酶活性的点突变(E703G)。这种显性负性GCN5b的稳定是通过与融合到该蛋白上的去稳定结构域(dd)的配体结合来介导的。ddHAGCN5b(E703G)蛋白的诱导积累导致寄生虫复制迅速停滞。生长停滞伴随着特定赖氨酸残基处组蛋白H3乙酰化的减少,以及GCN5b(E703G)寄生虫中GCN5b靶基因表达的降低,这些靶基因是通过染色质免疫沉淀结合微阵列杂交(ChIP-chip)鉴定出来的。蛋白质组学研究表明,GCN5b与AP2结构域蛋白、顶复门植物样转录因子以及一个“核心复合物”相互作用,该“核心复合物”包括共激活因子ADA2-A、TFIID亚基、LEO1聚合酶相关因子(Paf1)亚基和RRM蛋白。考虑到蛋白质组学和ChIP-chip数据,ddHAGCN5b(E703G)寄生虫的显性负性表型表明,GCN5b在转录和染色质重塑复合物中起核心作用。我们得出结论,GCN5b在调节弓形虫裂解周期所需的基因表达中具有非冗余且不可或缺的作用。
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