Ukaegbu Uchechi E, Kishore Sandeep P, Kwiatkowski Dacia L, Pandarinath Chethan, Dahan-Pasternak Noa, Dzikowski Ron, Deitsch Kirk W
Department of Microbiology and Immunology, Weill Medical College of Cornell University, New York, New York, United States of America.
Program in Computational Biology, Weill Medical College of Cornell University, New York, New York, United States of America.
PLoS Pathog. 2014 Jan;10(1):e1003854. doi: 10.1371/journal.ppat.1003854. Epub 2014 Jan 2.
Histone modifications are important regulators of gene expression in all eukaryotes. In Plasmodium falciparum, these epigenetic marks regulate expression of genes involved in several aspects of host-parasite interactions, including antigenic variation. While the identities and genomic positions of many histone modifications have now been cataloged, how they are targeted to defined genomic regions remains poorly understood. For example, how variant antigen encoding loci (var) are targeted for deposition of unique histone marks is a mystery that continues to perplex the field. Here we describe the recruitment of an ortholog of the histone modifier SET2 to var genes through direct interactions with the C-terminal domain (CTD) of RNA polymerase II. In higher eukaryotes, SET2 is a histone methyltransferase recruited by RNA pol II during mRNA transcription; however, the ortholog in P. falciparum (PfSET2) has an atypical architecture and its role in regulating transcription is unknown. Here we show that PfSET2 binds to the unphosphorylated form of the CTD, a property inconsistent with its recruitment during mRNA synthesis. Further, we show that H3K36me3, the epigenetic mark deposited by PfSET2, is enriched at both active and silent var gene loci, providing additional evidence that its recruitment is not associated with mRNA production. Over-expression of a dominant negative form of PfSET2 designed to disrupt binding to RNA pol II induced rapid var gene expression switching, confirming both the importance of PfSET2 in var gene regulation and a role for RNA pol II in its recruitment. RNA pol II is known to transcribe non-coding RNAs from both active and silent var genes, providing a possible mechanism by which it could recruit PfSET2 to var loci. This work unifies previous reports of histone modifications, the production of ncRNAs, and the promoter activity of var introns into a mechanism that contributes to antigenic variation by malaria parasites.
组蛋白修饰是所有真核生物中基因表达的重要调节因子。在恶性疟原虫中,这些表观遗传标记调节参与宿主 - 寄生虫相互作用多个方面的基因表达,包括抗原变异。虽然现在已经对许多组蛋白修饰的身份和基因组位置进行了编目,但它们如何靶向特定的基因组区域仍知之甚少。例如,变异抗原编码基因座(var)如何被靶向以沉积独特的组蛋白标记是一个继续困扰该领域的谜团。在这里,我们描述了组蛋白修饰因子SET2的一个直系同源物通过与RNA聚合酶II的C末端结构域(CTD)直接相互作用而被招募到var基因。在高等真核生物中,SET2是一种在mRNA转录过程中由RNA聚合酶II招募的组蛋白甲基转移酶;然而,恶性疟原虫中的直系同源物(PfSET2)具有非典型结构,其在调节转录中的作用尚不清楚。在这里,我们表明PfSET2与CTD的未磷酸化形式结合,这一特性与其在mRNA合成过程中的招募不一致。此外,我们表明PfSET2沉积的表观遗传标记H3K36me3在活跃和沉默的var基因座均富集,提供了额外证据表明其招募与mRNA产生无关。设计用于破坏与RNA聚合酶II结合的PfSET2显性负性形式的过表达诱导了快速的var基因表达转换,证实了PfSET2在var基因调控中的重要性以及RNA聚合酶II在其招募中的作用。已知RNA聚合酶II从活跃和沉默的var基因转录非编码RNA,这提供了一种它可以将PfSET2招募到var基因座的可能机制。这项工作将先前关于组蛋白修饰、非编码RNA的产生以及var内含子的启动子活性的报告统一到一种机制中,该机制有助于疟原虫的抗原变异。
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