Downloaded from genesdev.cshlp.org on September 27, 2021 - Published by Cold Spring Harbor Laboratory Press REVIEW Progress toward understanding chromosome silencing by Xist RNA Neil Brockdorff, Joseph S. Bowness, and Guifeng Wei Department of Biochemistry, University of Oxford, Oxford OX1 3QU, United Kingdom The X inactive-specific transcript (Xist) gene is the master mouse embryos and using mouse embryonic stem cell regulator of X chromosome inactivation in mammals. (mESC) models in vitro defined Xi features that are estab- Xist produces a long noncoding (lnc)RNA that accumu- lished early following the onset of Xist RNA expression, lates over the entire length of the chromosome from interpreted as indicating a role in establishment of X inac- which it is transcribed, recruiting factors to modify under- tivation. Important examples include exclusion of RNA lying chromatin and silence X-linked genes in cis. Recent Polymerase II (RNAPII), loss of histone modifications as- years have seen significant progress in identifying impor- sociated with gene activity, and acquisition of histone tant functional elements in Xist RNA, their associated modifications catalyzed by the Polycomb complexes RNA-binding proteins (RBPs), and the downstream path- PRC1 and PRC2. Conversely, Xi features that are estab- ways for chromatin modification and gene silencing. In lished after a delay following Xist RNA expression, for ex- this review, we summarize progress in understanding ample, CpG island DNA methylation and deposition of both how these pathways function in Xist-mediated si- the histone variant macroH2A, are thought to function lencing and the complex interplay between them. in maintenance rather than establishment of silencing. Significant progress toward defining the critical path- ways for establishment of gene silencing has come from X chromosome inactivation, the process that evolved in the identification of functional sequence elements in mammals to balance levels of X-linked gene expression in Xist RNA and the RNA-binding proteins (RBPs) that XX females relative to XY males, is controlled by a master they bind. Thus, deletion analysis defined the A repeat, regulator locus, Xist (X inactive-specific transcript), that is one of a number of conserved tandem repeat blocks (re- located on the X chromosome and functions in cis (for peated X7.5 in mice and X8 in humans) present in Xist review, see Heard et al. 1997). Xist produces a 15- to 17- RNA sequence (Fig. 2A), as being critical for silencing, kb-long noncoding RNA (lncRNA) that accumulates while multiple regions of the transcript were defined as over the chromosome from which it is transcribed, re- functioning redundantly to mediate local accumulation cruiting factors/complexes that act to modify the underly- of Xist RNA (Wutz et al. 2002). An important break- ing chromatin environment and repress X-linked gene through toward identifying the factors that interact with expression. Gene knockout and transgenic experiments the A repeat (and other regions of Xist RNA), came from demonstrated that Xist is both necessary and sufficient complementary studies that applied either proteomic or for chromosome inactivation (Penny et al. 1996; Lee and genetic screening strategies (Chu et al. 2015; McHugh Jaenisch 1997). et al. 2015; Minajigi et al. 2015; Moindrot et al. 2015; Studies over many years have defined chromatin fea- Monfort et al. 2015). Leading candidates that emerged tures, chromatin-associated factors, and higher-order from this work are summarized in Figure 2A,B. The RBP chromosome organization associated with the inactive SPEN, which functions through interaction with the his- X chromosome (Xi) (Fig. 1; Table 1). An important chal- tone deacetylase complex NCoR-HDAC3 (and possibly lenge for the field is to understand cause and effect. Which other factors), was shown to bind Xist A repeat directly features of Xi are required to establish gene silencing and (Monfort et al. 2015). The closely related RBP RBM15 depend on factors recruited directly by Xist RNA and also binds the A-repeat, and functions at least in part by which are secondary but possibly still important for recruiting the METTL3/14 complex responsible for cata- 6 6 long-term chromosome silencing through development lyzing N -methyladenosine (m A) on mRNA (Patil et al. and into adulthood? To address this issue, studies on early 2016). Additionally, the Lamin B receptor (LBR), was iden- tified as binding Xist RNA (McHugh et al. 2015). Al- though not a known RBP, subsequent work reported [Keywords: X chromosome inactivation; Xist; SPEN; NCoR–HDAC3; LBR; Polycomb; RBM15; m6A RNA methylation; chromatin] Corresponding authors: [email protected], neil.brockdorff@ bioch.ox.ac.uk © 2020 Brockdorff et al. This article, published in Genes & Development, Article is online at http://www.genesdev.org/cgi/doi/10.1101/gad.337196. is available under a Creative Commons License (Attribution-NonCom- 120. Freely available online through the Genes & Development Open Ac- mercial 4.0 International), as described at http://creativecommons.org/li- cess option. censes/by-nc/4.0/. GENES & DEVELOPMENT 34:733–744 Published by Cold Spring Harbor Laboratory Press; ISSN 0890-9369/20; www.genesdev.org 733 Downloaded from genesdev.cshlp.org on September 27, 2021 - Published by Cold Spring Harbor Laboratory Press Brockdorff et al. A Xi chromatin and in gene silencing by Xist RNA, includ- ing a summary of our understanding of their relative con- tribution and interplay. Assaying Xist-mediated chromosome silencing In considering recent advances in this field it is important to appreciate the varied models and assays that have been used in analyzing the contribution of different factors to Xist-mediated chromosome silencing, not least because reported findings may otherwise appear contradictory. As summarized in Figure 3A, the principal models that provide access to the developmental stage when X inacti- vation is established are early mouse embryos and plurip- B otent embryonic stem cells (mESCs). The latter include XX mESCs, which express Xist RNA from a single X chro- mosome when differentiated in vitro, XY mESCs with Xist expression driven by a doxycycline-activated promoter, ei- ther from the single X chromosome allele, or from an auto- somally integrated Xist transgene, and XX mESCs with a doxycycline inducible promoter engineered into one of the two Xist alleles. Models using inducible promoters of- fer the advantage of regulatable, synchronous, and homo- Figure 1. Features of the inactive X chromosome. (A) Compari- geneous Xist RNA expression within cell populations, son of chromatin features on the active X chromosome (Xa) and albeit at levels not necessarily equivalent to expression the inactive X chromosome (Xi) at the nucleosomal scale. Xi is Xist characterized by depletion of histone modifications associated from the physiological promoter. Analysis of X inacti- with gene activity, shown here histone acetylation, normally en- vation in embryos is important to verify observations in a riched at promoters and enhancers, H3K4me3, enriched at pro- physiological context. In addition to the aforementioned moters and H3K36me3, high levels of which occur within the models, some studies have analyzed XX somatic cells in bodies of active genes. Additionally, Xi chromatin has enhanced which X inactivation is already established. However, levels of histone modifications associated with gene repression; maintenance of X inactivation in somatic cells has been re- for example, H3K27me3, H2AK119ub1, H3K9me2/3, and high ported to be Xist-independent (Csankovszki et al. 1999), al- levels of the histone variant macroH2A. DNA methylation is ac- beit using relatively crude gene silencing assays, and as quired at CpG islands of Xi genes. RNA polymerase II (RNAPII) such these models may not be ideally suited to studying and associated general transcription factors (GTFs) are depleted the establishment of Xist-mediated silencing. from Xi, as are enhancer-bound transcription factors (TFs), as ev- idenced by reduced chromatin accessibility seen using ATAC- Assays for Xist-mediated silencing can be grouped into seq. Similarly, there are reduced levels of the insulator protein three categories; indirect phenotype/viability assays, di- CTCF and the cohesin complex at insulator/boundary elements. rect imaging based assays and direct molecular assays, (B) Changes in higher order structure of the Xi chromosome. Key for example, allelic RNA-seq, illustrated in Figure examples are an approximately twofold chromatin compaction 3B. Each of the approaches affords distinct advantages, relative to Xa, association of Xi with the nuclear and/or nucleolar but equally has specific limitations. Phenotypic assays periphery, reduced TAD and compartment structure (related to provide evidence for the importance of a given factor in reduced CTCF/cohesin binding), with interactions instead occur- a physiological setting, but do not quantify the underlying ring within one of two large megadomains, and synchronous rep- deficiency in gene silencing. Imaging-based assays provide lication across most of the chromosome, usually in late S phase. a good basis for measuring silencing in individual cells, within a population, for example, in early embryos, but provide limited quantitation and throughput (the number that LBR has an unstructured SR domain that mediates in- of X-linked genes that is practical to assay). Molecular as- teraction with Xist RNA (Chen et al. 2016). Finally the
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