Antisilencing role of the RNA-directed DNA methylation pathway and a histone acetyltransferase in Arabidopsis

REPRESSOR OF SILENCING 1 (ROS1) is a DNA demethylation enzyme that was previously identified during a genetic screen for the silencing of both RD29A-LUC and 35S-NPTII transgenes on a T-DNA construct. Here we performed a genetic screen to identify additional mutants in which the 35S-NPTII transgene is silenced. We identified several alleles of ros1 and of the following components of the RNA-directed DNA methylation (RdDM) pathway: NRPD1 (the largest subunit of polymerase IV), RDR2, NRPE1 (the largest subunit of polymerase V), NRPD2, AGO4, and DMS3. Our results show that the silencing of 35S-NPTII in the RdDM pathway mutants is due to the reduced expression of ROS1 in the mutants. We also identified a putative histone acetyltransferase (ROS4) from the genetic screen. The acetyltransferase contains a PHD-finger domain that binds to unmethylated histone H3K4. The mutation in ROS4 led to reduction of H3K18 and H3K23 acetylation levels. We show that the silencing of 35S-NPTII and some transposable element genes was released by the ddm1 mutation but that this also required ROS4. Our study identifies a unique antisilencing factor, and reveals that the RdDM pathway has an antisilencing function due to its role in maintaining ROS1 expression.     

PolIVb influences RNA-directed DNA methylation independently of its role in siRNA biogenesis

DNA-dependent RNA polymerase (Pol)IV in Arabidopsis exists in two isoforms (PolIVa and PolIVb), with NRPD1a and NRPD1b as their respective largest subunits. Both isoforms are implicated in production and activity of siRNAs and in RNA-directed DNA methylation (RdDM). Deep sequence analysis of siRNAs in WT Arabidopsis flowers and in nrpd1a and nrpd1b mutants identified >4,200 loci producing siRNAs in a PolIV-dependent manner, with PolIVb reinforcing siRNA production by PolIVa. Transposable element identity and pericentromeric localization are both features that predispose a locus for siRNA production via PolIV proteins and determine the extent to which siRNA production relies on PolIVb. Detailed analysis of DNA methylation at PolIV-dependent loci revealed unexpected deviations from the previously noted association of PolIVb-dependent siRNA production and RdDM. Notably, PolIVb functions independently in DNA methylation and siRNA generation. Additionally, we have uncovered siRNA-directed loss of DNA methylation, a process requiring both PolIV isoforms. From these findings, we infer that the role of PolIVb in siRNA production is secondary to a role in chromatin modification and is influenced by chromatin context.     

胃癌DNA甲基化研究进展

胃癌的发生发展是一个涉及多基因多步骤的复杂过程。随着研究的不断深入,人们开始关注DNA 甲基化这种表遗传学修饰方式在胃癌发生过程中的作用。DNA的异常甲基化通过影响基因转录,促基因突变,增加染色体结构的不稳定性等多方面促进胃癌的发生发展。随着DNA甲基化研究的不断深入,甲基化的检测技术也不断革新。基因启动子甲基化已经作为一种重要的肿瘤生物学标志被应用于胃癌的临床诊断,甲基化制剂作为抗肿瘤药物也逐步应用于临床。     

Features of the Arabidopsis recombination landscape resulting from the combined loss of sequence variation and DNA methylation

The rate of meiotic crossing over (CO) varies considerably along chromosomes, leading to marked distortions between physical and genetic distances. The causes underlying this variation are being unraveled, and DNA sequence and chromatin states have emerged as key factors. However, the extent to which the suppression of COs within the repeat-rich pericentromeric regions of plant and mammalian chromosomes results from their high level of DNA polymorphisms and from their heterochromatic state, notably their dense DNA methylation, remains unknown. Here, we test the combined effect of removing sequence polymorphisms and repeat-associated DNA methylation on the meiotic recombination landscape of an Arabidopsis mapping population. To do so, we use genome-wide DNA methylation data from a large panel of isogenic epigenetic recombinant inbred lines (epiRILs) to derive a recombination map based on 126 meiotically stable, differentially methylated regions covering 81.9% of the genome. We demonstrate that the suppression of COs within pericentromeric regions of chromosomes persists in this experimental setting. Moreover, suppression is reinforced within 3-Mb regions flanking pericentromeric boundaries, and this effect appears to be compensated by increased recombination activity in chromosome arms. A direct comparison with 17 classical Arabidopsis crosses shows that these recombination changes place the epiRILs at the boundary of the range of natural variation but are not severe enough to transgress that boundary significantly. This level of robustness is remarkable, considering that this population represents an extreme with key recombination barriers having been forced to a minimum.     

CG gene body DNA methylation changes and evolution of duplicated genes in cassava

DNA methylation is important for the regulation of gene expression and the silencing of transposons in plants. Here we present genome-wide methylation patterns at single-base pair resolution for cassava (Manihot esculenta, cultivar TME 7), a crop with a substantial impact in the agriculture of subtropical and tropical regions. On average, DNA methylation levels were higher in all three DNA sequence contexts (CG, CHG, and CHH, where H equals A, T, or C) than those of the most well-studied model plant Arabidopsis thaliana. As in other plants, DNA methylation was found both on transposons and in the transcribed regions (bodies) of many genes. Consistent with these patterns, at least one cassava gene copy of all of the known components of Arabidopsis DNA methylation pathways was identified. Methylation of LTR transposons (GYPSY and COPIA) was found to be unusually high compared with other types of transposons, suggesting that the control of the activity of these two types of transposons may be especially important. Analysis of duplicated gene pairs resulting from whole-genome duplication showed that gene body DNA methylation and gene expression levels have coevolved over short evolutionary time scales, reinforcing the positive relationship between gene body methylation and high levels of gene expression. Duplicated genes with the most divergent gene body methylation and expression patterns were found to have distinct biological functions and may have been under natural or human selection for cassava traits.DNA methylation plays an important role in the regulation of the expression of genes and the maintenance of transposable element (TE) silencing. In contrast to animals, in which methylation is often restricted to the CG context, plants exhibit robust methylation in every possible context CG, CHG (H is A, T, or C), and CHH. Previous research has identified different pathways responsible for the maintenance and establishment of DNA methylation patterns. In Arabidopsis thaliana, METHYLTRANSFERASE1 (MET1), a homolog of mammalian Dnmt1, mainly maintains methylation at the CG context, whereas CHROMOMETHYLASE3 (CMT3) mainly maintains CHG methylation. DOMAINS REARRANGED METHYLTRANSFERASE2 (DRM2) and CHROMOMETHYLASE2 (CMT2) maintain CHH methylation in the chromosome arms and pericentromeric regions, respectively (1–3). On the other hand, establishment of DNA methylation is performed by DRM2 through a complex pathway termed RNA-directed DNA methylation (RdDM) (4).To date, the majority of our knowledge about DNA methylation is derived from the model plant Arabidopsis. These studies have allowed the identification of different components involved in different methylation pathways, the genome-wide identification of methylation patterns, and the study of effects of DNA methylation on gene expression. The knowledge acquired from Arabidopsis can now be used as the basis for investigations of methylation in agronomically important plants. However, thus far very few crop species have been subjected to detailed DNA methylation studies (5). Cassava (Manihot esculenta) is cultivated for its starch-rich tuberous roots and is one of the world’s most important staple crops, especially in tropical America, Africa, and Asia (6). Cassava is a source of carbohydrates for nearly a billion people, but it is especially important for a large portion of Africa, where it serves as a subsistence crop because of its ability to tolerate drought and grow on poor soils, conditions unsuitable for rice and maize (6, 7). The genome sequence of cassava has been described recently with an estimated genome size of roughly 760 million base pairs (7). We have used bisulfite sequencing (BS-seq) to examine DNA methylation in cassava at single-base pair resolution. Broadly, the pattern of DNA methylation of both protein-coding genes and TEs is similar to other plants, although DNA methylation levels in cassava are higher than those in Arabidopsis. LTR retrotransposons, such as GYPSY and COPIA, tend to be more heavily methylated than other TEs. Interestingly, differentially expressed gene pairs derived from the last genome duplication tend to show differential gene body methylation, with the highly expressed paralogs displaying significantly higher gene body methylation. We also find that the most differentially gene body-methylated paralogs have distinct biological functions compared with genes that have maintained similar gene body methylation patterns.