A physical basis for quantitative ChIP-sequencing

Dickson, Bradley M.; Tiedemann, Rochelle L.; Chomiak, Alison A.; Cornett, Evan M.; Vaughan, Robert M.; Rothbart, Scott B.

doi:10.1074/jbc.ra120.015353

Cited by 15 publications

(35 citation statements)

References 27 publications

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“…In our samples, we used exogenous Drosophila (Orlando et al 2014) and synthetic nucleosome (EpiCypher) spike-ins (Supplemental Table S3). However, because of discrepancies (space limitations prevent us from discussing them here, but some of the problems are outlined in Dickson et al 2020), we eventually opted for mass spectrometry normalization. In our experience, we found this method to perform most reliably, but more research on optimizing quantitative normalization is necessary, particularly to distinguish small changes in the levels of epigenetic modifications.…”

Section: H3k36me2 Shapes Early Chromatin Landscapementioning

confidence: 99%

H3K36 dimethylation shapes the epigenetic interaction landscape by directing repressive chromatin modifications in embryonic stem cells

Chen

Horth

et al. 2022

Genome Res.

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Epigenetic modifications on the chromatin do not occur in isolation. Chromatin associated proteins and their modification products form a highly interconnected network, and disturbing one component may rearrange the entire system. We see this increasingly clearly in epigenetically dysregulated cancers. It is important to understand the rules governing epigenetic interactions. Here, we use the mouse embryonic stem cell (mESC) model to describe in detail the relationships within the H3K27-H3K36-DNA methylation subnetwork. In particular, we focus on the major epigenetic reorganization caused by deletion of the histone 3 lysine 36 methyltransferase NSD1, which in mESCs deposits nearly all of the intergenic H3K36me2. Although disturbing the H3K27 and DNA methylation (DNAme) components also affects this network to a certain extent, the removal of H3K36me2 has the most drastic effect on the epigenetic landscape, resulting in full intergenic spread of H3K27me3 and a substantial decrease in DNAme. By profiling DNMT3A and CHH methylation (mCHH), we show that H3K36me2 loss upon Nsd1-KO leads to a massive redistribution of DNMT3A and mCHH away from intergenic regions and towards active gene bodies, suggesting that DNAme reduction is at least in part caused by redistribution of de novo methylation. Additionally, we show that pervasive acetylation of H3K27 is regulated by the interplay of H3K36 and H3K27 methylation. Our analysis highlights the importance of H3K36me2 as a major determinant of the developmental epigenome and provides a framework for further consolidating our knowledge of epigenetic networks.

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Section: H3k36me2 Shapes Early Chromatin Landscapementioning

confidence: 99%

H3K36 dimethylation shapes the epigenetic interaction landscape by directing repressive chromatin modifications in embryonic stem cells

Chen

Horth

et al. 2022

Genome Res.

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“…In our previous work[11], we built the inherent ChIPseq quantitative scale by first noting that the total number of reads available in a given IP can be written as where is the total depth of the IP and R is the total possible depth if the full IP mass were sequenced. ℱ L substituted into α to produce is the fraction of library sequenced, ρ is the total library concentration divided by the theoretical library concentration (what we call the library efficiency ), and ℱ is the fraction of IP’d material taken into library prep.…”

Section: Resultsmentioning

confidence: 99%

“…[17] Meanwhile, under the same treatment and IP conditions, A485 produced a 6.1-fold reduction in H3K18ac IP mass and a 4.9-fold reduction in H3K27ac IP mass. We carried the 1.6 and 2.5 µ g antibody points into sequencing, because this is where we would predict the highest antibody specificity [11].…”

Section: Resultsmentioning

confidence: 99%

“…The formal model of the IP binding process at the heart of siQ-ChIP explicitly expands chromatin into a list of all possible chromatin modification states[11], where we call each state a species. Below we explore the possibility that genomic annotations may provide a means of grouping several distinct species into larger classes.…”

Section: Resultsmentioning

confidence: 99%

“…Along with siQ-ChIP, we previously introduced the fractional composition of the IP as a way to present the distribution of IP products, and we studied this distribution through simulations to show that it can behave in some counterintuitive ways. [11] The fractional composition is identical to the distribution of fragments over the annotations, . The use of annotations as a proxy for species allows us to examine the fractional composition of actual IPs, and to visualize how the distribution of IP products responded to different p300/CBP inhibition paradigms.…”

Section: Resultsmentioning

confidence: 99%

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Theoretical and practical refinements of sans spike-in quantitative ChIP-seq with application to p300/CBP inhibition

Dickson

Kupai

Vaughan

et al. 2022

Preprint

Self Cite

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Previously, we introduced an absolute and physical quantitative scale for chromatin immunoprecipitation followed by sequencing. The scale itself was detemined directly from measurements routinely made on sequencing samples without additional reagents or spike-ins. We called this approach sans spike-in quantitative ChIP, or siQ-ChIP. In this paper we extend those results in several ways. First, we simplified the calculations defining the quantitative scale. Second, we highlight the normalization constraint implied by the quantitative scale and introduce a new scheme for generating 'tracks' for siQ-ChIP. We next introduce some whole-genome analyses that are unique to siQ-ChIP which allow us, for example, to project the IP mass onto the genome to evaluate how much of any genomic interval was captured in the IP. We apply these analyses to p300/CBP inhibition and demonstrate that response to inhibition is a function of genomic architecture. In particular, active transcription start sites are only weakly perturbed by p300/CBP inhibition while enhancers are strongly perturbed. Similar observations have been reported in the literature, but without a quantitative scale, those observations have been misinterpreted. We discuss how the siQ-ChIP approach precludes such misinterpretations, which stem from the widespread community practice of treating unquantified and unnormalized ChIP-seq tracks as though they are quantitative.

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Ketolysis drives CD8+ T cell effector function through effects on histone acetylation

Luda,

Longo,

Kitchen-Goosen

et al. 2023

Immunity

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A physical basis for quantitative ChIP-sequencing

Cited by 15 publications

References 27 publications

H3K36 dimethylation shapes the epigenetic interaction landscape by directing repressive chromatin modifications in embryonic stem cells

H3K36 dimethylation shapes the epigenetic interaction landscape by directing repressive chromatin modifications in embryonic stem cells

Theoretical and practical refinements of sans spike-in quantitative ChIP-seq with application to p300/CBP inhibition

Ketolysis drives CD8+ T cell effector function through effects on histone acetylation

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