MNase-Sensitive Complexes in Yeast: Nucleosomes and Non-histone Barriers

Chereji, Răzvan V.; Ocampo, Josefina; Clark, David

doi:10.1016/j.molcel.2016.12.009

Cited by 124 publications

(183 citation statements)

References 68 publications

Supporting

Mentioning

164

Contrasting

Order By: Relevance

“…While using standard MNase-seq protocols, which have been applied effectively in organisms such as Saccharomyces cerevisiae, we noted variations in measuring nucleosome occupancy from experiment to experiment that confounded interpretation. We attributed this to the fact that nucleosomes are variably released by different MNase concentrations, changes that are likely to be influenced by H1 association, histone variants, and compaction (Iwafuchi-Doi et al 2016;Mieczkowski et al 2016;Chereji et al 2017). We therefore measured nucleosome occupancy on genes that were regulated during the UPR over a range of MNase concentrations.…”

Section: Mnase Titration As a Tool To Determine Occupancy And Accessimentioning

confidence: 99%

“…We therefore measured nucleosome occupancy on genes that were regulated during the UPR over a range of MNase concentrations. We included a histone immunoprecipitation step in the protocol, as nucleosome-sized protection might result from nonhistone proteins as opposed to nucleosomes (Mieczkowski et al 2016;Chereji et al 2017). We found numerous examples of locations where nucleosome occupancy was low or undetectable when high MNase concentration (100 U) was used to release nucleosomes, yet occupancy was high at low MNase concentration (1.5 U) (examples in Fig.…”

Section: Mnase Titration As a Tool To Determine Occupancy And Accessimentioning

confidence: 99%

“…We found previously that increased accessibility to MNase occurs on active genes and therefore were interested in determining how that accessibility changed during an acute response on both active genes and the surrounding regulatory regions. For example, others have shown previously, in disparate organisms, that nucleosomes at gene starts and ends or enhancers can have increased accessibility (Kubik et al 2015;Chereji et al 2016Chereji et al , 2017Iwafuchi-Doi et al 2016). We wished to assess these features during a genome-wide induction.…”

Section: Mnase Titration As a Tool To Determine Occupancy And Accessimentioning

confidence: 99%

“…The use of several MNase concentrations allowed us to capture nucleosomes that are preferentially released at both high and low levels of MNase, providing a more comprehensive occupancy map than is likely to be obtained at a single MNase amount (Iwafuchi-Doi et al 2016;Mieczkowski et al 2016;Chereji et al 2017). These experiments, further supported by experiments performed using ATACseq (assay for transposase-accessible chromatin [ATAC] using sequencing), allowed us to determine whether a nucleosome was accessible or inaccessible in addition to its genomic location.…”

mentioning

confidence: 99%

See 3 more Smart Citations

Widespread changes in nucleosome accessibility without changes in nucleosome occupancy during a rapid transcriptional induction

et al. 2017

View full text Add to dashboard Cite

Activation of transcription requires alteration of chromatin by complexes that increase the accessibility of nucleosomal DNA. Removing nucleosomes from regulatory sequences has been proposed to play a significant role in activation. We tested whether changes in nucleosome occupancy occurred on the set of genes that is activated by the unfolded protein response (UPR). We observed no decrease in occupancy on most promoters, gene bodies, and enhancers. Instead, there was an increase in the accessibility of nucleosomes, as measured by micrococcal nuclease (MNase) digestion and ATAC-seq (assay for transposase-accessible chromatin [ATAC] using sequencing), that did not result from removal of the nucleosome. Thus, changes in nucleosome accessibility predominate over changes in nucleosome occupancy during rapid transcriptional induction during the UPR.

show abstract

Section: Mnase Titration As a Tool To Determine Occupancy And Accessimentioning

confidence: 99%

Section: Mnase Titration As a Tool To Determine Occupancy And Accessimentioning

confidence: 99%

Section: Mnase Titration As a Tool To Determine Occupancy And Accessimentioning

confidence: 99%

mentioning

confidence: 99%

See 2 more Smart Citations

Widespread changes in nucleosome accessibility without changes in nucleosome occupancy during a rapid transcriptional induction

et al. 2017

View full text Add to dashboard Cite

show abstract

“…peaks in low-salt fractions may have resulted from disruption of chromatin at the boundaries of CENP-A/B/C due to the action of MNase used in N-ChIP experiments. MNase not only digests away linker DNA but also "nibbles" on free DNA ends and cleaves to a variable extent within nucleosomes (Xi et al 2011;Mieczkowski et al 2016;Chereji et al 2017). MNase also digests RNA, and this might have contributed to the loss of CCAN components by loss of α-satellite RNAs, which are required in cis for full occupancy of CENP-A and CENP-C (McNulty et al 2017).…”

Section: Solubility Of Cenp-a/b/c Reflects Particle Sizementioning

confidence: 99%

Unexpected conformational variations of the human centromeric chromatin complex

Thakur

Henikoff

2018

Genes Dev.

View full text Add to dashboard Cite

We combined classical salt fractionation with chromatin immunoprecipitation to recover human centromeric chromatin under native conditions. We found that >85% of the total centromeric chromatin is insoluble under conditions typically used for native chromatin extraction. To map both soluble and insoluble chromatin in situ, we combined CUT&RUN (cleavage under targets and release using nuclease), a targeted nuclease method, with salt fractionation. Using this approach, we observed unexpected structural and conformational variations of centromere protein A (CENP-A)-containing complexes on different α-satellite dimeric units within highly homogenous arrays. Our results suggest that slight α-satellite sequence differences control the structure and occupancy of the associated centromeric chromatin complex.

show abstract

Establishing nucleosome architecture and stability at promoters: Roles of pioneer transcription factors and the RSC chromatin remodeler

2017

View full text Add to dashboard Cite

Improvements in deep sequencing, together with methods to rapidly deplete essential transcription factors (TFs) and chromatin remodelers, have recently led to a more detailed picture of promoter nucleosome architecture in yeast and its relationship to transcriptional regulation. These studies revealed that ∼40% of all budding yeast protein-coding genes possess a unique promoter structure, where we propose that an unusually unstable nucleosome forms immediately upstream of the transcription start site (TSS). This "fragile" nucleosome (FN) promoter architecture relies on the combined action of the essential RSC (Remodels Structure of Chromatin) nucleosome remodeler and pioneer transcription factors (PTFs). FNs are associated with genes whose expression is high, coupled to cell growth, and characterized by low cell-to-cell variability (noise), suggesting that they may promote these features. Recent studies in metazoans suggest that the presence of dynamic nucleosomes upstream of the TSS at highly expressed genes may be conserved throughout evolution.

show abstract

MNase-Sensitive Complexes in Yeast: Nucleosomes and Non-histone Barriers

Cited by 124 publications

References 68 publications

Widespread changes in nucleosome accessibility without changes in nucleosome occupancy during a rapid transcriptional induction

Widespread changes in nucleosome accessibility without changes in nucleosome occupancy during a rapid transcriptional induction

Unexpected conformational variations of the human centromeric chromatin complex

Establishing nucleosome architecture and stability at promoters: Roles of pioneer transcription factors and the RSC chromatin remodeler

Contact Info

Product

Resources

About