Sources of artifact in measurements of 6mA and 4mC abundance in eukaryotic genomic DNA

O’Brown, Zach Klapholz; Boulias, Konstantinos; Wang, Jie; Wang, Simon Yuan; O'Brown, Natasha M; Hao, Ziyang; Shibuya, Hiroki; Fady, Paul-Enguerrand; Shi, Yang; He, Chuan; Megason, Sean G.; Liu, Tao; Greer, Eric Lieberman

doi:10.1186/s12864-019-5754-6

Cited by 130 publications

(154 citation statements)

References 54 publications

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“…The consistent and highly unusual pattern of mCpGs/CpGs flanking reported 6mdA sites strongly suggests that much of the reported 6mdA signal in mammals is an artifact. The tendency of SMRT-seq to overestimate 6mdA content was further demonstrated in a recent study comparing MS-based and SMRT-seq-based estimates of 6mdA in the DNA of 15 prokaryotic and eukaryotic genomes (18). Although SMRT-seq and DIP-seq are routinely used to cross-validate one another, closer inspection reveals very little overlap (1 to 8%) between these tech-niques when applied to mammalian DNA (Fig.…”

Section: Artifactual Detection Of 6mda In Mammalian Dna By Single-molmentioning

confidence: 76%

“…Specificity to guanine could not be tested as even short [4 base pairs (bp)] poly-guanine sequences form strong secondary structures (guanine tetraplexes), precluding synthesis of poly-guanine oligonucleotides. Given the vanishingly low levels of 6mdA reported in mammalian DNA (4,18), even a very low affinity for the far more abundant dA would result in detectable signal when using 6mdA antibodies. Given the affinity of 6mdA antibodies for unmethylated DNA, the frequent contamination of cultured mammalian cells with 6mdA-rich bacteria and lack of appropriate controls, the results of immunodot blot determination of 6mdA abundance in mammals is rendered invalid.…”

Section: Artifactual Detection Of 6mda By Anti-6mda Antibodiesmentioning

confidence: 99%

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No evidence for DNA N ⁶ -methyladenine in mammals

et al. 2020

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N 6 -methyladenine (6mdA) is a widespread DNA modification in bacteria. More recently, 6mdA has also been characterized in mammalian DNA. However, measurements of 6mdA abundance and profiles are often very dissimilar between studies, even when performed on DNA from identical mammalian cell types. Using comprehensive bioinformatics analyses of published data and novel experimental approaches, we reveal that efforts to assay 6mdA in mammals have been severely compromised by bacterial contamination, RNA contamination, technological limitations, and antibody nonspecificity. These complications render 6mdA an exceptionally problematic DNA modification to study and have resulted in erroneous detection of 6mdA in several mammalian systems. Together, our results strongly imply that the evidence published to date is not sufficient to support the presence of 6mdA in mammals.

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Section: Artifactual Detection Of 6mda In Mammalian Dna By Single-molmentioning

confidence: 76%

Section: Artifactual Detection Of 6mda By Anti-6mda Antibodiesmentioning

confidence: 99%

No evidence for DNA N ⁶ -methyladenine in mammals

et al. 2020

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“…Genome-wide distribution of 6mA varies between species (27–30, 51). An evolutionary conservation for 6mA in unicellular organisms has been proposed due to the similarities in 6mA distribution pattern and function between green algae and Tetrahymena (48).…”

Section: Discussionmentioning

confidence: 99%

“…6mA abundance was quantified as previously described (28, 51). 1.5 µg of genomic DNA in 30 ml ddH2O was digested to free nucleosides using 5 U of DNA Degradase Plus (Zymo Research) in 25 μl reactions incubated for 2 hours at 37°C.…”

Section: Methodsmentioning

confidence: 99%

Adenine DNA methylation, 3D genome organization and gene expression in the parasiteTrichomonas vaginalis

Lizarraga

O’Brown

Roach

et al. 2019

Preprint

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Trichomonas vaginalis is a common sexually transmitted parasite that colonizes the human urogenital tract causing infections that range from asymptomatic to highly inflammatory. Recent works have highlighted the importance of histone modifications in the regulation of transcription and parasite pathogenesis. However, the nature of DNA methylation in the parasite remains unexplored. Using a combination of immunological techniques and UHPLC, we analyzed the abundance of DNA methylation in strains with differential pathogenicity demonstrating that N6-methyladenine (6mA), and not 5-methylcytosine (5mC), is the main DNA methylation mark in T. vaginalis. Genome-wide distribution of 6mA reveals that this mark is enriched at intergenic regions, with a preference for certain super-families of DNA transposable elements. We show that 6mA in T. vaginalis is associated with silencing when present on genes. Interestingly, bioinformatics analysis revealed the presence of transcriptionally active or repressive intervals flanked by 6mA-enriched regions and results from chromatin conformation capture (3C) experiments suggest these 6mA flanked regions are in close spatial proximity. These associations were disrupted when parasites were treated with the demethylation activator ascorbic acid. This finding revealed a new role for 6mA in modulating 3D chromatin structure and gene expression in this divergent member of the Excavata.SIGNIFICANCE STATEMENTTrichomonas vaginalis causes the most common non-viral sexually transmitted infection yet little is known about the regulation of gene expression in this eukaryotic parasite. We demonstrate that N6-methyladenine (6mA) is the main methylation mark in the T. vaginalis genome. 6mA is widespread in DNA of eubacterial genera, but uncommon in genomes of most eukaryotes. Examination of the genome-wide distribution of 6mA reveals a preference for intergenic regions. Transcriptionally active or repressive intervals are found to be flanked by 6mA-enriched regions and data suggest 6mA flanked regions are in close 3D spatial proximity. Our findings describe for the first time the presence of DNA methylation in T. vaginalis and reveal a new role for 6mA in modulating 3D chromatin architecture.

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“…Minimum 25X and 250X coverage are recommended for the detection of m6A and m5C [46]. Although 6 mA in DNA is responsible for biological functions in bacteria, its function is unclear and it is very rare in metazoan [47]. It is suggested that SMRT sequencing overestimates 6 mA in DNA in which m6A is rare.…”

Section: Smrt (Single Molecule Real-time) Sequencingmentioning

confidence: 99%

Recent advances in the detection of base modifications using the Nanopore sequencer

Seki

2019

J Hum Genet

107

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DNA and RNA modifications have important functions, including the regulation of gene expression. Existing methods based on short-read sequencing for the detection of modifications show difficulty in determining the modification patterns of single chromosomes or an entire transcript sequence. Furthermore, the kinds of modifications for which detection methods are available are very limited. The Nanopore sequencer is a single-molecule, long-read sequencer that can directly sequence RNA as well as DNA. Moreover, the Nanopore sequencer detects modifications on long DNA and RNA molecules. In this review, we mainly focus on base modification detection in the DNA and RNA of mammals using the Nanopore sequencer. We summarize current studies of modifications using the Nanopore sequencer, detection tools using statistical tests or machine learning, and applications of this technology, such as analyses of open chromatin, DNA replication, and RNA metabolism.

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Sources of artifact in measurements of 6mA and 4mC abundance in eukaryotic genomic DNA

Cited by 130 publications

References 54 publications

No evidence for DNA N ⁶ -methyladenine in mammals

No evidence for DNA N ⁶ -methyladenine in mammals

Adenine DNA methylation, 3D genome organization and gene expression in the parasiteTrichomonas vaginalis

Recent advances in the detection of base modifications using the Nanopore sequencer

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Sources of artifact in measurements of 6mA and 4mC abundance in eukaryotic genomic DNA

Cited by 130 publications

References 54 publications

No evidence for DNA N 6 -methyladenine in mammals

No evidence for DNA N 6 -methyladenine in mammals

Adenine DNA methylation, 3D genome organization and gene expression in the parasiteTrichomonas vaginalis

Recent advances in the detection of base modifications using the Nanopore sequencer

Contact Info

Product

Resources

About

No evidence for DNA N ⁶ -methyladenine in mammals

No evidence for DNA N ⁶ -methyladenine in mammals