Adjusting for Batch Effects in DNA Methylation Microarray Data, a Lesson Learned

Price, Emily; Robinson, Wendy P.

doi:10.3389/fgene.2018.00083

Cited by 76 publications

(70 citation statements)

References 40 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Additionally, we evaluated CpG sites with significantly lower methylation levels in familial melanoma than in healthy control samples and found 35 hypomethylated CpGs in both members of a family (Supplementary Table 2). Fifteen CpG sites showed hypomethylation in all 5 families, suggestive of a batch effect as has been described for 450k methylation arrays [20]. Of the 35 hypomethylated CpG sites, only 2 were located in established cancer-related genes: BRCA1, an established breast and ovarian cancer susceptibility gene, and ROS1, encoding a receptor tyrosine kinase with a possible oncogenic role in melanoma [21].…”

Section: Resultssupporting

confidence: 51%

Genome-wide analysis of constitutional DNA methylation in familial melanoma

et al. 2020

View full text Add to dashboard Cite

Background: Heritable epigenetic alterations have been proposed as an explanation for familial clustering of melanoma. Here we performed genome-wide DNA methylation analysis on affected family members not carrying pathogenic variants in established melanoma susceptibility genes, compared with healthy volunteers. Results: All melanoma susceptibility genes showed the absence of epimutations in familial melanoma patients, and no loss of imprinting was detected. Unbiased genome-wide DNA methylation analysis revealed significantly different levels of methylation in single CpG sites. The methylation level differences were small and did not affect reported tumour predisposition genes. Conclusion: Our results provide no support for heritable epimutations as a cause of familial melanoma.

show abstract

Section: Resultssupporting

confidence: 51%

Genome-wide analysis of constitutional DNA methylation in familial melanoma

et al. 2020

View full text Add to dashboard Cite

show abstract

“…Raw intensity was read into Illumina Genome Studio software 2011.1, and background normalization was applied. Data processing was performed as described in Price et al [ 73 ], including sample quality checks, probe filtering, data normalization, and batch correction. This processing pipeline resulted in a final N = 442,355 cytosine-guanine dinucleotide (CpG) sites from the 450k array for analysis.…”

Section: Methodsmentioning

confidence: 99%

No evidence for association of MTHFR 677C>T and 1298A>C variants with placental DNA methylation

et al. 2018

Self Cite

View full text Add to dashboard Cite

Background5,10-Methylenetetrahydrofolate reductase (MTHFR) is a key enzyme in one-carbon metabolism that ensures the availability of methyl groups for methylation reactions. Two single-nucleotide polymorphisms (SNPs) in the MTHFR gene, 677C>T and 1298A>C, result in a thermolabile enzyme with reduced function. These variants, in both the maternal and/or fetal genes, have been associated with pregnancy complications including miscarriage, neural tube defects (NTDs), and preeclampsia (PE), perhaps due to altered capacity for DNA methylation (DNAm). In this study, we assessed the association between MTHFR 677TT and 1298CC genotypes and risk of NTDs, PE, or normotensive intrauterine growth restriction (nIUGR). Additionally, we assessed whether these high-risk genotypes are associated with altered DNAm in the placenta.ResultsIn 303 placentas screened for this study, we observed no significant association between the occurrence of NTDs (N = 55), PE (early-onset: N = 28, late-onset: N = 20), or nIUGR (N = 21) and placental (fetal) MTHFR 677TT or 1298CC genotypes compared to healthy pregnancies (N = 179), though a trend of increased 677TT genotype in PE/IUGR together was observed (OR 2.53, p = 0.048). DNAm was profiled in 10 high-risk 677 (677TT + 1298AA), 10 high-risk 1298 (677CC + 1298CC), and 10 reference (677CC + 1298AA) genotype placentas. Linear modeling identified no significantly differentially methylated sites between high-risk 677 or 1298 and reference placentas at a false discovery rate < 0.05 and Δβ ≥ 0.05 using the Illumina Infinium HumanMethylation450 BeadChip. Using a differentially methylated region analysis or separating cytosine-guanine dinucleotides (CpGs) by CpG density to reduce multiple comparisons also did not identify differential methylation. Additionally, there was no consistent evidence for altered methylation of repetitive DNA between high-risk and reference placentas.ConclusionsWe conclude that large-scale, genome-wide disruption in DNAm does not occur in placentas with the high-risk MTHFR 677TT or 1298CC genotypes. Furthermore, there was no evidence for an association of the 1298CC genotype and only a tendency to higher 677TT in pregnancy complications of PE/IUGR. This may be due to small sample sizes or folate repletion in our Canadian population attenuating effects of the high-risk MTHFR variants. However, given our results and the conflicting results in the literature, investigations into alternative mechanisms that may explain the link between MTHFR variants and pregnancy complications, or in populations at risk of folate deficiencies, are warranted.Electronic supplementary materialThe online version of this article (10.1186/s13148-018-0468-1) contains supplementary material, which is available to authorized users.

show abstract

“…It is now considered to be the gold standard method for performing reproductible and accurate measurements as well as for confirming the results from high-throughput platforms [ 108 ]. Finally, another possible source of discrepancy is the batch effect, a common source of technical variation that may then be interpreted as a biologically significant finding [ 109 ]. Pairs of non-lesional and lesional skin samples might not always be processed simultaneously, thus creating a batch effect inflating the number of differently expressed genes.…”

Section: Transcriptome Profiling Analysis For a Better Understandimentioning

confidence: 99%

Transcriptome Profiling Analyses in Psoriasis: A Dynamic Contribution of Keratinocytes to the Pathogenesis

Rioux

Ridha

Simard

et al. 2020

Genes

View full text Add to dashboard Cite

Psoriasis is an immune-mediated inflammatory skin disease with a complex etiology involving environmental and genetic factors. A better insight into related genomic alteration helps design precise therapies leading to better treatment outcome. Gene expression in psoriasis can provide relevant information about the altered expression of mRNA transcripts, thus giving new insights into the disease onset. Techniques for transcriptome analyses, such as microarray and RNA sequencing (RNA-seq), are relevant tools for the discovery of new biomarkers as well as new therapeutic targets. This review summarizes the findings related to the contribution of keratinocytes in the pathogenesis of psoriasis by an in-depth review of studies that have examined psoriatic transcriptomes in the past years. It also provides valuable information on reconstructed 3D psoriatic skin models using cells isolated from psoriatic patients for transcriptomic studies.

show abstract

Adjusting for Batch Effects in DNA Methylation Microarray Data, a Lesson Learned

Cited by 76 publications

References 40 publications

Genome-wide analysis of constitutional DNA methylation in familial melanoma

Genome-wide analysis of constitutional DNA methylation in familial melanoma

No evidence for association of MTHFR 677C>T and 1298A>C variants with placental DNA methylation

Transcriptome Profiling Analyses in Psoriasis: A Dynamic Contribution of Keratinocytes to the Pathogenesis

Contact Info

Product

Resources

About