Bisulfite sequencing remains the gold standard method for the detection of DNA methylome, due to the increasing throughput of NGS technologies and the decrement in cost. The mapping and alignment of bisulfite reads from NGS (e.g., RRBS, Agilent SureSelect Human Methyl-Seq, NimbleGen SeqCap Epi CpGiant, and whole genomic bisulfite sequencing) are more complicated than the regular sequence reads. However, this massive task can become less burdensome via computational tools, which can be filtered and quality controlled by using BALM, Bismark, BRAT-nova, BS-seeker, BSMAP, MAQ, MOABS, MACAU, MEDIPS, RMAP, PASH, TAMeBS, WALT, etc. [1]. Bisulfite treatment converts the unmethylated cytosines to uracils, and subsequently recognized as thymines in the sequencing reads. The degree of DNA methylation can be calculated from the frequency of cytosines and thymines at a specific CpG locus, by aligning the raw reads against cytosines in the reference genomic sequence [1]. In brief, wild card aligners (e.g., BSMAP, RMAP, and Pash 3.0) substitute cytosines with IUPAC letter “Y” and then align with hashing extension method, in order to match to thymines in the bisulfite reads [1]. Alternatively, three-letter aligners (e.g., Bismark, BS-seeker, and BRAT-nova) can be used to convert all cytosines to lower case “t” in both reference sequence and reads, followed by short read alignment (e.g., Bowtie or Bowtie 2) based on the three-letter code of DNA (A, G, and T) [1]. Upon obtaining the processed data, DNA methylation regions can be highly predictive based on the transcriptional activity of downstream genes, transcription start sites, transcription factor binding sites, presence or absence of TATA box, and/or RNA polymerase II occupancy on DNA [3]. Such computational predictions [3] are useful, particularly where experimental data are still lacking [11,12], which represent the first step toward quantitative analysis of DNA methylation data. When no a priori knowledge is available on a candidate gene methylation, it is more acceptable to assess the DNA methylated regions comprising a number of cytosines or known as “CpG island.” Although several statistical methods have been applied in the detection of differential DNA methylated regions [13], Fisher's exact test or paired nonparametric tests are the most common methods for comparing the methylation levels of the cytosines within the regions of interest. The false discovery rate is required to be corrected for multiple testing, based on the Benjamini–Hochberg procedure. Alternatively, probabilistic and more unbiased methods such as Hidden Markov Models (HMM) can be used for this segmentation problem. Additionally, a multivariate statistical model has been proposed for analyzing epigenetic data [14]. Such approaches are much more realistic than marginal models, in order to optimize the interpretation of the resulting epigenetic data.