Database Commons
Database Commons

a catalog of worldwide biological databases

Database Profile

General information

URL: http://bioinfo2.ugr.es/NGSmethDB
Full name: High-quality Methylation Maps
Description: A repository for single-base whole-genome methylome maps for the best-assembled eukaryotic genomes
Year founded: 2011
Last update: 2016-08-08
Version: v3
Accessibility:
Manual:
Accessible
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Country/Region: Spain

Contact information

University/Institution: University of Granada
Address: 18071-Granada, Spain and Laboratorio de Bioinformática, Instituto de Biotecnología, Centro de Investigación Biomédica, 18100-Granada, Spain
City: Granada
Province/State:
Country/Region: Spain
Contact name (PI/Team): José L Oliver
Contact email (PI/Helpdesk): oliver@ugr.es

Publications

27794041
NGSmethDB 2017: enhanced methylomes and differential methylation. [PMID: 27794041]
Lebrón R, Gómez-Martín C, Carpena P, Bernaola-Galván P, Barturen G, Hackenberg M, Oliver JL.

The 2017 update of NGSmethDB stores whole genome methylomes generated from short-read data sets obtained by bisulfite sequencing (WGBS) technology. To generate high-quality methylomes, stringent quality controls were integrated with third-part software, adding also a two-step mapping process to exploit the advantages of the new genome assembly models. The samples were all profiled under constant parameter settings, thus enabling comparative downstream analyses. Besides a significant increase in the number of samples, NGSmethDB now includes two additional data-types, which are a valuable resource for the discovery of methylation epigenetic biomarkers: (i) differentially methylated single-cytosines; and (ii) methylation segments (i.e. genome regions of homogeneous methylation). The NGSmethDB back-end is now based on MongoDB, a NoSQL hierarchical database using JSON-formatted documents and dynamic schemas, thus accelerating sample comparative analyses. Besides conventional database dumps, track hubs were implemented, which improved database access, visualization in genome browsers and comparative analyses to third-part annotations. In addition, the database can be also accessed through a RESTful API. Lastly, a Python client and a multiplatform virtual machine allow for program-driven access from user desktop. This way, private methylation data can be compared to NGSmethDB without the need to upload them to public servers. Database website: http://bioinfo2.ugr.es/NGSmethDB. © The Author(s) 2016. Published by Oxford University Press on behalf of Nucleic Acids Research.

Nucleic Acids Res. 2017:45(D1) | 7 Citations (from Europe PMC, 2024-04-20)
24271385
NGSmethDB: an updated genome resource for high quality, single-cytosine resolution methylomes. [PMID: 24271385]
Geisen S, Barturen G, Alganza ÁM, Hackenberg M, Oliver JL.

The updated release of 'NGSmethDB' (http://bioinfo2.ugr.es/NGSmethDB) is a repository for single-base whole-genome methylome maps for the best-assembled eukaryotic genomes. Short-read data sets from NGS bisulfite-sequencing projects of cell lines, fresh and pathological tissues are first pre-processed and aligned to the corresponding reference genome, and then the cytosine methylation levels are profiled. One major improvement is the application of a unique bioinformatics protocol to all data sets, thereby assuring the comparability of all values with each other. We implemented stringent quality controls to minimize important error sources, such as sequencing errors, bisulfite failures, clonal reads or single nucleotide variants (SNVs). This leads to reliable and high-quality methylomes, all obtained under uniform settings. Another significant improvement is the detection in parallel of SNVs, which might be crucial for many downstream analyses (e.g. SNVs and differential-methylation relationships). A next-generation methylation browser allows fast and smooth scrolling and zooming, thus speeding data download/upload, at the same time requiring fewer server resources. Several data mining tools allow the comparison/retrieval of methylation levels in different tissues or genome regions. NGSmethDB methylomes are also available as native tracks through a UCSC hub, which allows comparison with a wide range of third-party annotations, in particular phenotype or disease annotations.

Nucleic Acids Res. 2014:42(Database issue) | 10 Citations (from Europe PMC, 2024-04-20)
20965971
NGSmethDB: a database for next-generation sequencing single-cytosine-resolution DNA methylation data. [PMID: 20965971]
Hackenberg M, Barturen G, Oliver JL.

Next-generation sequencing (NGS) together with bisulphite conversion allows the generation of whole genome methylation maps at single-cytosine resolution. This allows studying the absence of methylation in a particular genome region over a range of tissues, the differential tissue methylation or the changes occurring along pathological conditions. However, no database exists fully addressing such requirements. We propose here NGSmethDB (http://bioinfo2.ugr.es/NGSmethDB/gbrowse/) for the storage and retrieval of methylation data derived from NGS. Two cytosine methylation contexts (CpG and CAG/CTG) are considered. Through a browser interface coupled to a MySQL backend and several data mining tools, the user can search for methylation states in a set of tissues, retrieve methylation values for a set of tissues in a given chromosomal region, or display the methylation of promoters among different tissues. NGSmethDB is currently populated with human, mouse and Arabidopsis data, but other methylomes will be incorporated through an automatic pipeline as soon as new data become available. Dump downloads for three coverage levels (1, 5 or 10 reads) are available. NGSmethDB will be useful for experimental researchers, as well as for bioinformaticians, who might use the data as input for further research.

Nucleic Acids Res. 2011:39(Database issue) | 39 Citations (from Europe PMC, 2024-04-20)

Ranking

All databases:
1919/6000 (68.033%)
Modification:
115/287 (60.279%)
1919
Total Rank
56
Citations
4.308
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Record metadata

Created on: 2015-06-20
Curated by:
Lina Ma [2017-06-21]
Shixiang Sun [2017-02-13]
Lin Liu [2016-03-30]
Lin Liu [2016-03-28]
Zhang Zhang [2016-01-03]
Li Yang [2015-06-26]