A new method for extracting skin microbes allows metagenomic analysis of whole-deep skin.

In the last decade, an extensive effort has been made to characterize the human microbiota, due to its clinical and economic interests. However, a metagenomic approach to the skin microbiota is hampered by the high proportion of host DNA that is recovered. In contrast with the burgeoning field of gu...

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Main Authors: Marc Garcia-Garcerà, Koldo Garcia-Etxebarria, Mireia Coscollà, Amparo Latorre, Francesc Calafell
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2013-01-01
Series:PLoS ONE
Online Access:https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/24073227/?tool=EBI
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spelling doaj-aa5ef7b0aaf644a8bdb425e804b30d9f2021-03-03T20:19:58ZengPublic Library of Science (PLoS)PLoS ONE1932-62032013-01-0189e7491410.1371/journal.pone.0074914A new method for extracting skin microbes allows metagenomic analysis of whole-deep skin.Marc Garcia-GarceràKoldo Garcia-EtxebarriaMireia CoscollàAmparo LatorreFrancesc CalafellIn the last decade, an extensive effort has been made to characterize the human microbiota, due to its clinical and economic interests. However, a metagenomic approach to the skin microbiota is hampered by the high proportion of host DNA that is recovered. In contrast with the burgeoning field of gut metagenomics, skin metagenomics has been hindered by the absence of an efficient method to avoid sequencing the host DNA. We present here a method for recovering microbial DNA from skin samples, based on a combination of molecular techniques. We have applied this method to mouse skin, and have validated it by standard, quantitative PCR and amplicon sequencing of 16S rRNA. The taxonomic diversity recovered was not altered by this new method, as proved by comparing the phylogenetic structure revealed by 16S rRNA sequencing in untreated vs. treated samples. As proof of concept, we also present the first two mouse skin metagenomes, which allowed discovering new taxa (not only prokaryotes but also viruses and eukaryots) not reachable by 16S rRNA sequencing, as well as to characterize the skin microbiome functional landscape. Our method paves the way for the development of skin metagenomics, which will allow a much deeper knowledge of the skin microbiome and its relationship with the host, both in a healthy state and in relation to disease.https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/24073227/?tool=EBI
collection DOAJ
language English
format Article
sources DOAJ
author Marc Garcia-Garcerà
Koldo Garcia-Etxebarria
Mireia Coscollà
Amparo Latorre
Francesc Calafell
spellingShingle Marc Garcia-Garcerà
Koldo Garcia-Etxebarria
Mireia Coscollà
Amparo Latorre
Francesc Calafell
A new method for extracting skin microbes allows metagenomic analysis of whole-deep skin.
PLoS ONE
author_facet Marc Garcia-Garcerà
Koldo Garcia-Etxebarria
Mireia Coscollà
Amparo Latorre
Francesc Calafell
author_sort Marc Garcia-Garcerà
title A new method for extracting skin microbes allows metagenomic analysis of whole-deep skin.
title_short A new method for extracting skin microbes allows metagenomic analysis of whole-deep skin.
title_full A new method for extracting skin microbes allows metagenomic analysis of whole-deep skin.
title_fullStr A new method for extracting skin microbes allows metagenomic analysis of whole-deep skin.
title_full_unstemmed A new method for extracting skin microbes allows metagenomic analysis of whole-deep skin.
title_sort new method for extracting skin microbes allows metagenomic analysis of whole-deep skin.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2013-01-01
description In the last decade, an extensive effort has been made to characterize the human microbiota, due to its clinical and economic interests. However, a metagenomic approach to the skin microbiota is hampered by the high proportion of host DNA that is recovered. In contrast with the burgeoning field of gut metagenomics, skin metagenomics has been hindered by the absence of an efficient method to avoid sequencing the host DNA. We present here a method for recovering microbial DNA from skin samples, based on a combination of molecular techniques. We have applied this method to mouse skin, and have validated it by standard, quantitative PCR and amplicon sequencing of 16S rRNA. The taxonomic diversity recovered was not altered by this new method, as proved by comparing the phylogenetic structure revealed by 16S rRNA sequencing in untreated vs. treated samples. As proof of concept, we also present the first two mouse skin metagenomes, which allowed discovering new taxa (not only prokaryotes but also viruses and eukaryots) not reachable by 16S rRNA sequencing, as well as to characterize the skin microbiome functional landscape. Our method paves the way for the development of skin metagenomics, which will allow a much deeper knowledge of the skin microbiome and its relationship with the host, both in a healthy state and in relation to disease.
url https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/24073227/?tool=EBI
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