Checkpoint
PascalFrancis
Racine
Checkpoint
PascalFrancis
Exploration
Accueil
Racine
Racine

Serveur d'exploration MERS

Attention, ce site est en cours de développement !
Attention, site généré par des moyens informatiques à partir de corpus bruts.
Les informations ne sont donc pas validées.

Evaluation of methods to concentrate and purify ocean virus communities through comparative, replicated metagenomics

Identifieur interne : 000053 ( PascalFrancis/Checkpoint ); précédent : 000052; suivant : 000054

Evaluation of methods to concentrate and purify ocean virus communities through comparative, replicated metagenomics

Auteurs : Bonnie L. Hurwitz [États-Unis] ; LI DENG [États-Unis] ; Bonnie T. Poulos [États-Unis] ; Matthew B. Sullivan [États-Unis]

Source :

RBID : Pascal:13-0209675

Descripteurs français

English descriptors

Abstract

Viruses have global impact through mortality, nutrient cycling and horizontal gene transfer, yet their study is limited by complex methodologies with little validation. Here, we use triplicate metagenomes to compare common aquatic viral concentration and purification methods across four combinations as follows: (i) tangential flow filtration (TFF) and DNase + CsCl, (ii) FeCl3 precipitation and DNase, (iii) FeCl3 precipitation and DNase + CsCl and (iv) FeCl3 precipitation and DNase + sucrose. Taxonomic data (30% of reads) suggested that purification methods were statistically indistinguishable at any taxonomic level while concentration methods were significantly different at family and genus levels. Specifically, TFF-concentrated viral metagenomes had significantly fewer abundant viral types (Podoviridae and Phycod-naviridae) and more variability among Myoviridae than FeCl3-precipitated viral metagenomes. More comprehensive analyses using protein clusters (66% of reads) and k-mers (100% of reads) showed 50-53% of these data were common to all four methods, and revealed trace bacterial DNA contamination in TFF-concentrated metagenomes and one of three replicates concentrated using FeCl3 and purified by DNase alone. Shared k-mer analyses also revealed that polymerases used in amplification impact the resulting metagenomes, with TaKaRa enriching for 'rare' reads relative to PfuTurbo. Together these results provide empirical data for making experimental design decisions in culture-independent viral ecology studies.


Affiliations:

Links toward previous steps (curation, corpus...)

Links to Exploration step

Pascal:13-0209675

Le document en format XML

<record>
<TEI>
<teiHeader>
<fileDesc>
<titleStmt>
<title xml:lang="en" level="a">Evaluation of methods to concentrate and purify ocean virus communities through comparative, replicated metagenomics</title>
<author>
<name sortKey="Hurwitz, Bonnie L" sort="Hurwitz, Bonnie L" uniqKey="Hurwitz B" first="Bonnie L." last="Hurwitz">Bonnie L. Hurwitz</name>
<affiliation wicri:level="2">
<inist:fA14 i1="01">
<s1>Ecology and Evolutionary Biology, University of Arizona</s1>
<s2>Tucson, AZ 85721</s2>
<s3>USA</s3>
<sZ>1 aut.</sZ>
<sZ>2 aut.</sZ>
<sZ>3 aut.</sZ>
<sZ>4 aut.</sZ>
</inist:fA14>
<country>États-Unis</country>
<placeName>
<region type="state">Arizona</region>
</placeName>
</affiliation>
</author>
<author>
<name sortKey="Li Deng" sort="Li Deng" uniqKey="Li Deng" last="Li Deng">LI DENG</name>
<affiliation wicri:level="2">
<inist:fA14 i1="01">
<s1>Ecology and Evolutionary Biology, University of Arizona</s1>
<s2>Tucson, AZ 85721</s2>
<s3>USA</s3>
<sZ>1 aut.</sZ>
<sZ>2 aut.</sZ>
<sZ>3 aut.</sZ>
<sZ>4 aut.</sZ>
</inist:fA14>
<country>États-Unis</country>
<placeName>
<region type="state">Arizona</region>
</placeName>
</affiliation>
</author>
<author>
<name sortKey="Poulos, Bonnie T" sort="Poulos, Bonnie T" uniqKey="Poulos B" first="Bonnie T." last="Poulos">Bonnie T. Poulos</name>
<affiliation wicri:level="2">
<inist:fA14 i1="01">
<s1>Ecology and Evolutionary Biology, University of Arizona</s1>
<s2>Tucson, AZ 85721</s2>
<s3>USA</s3>
<sZ>1 aut.</sZ>
<sZ>2 aut.</sZ>
<sZ>3 aut.</sZ>
<sZ>4 aut.</sZ>
</inist:fA14>
<country>États-Unis</country>
<placeName>
<region type="state">Arizona</region>
</placeName>
</affiliation>
</author>
<author>
<name sortKey="Sullivan, Matthew B" sort="Sullivan, Matthew B" uniqKey="Sullivan M" first="Matthew B." last="Sullivan">Matthew B. Sullivan</name>
<affiliation wicri:level="2">
<inist:fA14 i1="01">
<s1>Ecology and Evolutionary Biology, University of Arizona</s1>
<s2>Tucson, AZ 85721</s2>
<s3>USA</s3>
<sZ>1 aut.</sZ>
<sZ>2 aut.</sZ>
<sZ>3 aut.</sZ>
<sZ>4 aut.</sZ>
</inist:fA14>
<country>États-Unis</country>
<placeName>
<region type="state">Arizona</region>
</placeName>
</affiliation>
</author>
</titleStmt>
<publicationStmt>
<idno type="wicri:source">INIST</idno>
<idno type="inist">13-0209675</idno>
<date when="2013">2013</date>
<idno type="stanalyst">PASCAL 13-0209675 INIST</idno>
<idno type="RBID">Pascal:13-0209675</idno>
<idno type="wicri:Area/PascalFrancis/Corpus">000060</idno>
<idno type="wicri:Area/PascalFrancis/Curation">000034</idno>
<idno type="wicri:Area/PascalFrancis/Checkpoint">000053</idno>
<idno type="wicri:explorRef" wicri:stream="PascalFrancis" wicri:step="Checkpoint">000053</idno>
</publicationStmt>
<sourceDesc>
<biblStruct>
<analytic>
<title xml:lang="en" level="a">Evaluation of methods to concentrate and purify ocean virus communities through comparative, replicated metagenomics</title>
<author>
<name sortKey="Hurwitz, Bonnie L" sort="Hurwitz, Bonnie L" uniqKey="Hurwitz B" first="Bonnie L." last="Hurwitz">Bonnie L. Hurwitz</name>
<affiliation wicri:level="2">
<inist:fA14 i1="01">
<s1>Ecology and Evolutionary Biology, University of Arizona</s1>
<s2>Tucson, AZ 85721</s2>
<s3>USA</s3>
<sZ>1 aut.</sZ>
<sZ>2 aut.</sZ>
<sZ>3 aut.</sZ>
<sZ>4 aut.</sZ>
</inist:fA14>
<country>États-Unis</country>
<placeName>
<region type="state">Arizona</region>
</placeName>
</affiliation>
</author>
<author>
<name sortKey="Li Deng" sort="Li Deng" uniqKey="Li Deng" last="Li Deng">LI DENG</name>
<affiliation wicri:level="2">
<inist:fA14 i1="01">
<s1>Ecology and Evolutionary Biology, University of Arizona</s1>
<s2>Tucson, AZ 85721</s2>
<s3>USA</s3>
<sZ>1 aut.</sZ>
<sZ>2 aut.</sZ>
<sZ>3 aut.</sZ>
<sZ>4 aut.</sZ>
</inist:fA14>
<country>États-Unis</country>
<placeName>
<region type="state">Arizona</region>
</placeName>
</affiliation>
</author>
<author>
<name sortKey="Poulos, Bonnie T" sort="Poulos, Bonnie T" uniqKey="Poulos B" first="Bonnie T." last="Poulos">Bonnie T. Poulos</name>
<affiliation wicri:level="2">
<inist:fA14 i1="01">
<s1>Ecology and Evolutionary Biology, University of Arizona</s1>
<s2>Tucson, AZ 85721</s2>
<s3>USA</s3>
<sZ>1 aut.</sZ>
<sZ>2 aut.</sZ>
<sZ>3 aut.</sZ>
<sZ>4 aut.</sZ>
</inist:fA14>
<country>États-Unis</country>
<placeName>
<region type="state">Arizona</region>
</placeName>
</affiliation>
</author>
<author>
<name sortKey="Sullivan, Matthew B" sort="Sullivan, Matthew B" uniqKey="Sullivan M" first="Matthew B." last="Sullivan">Matthew B. Sullivan</name>
<affiliation wicri:level="2">
<inist:fA14 i1="01">
<s1>Ecology and Evolutionary Biology, University of Arizona</s1>
<s2>Tucson, AZ 85721</s2>
<s3>USA</s3>
<sZ>1 aut.</sZ>
<sZ>2 aut.</sZ>
<sZ>3 aut.</sZ>
<sZ>4 aut.</sZ>
</inist:fA14>
<country>États-Unis</country>
<placeName>
<region type="state">Arizona</region>
</placeName>
</affiliation>
</author>
</analytic>
<series>
<title level="j" type="main">Environmental microbiology : (Print)</title>
<title level="j" type="abbreviated">Environ. microbiol. : (Print)</title>
<idno type="ISSN">1462-2912</idno>
<imprint>
<date when="2013">2013</date>
</imprint>
</series>
</biblStruct>
</sourceDesc>
<seriesStmt>
<title level="j" type="main">Environmental microbiology : (Print)</title>
<title level="j" type="abbreviated">Environ. microbiol. : (Print)</title>
<idno type="ISSN">1462-2912</idno>
</seriesStmt>
</fileDesc>
<profileDesc>
<textClass>
<keywords scheme="KwdEn" xml:lang="en">
<term>Community</term>
<term>Concentrate</term>
<term>Metagenome</term>
<term>Method</term>
<term>Ocean</term>
<term>Virus</term>
</keywords>
<keywords scheme="Pascal" xml:lang="fr">
<term>Méthode</term>
<term>Concentrat</term>
<term>Océan</term>
<term>Communauté</term>
<term>Virus</term>
<term>Métagénome</term>
</keywords>
<keywords scheme="Wicri" type="topic" xml:lang="fr">
<term>Océan</term>
</keywords>
</textClass>
</profileDesc>
</teiHeader>
<front>
<div type="abstract" xml:lang="en">Viruses have global impact through mortality, nutrient cycling and horizontal gene transfer, yet their study is limited by complex methodologies with little validation. Here, we use triplicate metagenomes to compare common aquatic viral concentration and purification methods across four combinations as follows: (i) tangential flow filtration (TFF) and DNase + CsCl, (ii) FeCl
<sub>3</sub>
precipitation and DNase, (iii) FeCl
<sub>3</sub>
precipitation and DNase + CsCl and (iv) FeCl
<sub>3</sub>
precipitation and DNase + sucrose. Taxonomic data (30% of reads) suggested that purification methods were statistically indistinguishable at any taxonomic level while concentration methods were significantly different at family and genus levels. Specifically, TFF-concentrated viral metagenomes had significantly fewer abundant viral types (Podoviridae and Phycod-naviridae) and more variability among Myoviridae than FeCl
<sub>3</sub>
-precipitated viral metagenomes. More comprehensive analyses using protein clusters (66% of reads) and k-mers (100% of reads) showed 50-53% of these data were common to all four methods, and revealed trace bacterial DNA contamination in TFF-concentrated metagenomes and one of three replicates concentrated using FeCl
<sub>3</sub>
and purified by DNase alone. Shared k-mer analyses also revealed that polymerases used in amplification impact the resulting metagenomes, with TaKaRa enriching for 'rare' reads relative to PfuTurbo. Together these results provide empirical data for making experimental design decisions in culture-independent viral ecology studies.</div>
</front>
</TEI>
<inist>
<standard h6="B">
<pA>
<fA01 i1="01" i2="1">
<s0>1462-2912</s0>
</fA01>
<fA03 i2="1">
<s0>Environ. microbiol. : (Print)</s0>
</fA03>
<fA05>
<s2>15</s2>
</fA05>
<fA06>
<s2>5</s2>
</fA06>
<fA08 i1="01" i2="1" l="ENG">
<s1>Evaluation of methods to concentrate and purify ocean virus communities through comparative, replicated metagenomics</s1>
</fA08>
<fA09 i1="01" i2="1" l="ENG">
<s1>Special Issue on Marine Microbial Ecophysiology and Metagenomics</s1>
</fA09>
<fA11 i1="01" i2="1">
<s1>HURWITZ (Bonnie L.)</s1>
</fA11>
<fA11 i1="02" i2="1">
<s1>LI DENG</s1>
</fA11>
<fA11 i1="03" i2="1">
<s1>POULOS (Bonnie T.)</s1>
</fA11>
<fA11 i1="04" i2="1">
<s1>SULLIVAN (Matthew B.)</s1>
</fA11>
<fA14 i1="01">
<s1>Ecology and Evolutionary Biology, University of Arizona</s1>
<s2>Tucson, AZ 85721</s2>
<s3>USA</s3>
<sZ>1 aut.</sZ>
<sZ>2 aut.</sZ>
<sZ>3 aut.</sZ>
<sZ>4 aut.</sZ>
</fA14>
<fA20>
<s1>1428-1440</s1>
</fA20>
<fA21>
<s1>2013</s1>
</fA21>
<fA23 i1="01">
<s0>ENG</s0>
</fA23>
<fA43 i1="01">
<s1>INIST</s1>
<s2>28131</s2>
<s5>354000500700030140</s5>
</fA43>
<fA44>
<s0>0000</s0>
<s1>© 2013 INIST-CNRS. All rights reserved.</s1>
</fA44>
<fA45>
<s0>1 p.3/4</s0>
</fA45>
<fA47 i1="01" i2="1">
<s0>13-0209675</s0>
</fA47>
<fA60>
<s1>P</s1>
</fA60>
<fA61>
<s0>A</s0>
</fA61>
<fA64 i1="01" i2="1">
<s0>Environmental microbiology : (Print)</s0>
</fA64>
<fA66 i1="01">
<s0>GBR</s0>
</fA66>
<fC01 i1="01" l="ENG">
<s0>Viruses have global impact through mortality, nutrient cycling and horizontal gene transfer, yet their study is limited by complex methodologies with little validation. Here, we use triplicate metagenomes to compare common aquatic viral concentration and purification methods across four combinations as follows: (i) tangential flow filtration (TFF) and DNase + CsCl, (ii) FeCl
<sub>3</sub>
precipitation and DNase, (iii) FeCl
<sub>3</sub>
precipitation and DNase + CsCl and (iv) FeCl
<sub>3</sub>
precipitation and DNase + sucrose. Taxonomic data (30% of reads) suggested that purification methods were statistically indistinguishable at any taxonomic level while concentration methods were significantly different at family and genus levels. Specifically, TFF-concentrated viral metagenomes had significantly fewer abundant viral types (Podoviridae and Phycod-naviridae) and more variability among Myoviridae than FeCl
<sub>3</sub>
-precipitated viral metagenomes. More comprehensive analyses using protein clusters (66% of reads) and k-mers (100% of reads) showed 50-53% of these data were common to all four methods, and revealed trace bacterial DNA contamination in TFF-concentrated metagenomes and one of three replicates concentrated using FeCl
<sub>3</sub>
and purified by DNase alone. Shared k-mer analyses also revealed that polymerases used in amplification impact the resulting metagenomes, with TaKaRa enriching for 'rare' reads relative to PfuTurbo. Together these results provide empirical data for making experimental design decisions in culture-independent viral ecology studies.</s0>
</fC01>
<fC02 i1="01" i2="X">
<s0>002A14C01</s0>
</fC02>
<fC02 i1="02" i2="X">
<s0>002A05C04</s0>
</fC02>
<fC03 i1="01" i2="X" l="FRE">
<s0>Méthode</s0>
<s5>01</s5>
</fC03>
<fC03 i1="01" i2="X" l="ENG">
<s0>Method</s0>
<s5>01</s5>
</fC03>
<fC03 i1="01" i2="X" l="SPA">
<s0>Método</s0>
<s5>01</s5>
</fC03>
<fC03 i1="02" i2="X" l="FRE">
<s0>Concentrat</s0>
<s5>02</s5>
</fC03>
<fC03 i1="02" i2="X" l="ENG">
<s0>Concentrate</s0>
<s5>02</s5>
</fC03>
<fC03 i1="02" i2="X" l="SPA">
<s0>Concentrado</s0>
<s5>02</s5>
</fC03>
<fC03 i1="03" i2="X" l="FRE">
<s0>Océan</s0>
<s5>03</s5>
</fC03>
<fC03 i1="03" i2="X" l="ENG">
<s0>Ocean</s0>
<s5>03</s5>
</fC03>
<fC03 i1="03" i2="X" l="SPA">
<s0>Océano</s0>
<s5>03</s5>
</fC03>
<fC03 i1="04" i2="X" l="FRE">
<s0>Communauté</s0>
<s5>04</s5>
</fC03>
<fC03 i1="04" i2="X" l="ENG">
<s0>Community</s0>
<s5>04</s5>
</fC03>
<fC03 i1="04" i2="X" l="SPA">
<s0>Comunidad</s0>
<s5>04</s5>
</fC03>
<fC03 i1="05" i2="X" l="FRE">
<s0>Virus</s0>
<s2>NW</s2>
<s5>49</s5>
</fC03>
<fC03 i1="05" i2="X" l="ENG">
<s0>Virus</s0>
<s2>NW</s2>
<s5>49</s5>
</fC03>
<fC03 i1="05" i2="X" l="SPA">
<s0>Virus</s0>
<s2>NW</s2>
<s5>49</s5>
</fC03>
<fC03 i1="06" i2="X" l="FRE">
<s0>Métagénome</s0>
<s4>CD</s4>
<s5>96</s5>
</fC03>
<fC03 i1="06" i2="X" l="ENG">
<s0>Metagenome</s0>
<s4>CD</s4>
<s5>96</s5>
</fC03>
<fC07 i1="01" i2="X" l="FRE">
<s0>Milieu marin</s0>
<s5>17</s5>
</fC07>
<fC07 i1="01" i2="X" l="ENG">
<s0>Marine environment</s0>
<s5>17</s5>
</fC07>
<fC07 i1="01" i2="X" l="SPA">
<s0>Medio marino</s0>
<s5>17</s5>
</fC07>
<fN21>
<s1>196</s1>
</fN21>
<fN44 i1="01">
<s1>OTO</s1>
</fN44>
<fN82>
<s1>OTO</s1>
</fN82>
</pA>
</standard>
</inist>
<affiliations>
<list>
<country>
<li>États-Unis</li>
</country>
<region>
<li>Arizona</li>
</region>
</list>
<tree>
<country name="États-Unis">
<region name="Arizona">
<name sortKey="Hurwitz, Bonnie L" sort="Hurwitz, Bonnie L" uniqKey="Hurwitz B" first="Bonnie L." last="Hurwitz">Bonnie L. Hurwitz</name>
</region>
<name sortKey="Li Deng" sort="Li Deng" uniqKey="Li Deng" last="Li Deng">LI DENG</name>
<name sortKey="Poulos, Bonnie T" sort="Poulos, Bonnie T" uniqKey="Poulos B" first="Bonnie T." last="Poulos">Bonnie T. Poulos</name>
<name sortKey="Sullivan, Matthew B" sort="Sullivan, Matthew B" uniqKey="Sullivan M" first="Matthew B." last="Sullivan">Matthew B. Sullivan</name>
</country>
</tree>
</affiliations>
</record>

Pour manipuler ce document sous Unix (Dilib)

EXPLOR_STEP=$WICRI_ROOT/Sante/explor/MersV1/Data/PascalFrancis/Checkpoint

HfdSelect -h $EXPLOR_STEP/biblio.hfd -nk 000053 | SxmlIndent | more

Ou

HfdSelect -h $EXPLOR_AREA/Data/PascalFrancis/Checkpoint/biblio.hfd -nk 000053 | SxmlIndent | more

Pour mettre un lien sur cette page dans le réseau Wicri

{{Explor lien
   |wiki=    Sante
   |area=    MersV1
   |flux=    PascalFrancis
   |étape=   Checkpoint
   |type=    RBID
   |clé=     Pascal:13-0209675
   |texte=   Evaluation of methods to concentrate and purify ocean virus communities through comparative, replicated metagenomics
}}
Wicri

This area was generated with Dilib version V0.6.33.
Data generation: Mon Apr 20 23:26:43 2020. Site generation: Sat Mar 27 09:06:09 2021