Optimization of Low-Biomass Sample Collection and Quantitative PCR-Based Titration Impact 16S rRNA Microbiome Resolution

The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that i...

Full description

Saved in:
Bibliographic Details
Published inMicrobiology spectrum Vol. 10; no. 6; p. e0225522
Main Authors Clokie, Benjamin Gregory James, Elsheshtawy, Ahmed, Albalat, Amaya, Nylund, Are, Beveridge, Allan, Payne, Chris J., MacKenzie, Simon
Format Journal Article
LanguageEnglish
Published United States American Society for Microbiology 21.12.2022
Subjects
16S rRNA
Animals
Bacteria - genetics
Biomass
complex
DNA Contamination
DNA, Bacterial - genetics
Ecology
equicopy
Fishes - genetics
gill
low-biomass
Microbiota - genetics
Polymerase Chain Reaction - methods
Research Article
RNA, Ribosomal, 16S - genetics
titration
16S rRNA
equicopy
gill
titration
low-biomass
complex
Online AccessGet full text

Cover

Abstract The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that inhibit the ability to produce libraries that identify the components of microbial communities, present significant challenges. The major aquatic interface between host and environment in teleost finfish species is the gill. The diversity of this infraclass, high complexity of the organ, and its direct exposure to the surrounding environment make it an ideal candidate for furthering our understanding of the intertwined relationships between host and microbiome. Capturing the structure and diversity of bacterial communities from this low-biomass, inhibitor-rich tissue can, however, prove challenging. Lessons learned in doing so are directly applicable to similar sample types in other areas of microbiology. Through the development of a quantitative PCR assay for both host material and 16S rRNA genes, we tested and developed a robust method for low-biomass sample collection which minimized host DNA contamination. Quantification of 16S rRNA facilitated not only the screening of samples prior to costly library construction and sequencing but also the production of equicopy libraries based on 16S rRNA gene copies. A significant increase in diversity of bacteria captured was achieved, providing greater information on the true structure of the microbial community. Such findings offer important information for determining functional processes. Results were confirmed across fresh, brackish, and marine environs with four different fish species, with results showing broad homology between samples, demonstrating the robustness of the approach. Evidence presented is widely applicable to samples similar in composition, such as sputum or mucus, or those that are challenging due to the inherent inclusion of inhibitors. IMPORTANCE The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that inhibit the ability to produce libraries that identify the components of microbial communities, present significant challenges. Gill samples present both of these types of challenges. We developed methods for quantifying both the bacterial and host DNA material and established a sampling method which both reduced inhibitor content and maximized bacterial diversity. By quantifying and normalizing bacteria prior to library construction, we showed significant improvements with regards to the fidelity of the final data. Our results support wide-ranging applications for analyzing samples of similar composition, such as mucus and sputum, in other microbiological spheres.
AbstractList The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that inhibit the ability to produce libraries that identify the components of microbial communities, present significant challenges. The major aquatic interface between host and environment in teleost finfish species is the gill. The diversity of this infraclass, high complexity of the organ, and its direct exposure to the surrounding environment make it an ideal candidate for furthering our understanding of the intertwined relationships between host and microbiome. Capturing the structure and diversity of bacterial communities from this low-biomass, inhibitor-rich tissue can, however, prove challenging. Lessons learned in doing so are directly applicable to similar sample types in other areas of microbiology. Through the development of a quantitative PCR assay for both host material and 16S rRNA genes, we tested and developed a robust method for low-biomass sample collection which minimized host DNA contamination. Quantification of 16S rRNA facilitated not only the screening of samples prior to costly library construction and sequencing but also the production of equicopy libraries based on 16S rRNA gene copies. A significant increase in diversity of bacteria captured was achieved, providing greater information on the true structure of the microbial community. Such findings offer important information for determining functional processes. Results were confirmed across fresh, brackish, and marine environs with four different fish species, with results showing broad homology between samples, demonstrating the robustness of the approach. Evidence presented is widely applicable to samples similar in composition, such as sputum or mucus, or those that are challenging due to the inherent inclusion of inhibitors. IMPORTANCE The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that inhibit the ability to produce libraries that identify the components of microbial communities, present significant challenges. Gill samples present both of these types of challenges. We developed methods for quantifying both the bacterial and host DNA material and established a sampling method which both reduced inhibitor content and maximized bacterial diversity. By quantifying and normalizing bacteria prior to library construction, we showed significant improvements with regards to the fidelity of the final data. Our results support wide-ranging applications for analyzing samples of similar composition, such as mucus and sputum, in other microbiological spheres.
ABSTRACT The major aquatic interface between host and environment in teleost finfish species is the gill. The diversity of this infraclass, high complexity of the organ, and its direct exposure to the surrounding environment make it an ideal candidate for furthering our understanding of the intertwined relationships between host and microbiome. Capturing the structure and diversity of bacterial communities from this low-biomass, inhibitor-rich tissue can, however, prove challenging. Lessons learned in doing so are directly applicable to similar sample types in other areas of microbiology. Through the development of a quantitative PCR assay for both host material and 16S rRNA genes, we tested and developed a robust method for low-biomass sample collection which minimized host DNA contamination. Quantification of 16S rRNA facilitated not only the screening of samples prior to costly library construction and sequencing but also the production of equicopy libraries based on 16S rRNA gene copies. A significant increase in diversity of bacteria captured was achieved, providing greater information on the true structure of the microbial community. Such findings offer important information for determining functional processes. Results were confirmed across fresh, brackish, and marine environs with four different fish species, with results showing broad homology between samples, demonstrating the robustness of the approach. Evidence presented is widely applicable to samples similar in composition, such as sputum or mucus, or those that are challenging due to the inherent inclusion of inhibitors. IMPORTANCE The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that inhibit the ability to produce libraries that identify the components of microbial communities, present significant challenges. Gill samples present both of these types of challenges. We developed methods for quantifying both the bacterial and host DNA material and established a sampling method which both reduced inhibitor content and maximized bacterial diversity. By quantifying and normalizing bacteria prior to library construction, we showed significant improvements with regards to the fidelity of the final data. Our results support wide-ranging applications for analyzing samples of similar composition, such as mucus and sputum, in other microbiological spheres.
The major aquatic interface between host and environment in teleost finfish species is the gill. The diversity of this infraclass, high complexity of the organ, and its direct exposure to the surrounding environment make it an ideal candidate for furthering our understanding of the intertwined relationships between host and microbiome. Capturing the structure and diversity of bacterial communities from this low-biomass, inhibitor-rich tissue can, however, prove challenging. Lessons learned in doing so are directly applicable to similar sample types in other areas of microbiology. Through the development of a quantitative PCR assay for both host material and 16S rRNA genes, we tested and developed a robust method for low-biomass sample collection which minimized host DNA contamination. Quantification of 16S rRNA facilitated not only the screening of samples prior to costly library construction and sequencing but also the production of equicopy libraries based on 16S rRNA gene copies. A significant increase in diversity of bacteria captured was achieved, providing greater information on the true structure of the microbial community. Such findings offer important information for determining functional processes. Results were confirmed across fresh, brackish, and marine environs with four different fish species, with results showing broad homology between samples, demonstrating the robustness of the approach. Evidence presented is widely applicable to samples similar in composition, such as sputum or mucus, or those that are challenging due to the inherent inclusion of inhibitors. IMPORTANCE The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that inhibit the ability to produce libraries that identify the components of microbial communities, present significant challenges. Gill samples present both of these types of challenges. We developed methods for quantifying both the bacterial and host DNA material and established a sampling method which both reduced inhibitor content and maximized bacterial diversity. By quantifying and normalizing bacteria prior to library construction, we showed significant improvements with regards to the fidelity of the final data. Our results support wide-ranging applications for analyzing samples of similar composition, such as mucus and sputum, in other microbiological spheres.The major aquatic interface between host and environment in teleost finfish species is the gill. The diversity of this infraclass, high complexity of the organ, and its direct exposure to the surrounding environment make it an ideal candidate for furthering our understanding of the intertwined relationships between host and microbiome. Capturing the structure and diversity of bacterial communities from this low-biomass, inhibitor-rich tissue can, however, prove challenging. Lessons learned in doing so are directly applicable to similar sample types in other areas of microbiology. Through the development of a quantitative PCR assay for both host material and 16S rRNA genes, we tested and developed a robust method for low-biomass sample collection which minimized host DNA contamination. Quantification of 16S rRNA facilitated not only the screening of samples prior to costly library construction and sequencing but also the production of equicopy libraries based on 16S rRNA gene copies. A significant increase in diversity of bacteria captured was achieved, providing greater information on the true structure of the microbial community. Such findings offer important information for determining functional processes. Results were confirmed across fresh, brackish, and marine environs with four different fish species, with results showing broad homology between samples, demonstrating the robustness of the approach. Evidence presented is widely applicable to samples similar in composition, such as sputum or mucus, or those that are challenging due to the inherent inclusion of inhibitors. IMPORTANCE The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that inhibit the ability to produce libraries that identify the components of microbial communities, present significant challenges. Gill samples present both of these types of challenges. We developed methods for quantifying both the bacterial and host DNA material and established a sampling method which both reduced inhibitor content and maximized bacterial diversity. By quantifying and normalizing bacteria prior to library construction, we showed significant improvements with regards to the fidelity of the final data. Our results support wide-ranging applications for analyzing samples of similar composition, such as mucus and sputum, in other microbiological spheres.
The major aquatic interface between host and environment in teleost finfish species is the gill. The diversity of this infraclass, high complexity of the organ, and its direct exposure to the surrounding environment make it an ideal candidate for furthering our understanding of the intertwined relationships between host and microbiome. Capturing the structure and diversity of bacterial communities from this low-biomass, inhibitor-rich tissue can, however, prove challenging. Lessons learned in doing so are directly applicable to similar sample types in other areas of microbiology. Through the development of a quantitative PCR assay for both host material and 16S rRNA genes, we tested and developed a robust method for low-biomass sample collection which minimized host DNA contamination. Quantification of 16S rRNA facilitated not only the screening of samples prior to costly library construction and sequencing but also the production of equicopy libraries based on 16S rRNA gene copies. A significant increase in diversity of bacteria captured was achieved, providing greater information on the true structure of the microbial community. Such findings offer important information for determining functional processes. Results were confirmed across fresh, brackish, and marine environs with four different fish species, with results showing broad homology between samples, demonstrating the robustness of the approach. Evidence presented is widely applicable to samples similar in composition, such as sputum or mucus, or those that are challenging due to the inherent inclusion of inhibitors. The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that inhibit the ability to produce libraries that identify the components of microbial communities, present significant challenges. Gill samples present both of these types of challenges. We developed methods for quantifying both the bacterial and host DNA material and established a sampling method which both reduced inhibitor content and maximized bacterial diversity. By quantifying and normalizing bacteria prior to library construction, we showed significant improvements with regards to the fidelity of the final data. Our results support wide-ranging applications for analyzing samples of similar composition, such as mucus and sputum, in other microbiological spheres.
The major aquatic interface between host and environment in teleost finfish species is the gill. The diversity of this infraclass, high complexity of the organ, and its direct exposure to the surrounding environment make it an ideal candidate for furthering our understanding of the intertwined relationships between host and microbiome. Capturing the structure and diversity of bacterial communities from this low-biomass, inhibitor-rich tissue can, however, prove challenging. Lessons learned in doing so are directly applicable to similar sample types in other areas of microbiology. Through the development of a quantitative PCR assay for both host material and 16S rRNA genes, we tested and developed a robust method for low-biomass sample collection which minimized host DNA contamination. Quantification of 16S rRNA facilitated not only the screening of samples prior to costly library construction and sequencing but also the production of equicopy libraries based on 16S rRNA gene copies. A significant increase in diversity of bacteria captured was achieved, providing greater information on the true structure of the microbial community. Such findings offer important information for determining functional processes. Results were confirmed across fresh, brackish, and marine environs with four different fish species, with results showing broad homology between samples, demonstrating the robustness of the approach. Evidence presented is widely applicable to samples similar in composition, such as sputum or mucus, or those that are challenging due to the inherent inclusion of inhibitors. IMPORTANCE The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that inhibit the ability to produce libraries that identify the components of microbial communities, present significant challenges. Gill samples present both of these types of challenges. We developed methods for quantifying both the bacterial and host DNA material and established a sampling method which both reduced inhibitor content and maximized bacterial diversity. By quantifying and normalizing bacteria prior to library construction, we showed significant improvements with regards to the fidelity of the final data. Our results support wide-ranging applications for analyzing samples of similar composition, such as mucus and sputum, in other microbiological spheres.
The major aquatic interface between host and environment in teleost finfish species is the gill. The diversity of this infraclass, high complexity of the organ, and its direct exposure to the surrounding environment make it an ideal candidate for furthering our understanding of the intertwined relationships between host and microbiome. Capturing the structure and diversity of bacterial communities from this low-biomass, inhibitor-rich tissue can, however, prove challenging. Lessons learned in doing so are directly applicable to similar sample types in other areas of microbiology. Through the development of a quantitative PCR assay for both host material and 16S rRNA genes, we tested and developed a robust method for low-biomass sample collection which minimized host DNA contamination. Quantification of 16S rRNA facilitated not only the screening of samples prior to costly library construction and sequencing but also the production of equicopy libraries based on 16S rRNA gene copies. A significant increase in diversity of bacteria captured was achieved, providing greater information on the true structure of the microbial community. Such findings offer important information for determining functional processes. Results were confirmed across fresh, brackish, and marine environs with four different fish species, with results showing broad homology between samples, demonstrating the robustness of the approach. Evidence presented is widely applicable to samples similar in composition, such as sputum or mucus, or those that are challenging due to the inherent inclusion of inhibitors. IMPORTANCE The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish, free-floating bacteria, and the bacterial microbiome on the gill surface. Samples that are inherently low in bacteria, or that have components that inhibit the ability to produce libraries that identify the components of microbial communities, present significant challenges. Gill samples present both of these types of challenges. We developed methods for quantifying both the bacterial and host DNA material and established a sampling method which both reduced inhibitor content and maximized bacterial diversity. By quantifying and normalizing bacteria prior to library construction, we showed significant improvements with regards to the fidelity of the final data. Our results support wide-ranging applications for analyzing samples of similar composition, such as mucus and sputum, in other microbiological spheres.
Author Payne, Chris J.
Albalat, Amaya
Beveridge, Allan
Elsheshtawy, Ahmed
Clokie, Benjamin Gregory James
Nylund, Are
MacKenzie, Simon
Author_xml – sequence: 1
  givenname: Benjamin Gregory James
  orcidid: 0000-0003-4692-4711
  surname: Clokie
  fullname: Clokie, Benjamin Gregory James
  organization: Institute of Aquaculture, University of Stirling, Stirling, United Kingdom
– sequence: 2
  givenname: Ahmed
  surname: Elsheshtawy
  fullname: Elsheshtawy, Ahmed
  organization: Institute of Aquaculture, University of Stirling, Stirling, United Kingdom, Faculty of Aquatic and Fisheries Sciences, Kafrelsheikh University, Kafr El Sheikh City, Egypt
– sequence: 3
  givenname: Amaya
  surname: Albalat
  fullname: Albalat, Amaya
  organization: Institute of Aquaculture, University of Stirling, Stirling, United Kingdom
– sequence: 4
  givenname: Are
  surname: Nylund
  fullname: Nylund, Are
  organization: Fish Disease Research Group, Department of Biological Sciences, University of Bergen, Bergen, Norway
– sequence: 5
  givenname: Allan
  surname: Beveridge
  fullname: Beveridge, Allan
  organization: Institute of Aquaculture, University of Stirling, Stirling, United Kingdom
– sequence: 6
  givenname: Chris J.
  surname: Payne
  fullname: Payne, Chris J.
  organization: Institute of Aquaculture, University of Stirling, Stirling, United Kingdom
– sequence: 7
  givenname: Simon
  surname: MacKenzie
  fullname: MacKenzie, Simon
  organization: Institute of Aquaculture, University of Stirling, Stirling, United Kingdom
BackLink https://www.ncbi.nlm.nih.gov/pubmed/36377933$$D View this record in MEDLINE/PubMed
BookMark eNp9kUtv1DAUhSNUREvpD2CDvGSTwXZiO9kgtSMeIw0UpmVt3Tg3xaMkDnZSHr8eZ6aDWiTwxtb1Od-99nmaHPWuxyR5zuiCMV68CgOa0U_dgnIuRMr5o-SEMylSmpfq6N75ODkLYUspZYwKLviT5DiTmVJllp0kPy6H0Xb2F4zW9cQ1ZO2-pxfWdRACuYJuaJEsXdvGXrMA-pp8nqAf7Rgdt0g-LTfpBQSsybUd_Z6y6gYwI2HyivjNx3PywRrvqshEssHg2mlWPUseN9AGPLvbT5Mvb99cL9-n68t3q-X5OgVB8zEFXqICMDlWgpu6lqrAmuZ5Q2klCkUZVhnLeCGhUJUEqqJGNWCMLKTiqshOk9WeWzvY6sHbDvxP7cDqXcH5Gw1-tKZF3WSFNCJnFVAW-1WVKIXhAlHQgilKI-v1njVMVYe1wT4-uX0AfXjT26_6xt3qUslSUBYBL-8A3n2bMIy6s8Fg20KPbgqaq0zOS8y9FnsphI7rrZt8H79JM6rn9PUhfb1LX3MeDS_uD_dnqkPWUaD2gphGCB4bbXYpunlW2_4Xzf5yHuD_9vwGV4rT5A
CitedBy_id crossref_primary_10_3389_fvets_2024_1374803
crossref_primary_10_1016_j_aquaculture_2023_740455
crossref_primary_10_1038_s41564_024_01635_8
crossref_primary_10_1038_s42255_024_01065_0
crossref_primary_10_1016_j_onehlt_2024_100933
crossref_primary_10_1016_j_scitotenv_2023_165212
crossref_primary_10_1128_spectrum_00295_24
crossref_primary_10_1111_jfb_15650
Cites_doi 10.1128/AEM.00411-20
10.1128/mSystems.00095-16
10.3389/fmicb.2019.02576
10.3389/fmicb.2017.02043
10.1016/j.aquaculture.2018.12.037
10.1093/femsec/fix051
10.1016/j.fsigen.2014.12.001
10.1371/journal.pone.0061217
10.1111/j.2517-6161.1995.tb02031.x
10.5962/bhl.title.143318
10.1371/journal.pone.0170622
10.21203/rs.3.rs-29747/v1
10.1371/journal.pbio.3000298
10.1128/AEM.02692-09
10.1016/j.aqrep.2020.100309
10.32614/CRAN.package.rstatix
10.1128/AEM.02627-17
10.1371/journal.pcbi.1005404
10.1111/j.1365-2672.2012.05384.x
10.1128/mSystems.00218-17
10.1016/j.anaerobe.2009.04.009
10.1016/j.fsi.2018.11.079
10.1111/raq.12601
10.1371/journal.pone.0076096
10.1038/s41598-022-17008-2
10.1371/journal.pone.0053608
10.1371/journal.pone.0146064
10.1007/978-3-319-24277-4_12
10.3389/fmicb.2017.02664
10.1093/nar/gks1219
10.1128/AEM.01541-09
10.1128/AEM.00902-16
10.1016/s0167-7012(03)00024-1
10.1016/J.ENG.2017.01.020
10.1186/s12915-014-0087-z
10.1093/cid/ciy303
10.1016/j.aquaculture.2009.05.006
10.1128/JCM.39.2.485-493.2001
10.1111/jam.14969
10.1186/s40168-018-0426-3
10.1016/j.mimet.2015.07.003
10.1038/nbt.3601
10.1007/978-1-60327-353-4_4
10.1128/AEM.00063-18
ContentType Journal Article
Copyright Copyright © 2022 Clokie et al.
Copyright © 2022 Clokie et al. 2022 Clokie et al.
Copyright_xml – notice: Copyright © 2022 Clokie et al.
– notice: Copyright © 2022 Clokie et al. 2022 Clokie et al.
DBID AAYXX
CITATION
CGR
CUY
CVF
ECM
EIF
NPM
7X8
5PM
DOA
DOI 10.1128/spectrum.02255-22
DatabaseName CrossRef
Medline
MEDLINE
MEDLINE (Ovid)
MEDLINE
MEDLINE
PubMed
MEDLINE - Academic
PubMed Central (Full Participant titles)
DOAJ Directory of Open Access Journals
DatabaseTitle CrossRef
MEDLINE
Medline Complete
MEDLINE with Full Text
PubMed
MEDLINE (Ovid)
MEDLINE - Academic
DatabaseTitleList CrossRef

MEDLINE - Academic
MEDLINE
Database_xml – sequence: 1
  dbid: DOA
  name: DOAJ Directory of Open Access Journals
  url: https://www.doaj.org/
  sourceTypes: Open Website
– sequence: 2
  dbid: NPM
  name: PubMed
  url: https://proxy.k.utb.cz/login?url=http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed
  sourceTypes: Index Database
– sequence: 3
  dbid: EIF
  name: MEDLINE
  url: https://proxy.k.utb.cz/login?url=https://www.webofscience.com/wos/medline/basic-search
  sourceTypes: Index Database
DeliveryMethod fulltext_linktorsrc
Discipline Biology
Ecology
EISSN 2165-0497
Editor Khursigara, Cezar M.
Editor_xml – sequence: 1
  givenname: Cezar M.
  surname: Khursigara
  fullname: Khursigara, Cezar M.
ExternalDocumentID oai_doaj_org_article_f386c541ba014ebbb595c25ee5081700
PMC9769501
02255-22
36377933
10_1128_spectrum_02255_22
Genre Research Support, Non-U.S. Gov't
Journal Article
GrantInformation_xml – fundername: Fiskeri - og havbruksnæringens forskningsfond (FHF)
  grantid: 901514
  funderid: https://doi.org/10.13039/501100010197
– fundername: Newton-Musharafa Fund
  funderid: https://doi.org/10.13039/100010897
– fundername: ;
– fundername: ;
  grantid: 901514
GroupedDBID 53G
AAGFI
AAUOK
AAYXX
ADBBV
AGVNZ
ALMA_UNASSIGNED_HOLDINGS
CITATION
EJD
FF~
FRP
GROUPED_DOAJ
H13
M~E
OK1
RPM
RSF
CGR
CUY
CVF
ECM
EIF
NPM
UCJ
EBS
7X8
5PM
ID FETCH-LOGICAL-a504t-a29e7aac4eb52cdd678ed044f00b58701eb313286a87b6a07cdd7facc68672783
IEDL.DBID AAUOK
ISSN 2165-0497
IngestDate Wed Aug 27 00:42:29 EDT 2025
Thu Aug 21 18:40:03 EDT 2025
Fri Jul 11 02:56:41 EDT 2025
Wed Dec 21 20:55:14 EST 2022
Thu Jan 02 22:53:44 EST 2025
Tue Jul 01 00:42:41 EDT 2025
Thu Apr 24 23:05:57 EDT 2025
IsDoiOpenAccess true
IsOpenAccess true
IsPeerReviewed true
IsScholarly true
Issue 6
Keywords 16S rRNA
equicopy
gill
titration
low-biomass
complex
Language English
License This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license. https://creativecommons.org/licenses/by/4.0
This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license.
LinkModel DirectLink
MergedId FETCHMERGED-LOGICAL-a504t-a29e7aac4eb52cdd678ed044f00b58701eb313286a87b6a07cdd7facc68672783
Notes ObjectType-Article-1
SourceType-Scholarly Journals-1
ObjectType-Feature-2
content type line 23
Benjamin Gregory James Clokie and Ahmed Elsheshtawy contributed equally to this work. Author order is in order of increasing seniority.
The authors declare no conflict of interest.
ORCID 0000-0003-4692-4711
OpenAccessLink https://journals.asm.org/doi/10.1128/spectrum.02255-22
PMID 36377933
PQID 2736666650
PQPubID 23479
PageCount 12
ParticipantIDs doaj_primary_oai_doaj_org_article_f386c541ba014ebbb595c25ee5081700
pubmedcentral_primary_oai_pubmedcentral_nih_gov_9769501
proquest_miscellaneous_2736666650
asm2_journals_10_1128_spectrum_02255_22
pubmed_primary_36377933
crossref_citationtrail_10_1128_spectrum_02255_22
crossref_primary_10_1128_spectrum_02255_22
ProviderPackageCode CITATION
AAYXX
PublicationCentury 2000
PublicationDate 2022-12-21
PublicationDateYYYYMMDD 2022-12-21
PublicationDate_xml – month: 12
  year: 2022
  text: 2022-12-21
  day: 21
PublicationDecade 2020
PublicationPlace United States
PublicationPlace_xml – name: United States
– name: 1752 N St., N.W., Washington, DC
PublicationTitle Microbiology spectrum
PublicationTitleAbbrev Microbiol Spectr
PublicationTitleAlternate Microbiol Spectr
PublicationYear 2022
Publisher American Society for Microbiology
Publisher_xml – name: American Society for Microbiology
References e_1_3_3_17_2
e_1_3_3_16_2
e_1_3_3_19_2
e_1_3_3_38_2
e_1_3_3_18_2
e_1_3_3_39_2
e_1_3_3_36_2
e_1_3_3_12_2
e_1_3_3_37_2
e_1_3_3_15_2
e_1_3_3_34_2
e_1_3_3_14_2
e_1_3_3_35_2
e_1_3_3_32_2
e_1_3_3_33_2
e_1_3_3_11_2
e_1_3_3_30_2
e_1_3_3_10_2
e_1_3_3_31_2
e_1_3_3_40_2
Wen Y (e_1_3_3_13_2) 2016; 8
e_1_3_3_6_2
e_1_3_3_5_2
e_1_3_3_8_2
e_1_3_3_7_2
e_1_3_3_28_2
e_1_3_3_9_2
e_1_3_3_27_2
e_1_3_3_29_2
e_1_3_3_24_2
e_1_3_3_47_2
e_1_3_3_23_2
e_1_3_3_48_2
e_1_3_3_26_2
e_1_3_3_45_2
e_1_3_3_25_2
e_1_3_3_46_2
e_1_3_3_2_2
e_1_3_3_20_2
e_1_3_3_43_2
e_1_3_3_44_2
e_1_3_3_4_2
e_1_3_3_22_2
e_1_3_3_41_2
e_1_3_3_3_2
e_1_3_3_21_2
e_1_3_3_42_2
Reverter, M, Sasal, P, Tapissier-Bontemps, N, Lecchini, D, Suzuki, M (B24) 2017; 93
Salter, SJ, Cox, MJ, Turek, EM, Calus, ST, Cookson, WO, Moffatt, MF, Turner, P, Parkhill, J, Loman, NJ, Walker, AW (B8) 2014; 12
B44
B45
Gohl, DM, Vangay, P, Garbe, J, MacLean, A, Hauge, A, Becker, A, Gould, TJ, Clayton, JB, Johnson, TJ, Hunter, R, Knights, D, Beckman, KB (B9) 2016; 34
Benjamini, Y, Hochberg, Y (B43) 1995; 57
Al-Soud, WA, Rådström, P (B31) 2001; 39
Arenz, BE, Schlatter, DC, Bradeen, JM, Kinkel, LL (B16) 2015; 117
Urakawa, H, Martens-Habbena, W, Stahl, DA (B32) 2010; 76
Thoendel, MJ, Jeraldo, PR, Greenwood-Quaintance, KE, Yao, JZ, Chia, N, Hanssen, AD, Abdel, MP, Patel, R (B14) 2018; 67
Pratte, ZA, Besson, M, Hollman, RD, Stewart, FJ (B21) 2018; 84
Zhang, Z, Li, D, Xu, W, Tang, R, Li, L (B22) 2019; 10
Steinum, T, Sjåstad, K, Falk, K, Kvellestad, A, Colquhoun, DJ (B27) 2009; 293
Schmidt, V, Amaral-Zettler, L, Davidson, J, Summerfelt, S, Good, C (B3) 2016; 82
Minich, JJ, Zhu, Q, Janssen, S, Hendrickson, R, Amir, A, Vetter, R, Hyde, J, Doty, MM, Stillwell, K, Benardini, J, Kim, JH, Allen, EE, Venkateswaran, K, Knight, R (B29) 2018; 3
Hansen, WL, Bruggeman, CA, Wolffs, PF (B13) 2013; 943
Feehery, GR, Yigit, E, Oyola, SO, Langhorst, BW, Schmidt, VT, Stewart, FJ, Dimalanta, ET, Amaral-Zettler, LA, Davis, T, Quail, MA, Pradhan, S (B17) 2013; 8
Birlanga, V, McCormack, G, Ijaz, U, McCarthy, E, Smith, C, Collins, G (B2) 2020; 12
Wen, Y, Xiao, F, Wang, C, Wang, Z (B12) 2016; 8
Minich, JJ, Poore, GD, Jantawongsri, K, Johnston, C, Bowie, K, Bowman, J, Knight, R, Nowak, B, Allen, EE (B1) 2020; 86
Xu, J, Ma, B, Su, X, Huang, S, Xu, X, Zhou, X, Huang, WE, Knight, R (B5) 2017; 3
Schloss, PD, Westcott, SL, Ryabin, T, Hall, JR, Hartmann, M, Hollister, EB, Lesniewski, RA, Oakley, BB, Parks, DH, Robinson, CJ, Sahl, JW, Stres, B, Thallinger, GG, Van Horn, DJ, Weber, CF (B39) 2009; 75
Horz, H-P, Scheer, S, Vianna, ME, Conrads, G (B15) 2010; 16
Schrader, C, Schielke, A, Ellerbroek, L, Johne, R (B30) 2012; 113
Pollock, J, Glendinning, L, Wisedchanwet, T, Watson, M (B26) 2018; 84
Birlanga, VB, McCormack, G, Ijaz, UZ, McCarthy, E, Smith, C, Collins, G (B34) 2020
Marotz, CA, Sanders, JG, Zuniga, C, Zaramela, LS, Knight, R, Zengler, K (B11) 2018; 6
Wickham, H (B46) 2016
Legrand, TPRA, Catalano, SR, Wos-Oxley, ML, Stephens, F, Landos, M, Bansemer, MS, Stone, DAJ, Qin, JG, Oxley, APA (B25) 2017; 8
Knudsen, BE, Bergmark, L, Munk, P, Lukjancenko, O, Priemé, A, Aarestrup, FM, Pamp, SJ (B7) 2016; 1
Brown, RM, Wiens, GD, Salinas, I (B19) 2019; 86
Wang, M, Yi, M, Lu, M, Gao, F, Liu, Z, Huang, Q, Li, Q, Zhu, D (B23) 2020; 17
Longmire, JL, Maltbie, M, Baker, RJ (B38) 1997
Slinger, J, Adams, MB, Wynne, JW (B37) 2021; 131
Foster, ZS, Sharpton, TJ, Grünwald, NJ (B47) 2017; 13
Sieber, M, Pita, L, Weiland-Bräuer, N, Dirksen, P, Wang, J, Mortzfeld, B, Franzenburg, S, Schmitz, RA, Baines, JF, Fraune, S, Hentschel, U, Schulenburg, H, Bosch, TCG, Traulsen, A (B28) 2019; 17
Bastos Gomes, G, Hutson, KS, Domingos, JA, Infante Villamil, S, Huerlimann, R, Miller, TL, Jerry, DR (B20) 2019; 502
Quast, C, Pruesse, E, Yilmaz, P, Gerken, J, Schweer, T, Yarza, P, Peplies, J, Glöckner, FO (B41) 2013; 41
McMurdie, PJ, Holmes, S (B42) 2013; 8
Minniti, G, Hagen, LH, Porcellato, D, Jørgensen, SM, Pope, PB, Vaaje-Kolstad, G (B36) 2017; 8
Mizrahi-Man, O, Davenport, ER, Gilad, Y (B10) 2013; 8
Barreto, MO, Rey Planellas, S, Yang, Y, Phillips, C, Descovich, K (B4) 2020; 14
Liu, G, Weston, CQ, Pham, LK, Waltz, S, Barnes, H, King, P, Sphar, D, Yamamoto, RT, Forsyth, RA (B18) 2016; 11
Hu, Q, Liu, Y, Yi, S, Huang, D (B33) 2015; 16
Cox, MJ, Turek, EM, Hennessy, C, Mirza, GK, James, PL, Coleman, M, Jones, A, Wilson, R, Bilton, D, Cookson, WOC, Moffatt, MF, Loebinger, MR (B35) 2017; 12
Greene, EA, Voordouw, G (B6) 2003; 53
B40
References_xml – ident: e_1_3_3_2_2
  doi: 10.1128/AEM.00411-20
– ident: e_1_3_3_8_2
  doi: 10.1128/mSystems.00095-16
– ident: e_1_3_3_23_2
  doi: 10.3389/fmicb.2019.02576
– ident: e_1_3_3_37_2
  doi: 10.3389/fmicb.2017.02043
– ident: e_1_3_3_21_2
  doi: 10.1016/j.aquaculture.2018.12.037
– ident: e_1_3_3_25_2
  doi: 10.1093/femsec/fix051
– ident: e_1_3_3_34_2
  doi: 10.1016/j.fsigen.2014.12.001
– ident: e_1_3_3_43_2
  doi: 10.1371/journal.pone.0061217
– ident: e_1_3_3_44_2
  doi: 10.1111/j.2517-6161.1995.tb02031.x
– ident: e_1_3_3_39_2
  doi: 10.5962/bhl.title.143318
– ident: e_1_3_3_36_2
  doi: 10.1371/journal.pone.0170622
– ident: e_1_3_3_35_2
  doi: 10.21203/rs.3.rs-29747/v1
– ident: e_1_3_3_29_2
  doi: 10.1371/journal.pbio.3000298
– ident: e_1_3_3_33_2
  doi: 10.1128/AEM.02692-09
– ident: e_1_3_3_24_2
  doi: 10.1016/j.aqrep.2020.100309
– ident: e_1_3_3_45_2
  doi: 10.32614/CRAN.package.rstatix
– ident: e_1_3_3_27_2
  doi: 10.1128/AEM.02627-17
– ident: e_1_3_3_48_2
  doi: 10.1371/journal.pcbi.1005404
– volume: 8
  start-page: 1412
  year: 2016
  ident: e_1_3_3_13_2
  article-title: The impact of different methods of DNA extraction on microbial community measures of BALF samples based on metagenomic data
  publication-title: Am J Transl Res
– ident: e_1_3_3_31_2
  doi: 10.1111/j.1365-2672.2012.05384.x
– ident: e_1_3_3_30_2
  doi: 10.1128/mSystems.00218-17
– ident: e_1_3_3_16_2
  doi: 10.1016/j.anaerobe.2009.04.009
– ident: e_1_3_3_20_2
  doi: 10.1016/j.fsi.2018.11.079
– ident: e_1_3_3_5_2
  doi: 10.1111/raq.12601
– ident: e_1_3_3_18_2
  doi: 10.1371/journal.pone.0076096
– ident: e_1_3_3_3_2
  doi: 10.1038/s41598-022-17008-2
– ident: e_1_3_3_11_2
  doi: 10.1371/journal.pone.0053608
– ident: e_1_3_3_19_2
  doi: 10.1371/journal.pone.0146064
– ident: e_1_3_3_47_2
  doi: 10.1007/978-3-319-24277-4_12
– ident: e_1_3_3_26_2
  doi: 10.3389/fmicb.2017.02664
– ident: e_1_3_3_41_2
– ident: e_1_3_3_42_2
  doi: 10.1093/nar/gks1219
– ident: e_1_3_3_40_2
  doi: 10.1128/AEM.01541-09
– ident: e_1_3_3_4_2
  doi: 10.1128/AEM.00902-16
– ident: e_1_3_3_7_2
  doi: 10.1016/s0167-7012(03)00024-1
– ident: e_1_3_3_6_2
  doi: 10.1016/J.ENG.2017.01.020
– ident: e_1_3_3_9_2
  doi: 10.1186/s12915-014-0087-z
– ident: e_1_3_3_15_2
  doi: 10.1093/cid/ciy303
– ident: e_1_3_3_28_2
  doi: 10.1016/j.aquaculture.2009.05.006
– ident: e_1_3_3_32_2
  doi: 10.1128/JCM.39.2.485-493.2001
– ident: e_1_3_3_38_2
  doi: 10.1111/jam.14969
– ident: e_1_3_3_46_2
– ident: e_1_3_3_12_2
  doi: 10.1186/s40168-018-0426-3
– ident: e_1_3_3_17_2
  doi: 10.1016/j.mimet.2015.07.003
– ident: e_1_3_3_10_2
  doi: 10.1038/nbt.3601
– ident: e_1_3_3_14_2
  doi: 10.1007/978-1-60327-353-4_4
– ident: e_1_3_3_22_2
  doi: 10.1128/AEM.00063-18
– volume: 14
  start-page: 343
  year: 2020
  end-page: 361
  ident: B4
  article-title: Emerging indicators of fish welfare in aquaculture
  publication-title: Rev Aquaculture
  doi: 10.1111/raq.12601
– volume: 86
  year: 2020
  ident: B1
  article-title: Microbial ecology of Atlantic salmon, Salmo salar, hatcheries: impacts of the built environment on fish mucosal microbiota
  publication-title: Appl Environ Microbiol
  doi: 10.1128/AEM.00411-20
– volume: 117
  start-page: 1
  year: 2015
  end-page: 3
  ident: B16
  article-title: Blocking primers reduce co-amplification of plant DNA when studying bacterial endophyte communities
  publication-title: J Microbiol Methods
  doi: 10.1016/j.mimet.2015.07.003
– volume: 8
  start-page: 2664
  year: 2017
  ident: B25
  article-title: The inner workings of the outer surface: skin and gill microbiota as indicators of changing gut health in yellowtail kingfish
  publication-title: Front Microbiol
  doi: 10.3389/fmicb.2017.02664
– volume: 67
  start-page: 1333
  year: 2018
  end-page: 1338
  ident: B14
  article-title: Identification of prosthetic joint infection pathogens using a shotgun metagenomics approach
  publication-title: Clin Infect Dis
  doi: 10.1093/cid/ciy303
– volume: 3
  year: 2018
  ident: B29
  article-title: KatharoSeq enables high-throughput microbiome analysis from low-biomass samples
  publication-title: mSystems
  doi: 10.1128/mSystems.00218-17
– volume: 75
  start-page: 7537
  year: 2009
  end-page: 7541
  ident: B39
  article-title: Introducing mothur: open-source, platform-independent, community-supported software for describing and comparing microbial communities
  publication-title: Appl Environ Microbiol
  doi: 10.1128/AEM.01541-09
– volume: 3
  start-page: 66
  year: 2017
  end-page: 70
  ident: B5
  article-title: Emerging trends for microbiome analysis: from single-cell functional imaging to microbiome big data
  publication-title: Engineering
  doi: 10.1016/J.ENG.2017.01.020
– volume: 943
  start-page: 81
  year: 2013
  end-page: 90
  ident: B13
  article-title: Pre-analytical sample treatment and DNA extraction protocols for the detection of bacterial pathogens from whole blood
  publication-title: Methods Mol Biol
  doi: 10.1007/978-1-60327-353-4_4
– volume: 8
  start-page: 2043
  year: 2017
  ident: B36
  article-title: The skin-mucus microbial community of farmed Atlantic salmon (Salmo salar)
  publication-title: Front Microbiol
  doi: 10.3389/fmicb.2017.02043
– volume: 131
  start-page: 80
  year: 2021
  end-page: 92
  ident: B37
  article-title: Comparison of bacterial diversity and distribution on the gills of Atlantic salmon (Salmo salar L.): an evaluation of sampling techniques
  publication-title: J Appl Microbiol
  doi: 10.1111/jam.14969
– volume: 16
  start-page: 47
  year: 2010
  end-page: 53
  ident: B15
  article-title: New methods for selective isolation of bacterial DNA from human clinical specimens
  publication-title: Anaerobe
  doi: 10.1016/j.anaerobe.2009.04.009
– volume: 86
  start-page: 497
  year: 2019
  end-page: 506
  ident: B19
  article-title: Analysis of the gut and gill microbiome of resistant and susceptible lines of rainbow trout (Oncorhynchus mykiss)
  publication-title: Fish Shellfish Immunol
  doi: 10.1016/j.fsi.2018.11.079
– volume: 82
  start-page: 4470
  year: 2016
  end-page: 4481
  ident: B3
  article-title: Influence of fishmeal-free diets on microbial communities in Atlantic salmon (Salmo salar) recirculation aquaculture systems
  publication-title: Appl Environ Microbiol
  doi: 10.1128/AEM.00902-16
– volume: 17
  year: 2019
  ident: B28
  article-title: Neutrality in the metaorganism
  publication-title: PLoS Biol
  doi: 10.1371/journal.pbio.3000298
– volume: 1
  year: 2016
  ident: B7
  article-title: Impact of sample type and DNA isolation procedure on genomic inference of microbiome composition
  publication-title: mSystems
  doi: 10.1128/mSystems.00095-16
– volume: 12
  year: 2017
  ident: B35
  article-title: Longitudinal assessment of sputum microbiome by sequencing of the 16S rRNA gene in non-cystic fibrosis bronchiectasis patients
  publication-title: PLoS One
  doi: 10.1371/journal.pone.0170622
– volume: 53
  start-page: 211
  year: 2003
  end-page: 219
  ident: B6
  article-title: Analysis of environmental microbial communities by reverse sample genome probing
  publication-title: J Microbiol Methods
  doi: 10.1016/s0167-7012(03)00024-1
– volume: 84
  year: 2018
  ident: B26
  article-title: The madness of microbiome: attempting to find consensus “best practice” for 16S microbiome studies
  publication-title: Appl Environ Microbiol
  doi: 10.1128/AEM.02627-17
– volume: 41
  start-page: D590
  year: 2013
  end-page: D596
  ident: B41
  article-title: The SILVA ribosomal RNA gene database project: improved data processing and web-based tools
  publication-title: Nucleic Acids Res
  doi: 10.1093/nar/gks1219
– volume: 12
  start-page: 87
  year: 2014
  ident: B8
  article-title: Reagent and laboratory contamination can critically impact sequence-based microbiome analyses
  publication-title: BMC Biol
  doi: 10.1186/s12915-014-0087-z
– volume: 84
  year: 2018
  ident: B21
  article-title: The gills of reef fish support a distinct microbiome influenced by host-specific factors
  publication-title: Appl Environ Microbiol
  doi: 10.1128/AEM.00063-18
– volume: 39
  start-page: 485
  year: 2001
  end-page: 493
  ident: B31
  article-title: Purification and characterization of PCR-inhibitory components in blood cells
  publication-title: J Clin Microbiol
  doi: 10.1128/JCM.39.2.485-493.2001
– year: 2020
  ident: B34
  article-title: Dynamic gill and mucous microbiomes track an amoebic gill disease episode in farmed Atlantic salmon
  publication-title: Res Square
  doi: 10.21203/rs.3.rs-29747/v1
– ident: B44
  article-title: Kassambara A . 2020 . RSTATIX: Pipe-friendly framework for basic statistical test . https://rpkgsdatanoviacom/rstatix/ . Accessed 27 April 2021 .
– volume: 11
  year: 2016
  ident: B18
  article-title: Epigenetic segregation of microbial genomes from complex samples using restriction endonucleases HpaII and McrB
  publication-title: PLoS One
  doi: 10.1371/journal.pone.0146064
– ident: B40
  article-title: Schloss PD . 2019 . MiSeq SOP . https://mothur.org/wiki/ . Accessed 1 July 2020 .
– volume: 8
  start-page: 1412
  year: 2016
  end-page: 1425
  ident: B12
  article-title: The impact of different methods of DNA extraction on microbial community measures of BALF samples based on metagenomic data
  publication-title: Am J Transl Res
– year: 1997
  ident: B38
  publication-title: Use of' lysis buffer” in DNA isolation and its implication for museum collections. ;Museum of Texas Tech University ;Lubbock, TX
– ident: B45
  article-title: Oksanen J , Blanchet FG , Kindt R , Legendre P , Minchin PR , O’hara R , Simpson GL , Solymos P , Stevens MHH , Wagner H . 2013 . Vegan: community ecology package, version 2 . https://github.com/vegandevs/vegan/ .
– volume: 17
  start-page: 100309
  year: 2020
  ident: B23
  article-title: Effects of probiotics Bacillus cereus NY5 and Alcaligenes faecalis Y311 used as water additives on the microbiota and immune enzyme activities in three mucosal tissues in Nile tilapia Oreochromis niloticus reared in outdoor tanks
  publication-title: Aquaculture Rep
  doi: 10.1016/j.aqrep.2020.100309
– volume: 502
  start-page: 196
  year: 2019
  end-page: 201
  ident: B20
  article-title: Parasitic protozoan interactions with bacterial microbiome in a tropical fish farm
  publication-title: Aquaculture
  doi: 10.1016/j.aquaculture.2018.12.037
– start-page: 241
  year: 2016
  end-page: 253
  ident: B46
  publication-title: ggplot2: elegant graphics for data analysis ;Springer International Publishing ;Cham, Switzerland
  doi: 10.1007/978-3-319-24277-4_12
– volume: 57
  start-page: 289
  year: 1995
  end-page: 300
  ident: B43
  article-title: Controlling the false discovery rate: a practical and powerful approach to multiple testing
  publication-title: J R Stat Soc B Stat Methodol
  doi: 10.1111/j.2517-6161.1995.tb02031.x
– volume: 8
  year: 2013
  ident: B10
  article-title: Taxonomic classification of bacterial 16S rRNA genes using short sequencing reads: evaluation of effective study designs
  publication-title: PLoS One
  doi: 10.1371/journal.pone.0053608
– volume: 12
  start-page: 16719
  year: 2020
  ident: B2
  article-title: Dynamic gill and mucous microbiomes track an amoebic gill disease episode in farmed Atlantic salmon
  publication-title: Sci Rep
  doi: 10.1038/s41598-022-17008-2
– volume: 113
  start-page: 1014
  year: 2012
  end-page: 1026
  ident: B30
  article-title: PCR inhibitors–occurrence, properties and removal
  publication-title: J Appl Microbiol
  doi: 10.1111/j.1365-2672.2012.05384.x
– volume: 93
  year: 2017
  ident: B24
  article-title: Characterisation of the gill mucosal bacterial communities of four butterflyfish species: a reservoir of bacterial diversity in coral reef ecosystems
  publication-title: FEMS Microbiol Ecol
  doi: 10.1093/femsec/fix051
– volume: 13
  year: 2017
  ident: B47
  article-title: Metacoder: an R package for visualization and manipulation of community taxonomic diversity data
  publication-title: PLoS Comput Biol
  doi: 10.1371/journal.pcbi.1005404
– volume: 10
  start-page: 2576
  year: 2019
  ident: B22
  article-title: Microbiome of co-cultured fish exhibits host selection and niche differentiation at the organ scale
  publication-title: Front Microbiol
  doi: 10.3389/fmicb.2019.02576
– volume: 8
  year: 2013
  ident: B17
  article-title: A method for selectively enriching microbial DNA from contaminating vertebrate host DNA
  publication-title: PLoS One
  doi: 10.1371/journal.pone.0076096
– volume: 293
  start-page: 172
  year: 2009
  end-page: 179
  ident: B27
  article-title: An RT PCR-DGGE survey of gill-associated bacteria in Norwegian seawater-reared Atlantic salmon suffering proliferative gill inflammation
  publication-title: Aquaculture
  doi: 10.1016/j.aquaculture.2009.05.006
– volume: 76
  start-page: 2129
  year: 2010
  end-page: 2135
  ident: B32
  article-title: High abundance of ammonia-oxidizing Archaea in coastal waters, determined using a modified DNA extraction method
  publication-title: Appl Environ Microbiol
  doi: 10.1128/AEM.02692-09
– volume: 8
  year: 2013
  ident: B42
  article-title: phyloseq: an R package for reproducible interactive analysis and graphics of microbiome census data
  publication-title: PLoS One
  doi: 10.1371/journal.pone.0061217
– volume: 6
  start-page: 42
  year: 2018
  end-page: 42
  ident: B11
  article-title: Improving saliva shotgun metagenomics by chemical host DNA depletion
  publication-title: Microbiome
  doi: 10.1186/s40168-018-0426-3
– volume: 16
  start-page: 94
  year: 2015
  end-page: 97
  ident: B33
  article-title: A comparison of four methods for PCR inhibitor removal
  publication-title: Forensic Sci Int Genet
  doi: 10.1016/j.fsigen.2014.12.001
– volume: 34
  start-page: 942
  year: 2016
  end-page: 949
  ident: B9
  article-title: Systematic improvement of amplicon marker gene methods for increased accuracy in microbiome studies
  publication-title: Nat Biotechnol
  doi: 10.1038/nbt.3601
SSID ssj0001105252
Score 2.303085
Snippet The interaction between the fish gill and surrounding bacteria-rich water provides an intriguing model for examining the interaction between the fish,...
The major aquatic interface between host and environment in teleost finfish species is the gill. The diversity of this infraclass, high complexity of the...
ABSTRACT The major aquatic interface between host and environment in teleost finfish species is the gill. The diversity of this infraclass, high complexity of...
SourceID doaj
pubmedcentral
proquest
asm2
pubmed
crossref
SourceType Open Website
Open Access Repository
Aggregation Database
Index Database
Enrichment Source
StartPage e0225522
SubjectTerms 16S rRNA
Animals
Bacteria - genetics
Biomass
complex
DNA Contamination
DNA, Bacterial - genetics
Ecology
equicopy
Fishes - genetics
gill
low-biomass
Microbiota - genetics
Polymerase Chain Reaction - methods
Research Article
RNA, Ribosomal, 16S - genetics
titration
SummonAdditionalLinks – databaseName: DOAJ Directory of Open Access Journals
  dbid: DOA
  link: http://utb.summon.serialssolutions.com/2.0.0/link/0/eLvHCXMwrV3daxQxEA9yIPgifnt-EUEQhNgkm2Szj22xVLFV-wF9C0k2wQN3T3o91P_emezecSdSX9zH3QkbJjOZXz7mN4S8CqYKlmvLcjaaKSsUAxTCmQ2Jp1babEuG3NGxOTxXHy70xUapL7wTNtADD4rbyZU1USsRPID5FELQjY5SpwTIArnlcPaFmLexmCq7KwLrs8nxGBPm4J2SuHi57N5C0NKaYbHciV90ciseFdr-v2HNP69MbsSggzvk9gge6e7Q6bvkRurvkZtDOclf98nPT-D_3ZhYSeeZfpz_YPC1A4BMTz3yANOyUVByGajvW_pl6fuSZgaTHv28f8L2IKq19Gw2sunS9yWLkgpzSi9Pjnfp0WxgbuoSxZ3_wW4fkPODd2f7h2ysrMC85uqKedmk2vsICtUyti1ErNRypTLnQYMHC1hiwzLVGm_rYDyvQabOPkZj8eTWVg_JpJ_36TGhCvUpZKxMrVTlRYh1KxqYJ2yMOTd8Sl6jmt3oGgtXVh3SutWAuDIgTsop4auRcHEkKMc6Gd-ua_Jm3eT7wM5xnfAeDu9aEIm1ywswNzeam_uXuU3Jy5VxOHBEPF3xfZovFw5woMFHg8yjwVjWv6oM8jpW1ZTUW2a01ZftL_3sayH7BrjYaC6e_I_OPyW3JGZvCMmkeEYmoJ70HDDVVXhR3Oc3f8Mf6w
  priority: 102
  providerName: Directory of Open Access Journals
Title Optimization of Low-Biomass Sample Collection and Quantitative PCR-Based Titration Impact 16S rRNA Microbiome Resolution
URI https://www.ncbi.nlm.nih.gov/pubmed/36377933
https://journals.asm.org/doi/10.1128/spectrum.02255-22
https://www.proquest.com/docview/2736666650
https://pubmed.ncbi.nlm.nih.gov/PMC9769501
https://doaj.org/article/f386c541ba014ebbb595c25ee5081700
Volume 10
hasFullText 1
inHoldings 1
isFullTextHit
isPrint
link http://utb.summon.serialssolutions.com/2.0.0/link/0/eLvHCXMwjV3ta9QwGA_jhuAX8d1zOiIIgpCZpEmafryNjfmyTbcd7FtI0hQPbG_sduj-e5-k6enJGPZTaZ7Qkuc9T59fEHrrVOE0lZo0jZJEaCYIRCGUaBdoqLludOqQOzpWh1Px6UJebCA19MLkFVzs2EWbCvkrzeb6Q2o-vFq2O-B4pCQcTO-m5JWgI7Q5mUxPPv_ZXWHxfDaey5i3zgUbDO_ga_4owfbfFmv--8vkXz7o4CF6kINHPOm5_QhthO4xutcfJ3kDd_sJgvrmCfp1ApagzS2WeN7gL_OfBOhaCJXxmY2IwDhtGaSuBmy7Gn9b2i41nIH5w1_3Tsku-Lcan88yri7-mPopMVNn-Or0eIKPZj2GUxtwrAH0EvwUTQ_2z_cOST5jgVhJxTWxvAqltV4EJ7mva_BdoaZCNJQ6CbrMINmGhFUrq0unLC2Bpmys90rHGq4unqFRN-_CC4RFXFnGfaFKIQrLnC9rVoHF0N43TUXH6F1ccDOw2KT8g2szsMYk1hjOx4gOPDE-Q5XHEzN-3DXl_WrKZY_TcRfxbmT0ijBCbKcHIHAma6xpCq28FMxZyCKDc05W0nMZAoS0EdRwjN4MYmJAJWOdxXZhvlwYiAhVvCTQPO_FZvWqQkWEx6IYo3JNoNa-ZX2km31PsN8QOFaSspf_vYxb6D6PzRqME85eoREMhtcQQl277awv22kL4jcF5xuu
linkProvider American Society for Microbiology
linkToHtml http://utb.summon.serialssolutions.com/2.0.0/link/0/eLvHCXMwjV3da9swEBejZWwvY9_NPjUYDAbqJFmSlce0tKRrkm5tAn0TkiyzjMYZTcPW_34nWcmWUcr8ZOwTNrpP6XS_Q-i9U4XTVGpS10oSoZkgEIVQol2goeK61qlCbjhS_Yn4fC7P86nKWAvzPfblvVjs2sUs5fGjYseN6NyPUH9KBYiXy9kuOB8pCQfzux1zhyDd273e5OT4zw4Liz3aeE5l3jgW7DB8iG_4pATdf1O8-e-xyb_80OFD9CAHkLjXcvwRuhOax-hu21LyGu4OEgz19RP06wSswSyXWeJ5jQfznwToZhAu4zMbUYFx2jZIlQ3YNhX-urRNKjoDE4i_7J-SPfBxFR5PM7YuPko1lZipM3x5Ourh4bTFcZoFHPMArRQ_RZPDg_F-n-Q-C8RKKq6I5d1QWutFcJL7qgL_FSoqRE2pk6DPDBbcsGjVyurSKUtLoClr673SMY-ri2doq5k3YQdhEWeWcV-oUojCMufLinXBamjv67pLO-hDnHCTFWVh0hqEa7NijUmsMZx3EF3xxPgMVx67ZlzcNuTjesiPFqvjNuK9yOg1YYTZTg9A6kzWWlMXWnkpmLOwkgzOOdmVnssQIKyNwIYd9G4lJgbUMuZabBPmy4WBqFDFSwLN81Zs1p8qVER5LIoOKjcEauNfNt80028J-huCx66k7MV_T-NbdK8_Hg7M4Gh0_BLd57F4g3HC2Su0BYThNYRUV-5N1p3fIT4fHA
linkToPdf http://utb.summon.serialssolutions.com/2.0.0/link/0/eLvHCXMwjV3da9swEBejZWMvY99Luw8NBoOBOkmWZOUx7RratU27toG-CUmWWWB2StOw9b_fSVayZZQyPxn7hI3uUzrd7xD64FThNJWa1LWSRGgmCEQhlGgXaKi4rnWqkDsaqb2x-HohL_KpylgLk2dwtmVnTUrkR82-rOrcj1B_TgWIV_NmC5yPlISD-V2PySqQ8fXBYHx88GeHhcUebTynMm8dC3YYvsNXfFKC7r8t3vz32ORffmj4GD3KASQedBx_gu6F9im637WUvIG73QRDffMM_ToGa9DkMks8rfHh9CcBugbCZXxmIyowTtsGqbIB27bC3-a2TUVnYALxyc4p2QYfV-HzScbWxfupphIzdYavTkcDfDTpcJyagGMeoJPi52g83D3f2SO5zwKxkoprYnk_lNZ6EZzkvqrAf4WKClFT6iToM4MFNyxatbK6dMrSEmjK2nqvdMzj6uIFWmunbXiFsIgzy7gvVClEYZnzZcX6YDW093Xdpz30MU64WbDZpDUI12bBGpNYYzjvIbrgifEZrjx2zfhx15BPyyGXHVbHXcTbkdFLwgiznR6A0JmstaYutPJSMGdhJRmcc7IvPZchQFgbgQ176P1CTAyoZcy12DZM5zMDUaGKlwSal53YLD9VqIjyWBQ9VK4I1Mq_rL5pJ98T9DcEj31J2cZ_T-M79ODky9Ac7o8ONtFDHms3GCecvUZrQBfeQER17d5m1fkN44AeuA
openUrl ctx_ver=Z39.88-2004&ctx_enc=info%3Aofi%2Fenc%3AUTF-8&rfr_id=info%3Asid%2Fsummon.serialssolutions.com&rft_val_fmt=info%3Aofi%2Ffmt%3Akev%3Amtx%3Ajournal&rft.genre=article&rft.atitle=Optimization+of+Low-Biomass+Sample+Collection+and+Quantitative+PCR-Based+Titration+Impact+16S+rRNA+Microbiome+Resolution&rft.jtitle=Microbiology+spectrum&rft.au=Clokie%2C+Benjamin+Gregory+James&rft.au=Elsheshtawy%2C+Ahmed&rft.au=Albalat%2C+Amaya&rft.au=Nylund%2C+Are&rft.date=2022-12-21&rft.issn=2165-0497&rft.eissn=2165-0497&rft.volume=10&rft.issue=6&rft.spage=e0225522&rft_id=info:doi/10.1128%2Fspectrum.02255-22&rft.externalDBID=NO_FULL_TEXT
thumbnail_l http://covers-cdn.summon.serialssolutions.com/index.aspx?isbn=/lc.gif&issn=2165-0497&client=summon
thumbnail_m http://covers-cdn.summon.serialssolutions.com/index.aspx?isbn=/mc.gif&issn=2165-0497&client=summon
thumbnail_s http://covers-cdn.summon.serialssolutions.com/index.aspx?isbn=/sc.gif&issn=2165-0497&client=summon