User:Cchellard/Viral metagenomics
This is the sandbox page where you will draft your initial Wikipedia contribution.
If you're starting a new article, you can develop it here until it's ready to go live. If you're working on improvements to an existing article, copy only one section at a time of the article to this sandbox to work on, and be sure to use an edit summary linking to the article you copied from. Do not copy over the entire article. You can find additional instructions here. Remember to save your work regularly using the "Publish page" button. (It just means 'save'; it will still be in the sandbox.) You can add bold formatting to your additions to differentiate them from existing content. |
Article Draft
[edit]Viral metagenomics is the study of viral genetic material obtained from environmental DNA samples instead of a host or natural reservoir[1]. Metagenomic methods can be applied to study viruses in any system and has been used to describe various viruses associated with cancerous tumors, extreme environments, terrestrial ecosystems, and the blood and feces of humans[2]. The term virome is also used to refer to viruses investigated by metagenomic sequencing of viral nucleic acids and is frequently used to describe environmental shotgun metagenomes[3][4]. Viral metagenomics is a culture independent methodology that provides insights on viral diversity, abundance, and functional potential of viruses within the environment [1]. Viruses lack a universal phylogenetic marker making metagenomics the only way to assess the genetic diversity of viruses in an environmental sample . With the advancements of techniques that can exploit next-generation sequencing, viruses can now be studied outside of culturable virus-host pairs [1]. This approach has created improvements in molecular epidemiology and accelerated the discovery of novel viruses[5][6].
History
[edit]The term metagenomics was coined in 1998, with the first viral metagenomic study reported a few years later describing uncultured near shore viral communities using shotgun sequencing[2]. The earliest metagenomic studies of viruses were performed using ocean samples, and found that most of the sequenced DNA and RNA viruses had no matches in Virus databases[7][8]. The researchers also found that previously overlooked ssDNA viruses and prophages are major constituents in some marine environments. Subsequent studies of the soil virome discovered that bacteriophages were equally as prevalent as bacteria in the soil[9]. Acknowledging the importance of viral metagenomics, the International Committee on Taxonomy of Viruses (ICTV) recognizes that genomes assembled from metagenomic data represent a virus and can be classified using the same procedures for viruses isolated via classical virology approaches[10].
The IMG/VR system and the IMG/VR v.2.0 are the largest interactive public virus databases with over 760,000 metagenomic viral sequences and isolate viruses and serves as a starting point for the sequence analysis of viral fragments derived from metagenomic samples[11][12].
The Global Virome Project
[edit]The Global Virome Project (GVP) is an American-led international collaborative research initiative based at the One Health Institute at the University of California, Davis.[13][14] The project was co-launched by EcoHealth Alliance president Peter Daszak, Nathan Wolfe and Edward Rubin of Metabiota, and former Chinese Center for Disease Control and Prevention director George F. Gao.[15]
The goal of the Global Virome Project (GVP) is to identify and prevent future virus outbreaks.[16] The GVP is centered on the massive collection and sequencing of the planet’s unknown viruses, with an estimated 1.6 million viral species yet to be discovered in mammal and bird populations. Of these, 631,000 to 827,000 have zoonotic potential[16]. The cost of identifying these unidentified viruses is a major limitation of the GVP, with a total cost estimate of $1.2 billion. That being said, preventing an outbreak is still less costly than reacting to one, with the total estimated cost of the ongoing COVID-19 pandemic estimated at more than $16 trillion[17].The Global Virome project also aims to boost infectious disease surveillance around the globe by using low cost sequencing methods in high risk countries to prevent disease outbreaks by expanding on the efforts of the USAID (agency for international development) EPT (Emerging Pandemic Threats) PREDICT project. The PREDICT project was founded to discover unidentified viral species by sampling animals and humans in countries with high zoonotic disease threat and determine the mechanisms that cause viral spillover into human populations. The Predict project found over 1000 unique viruses in animals and humans[18].
The Global Virome Project could aid in pandemic surveillance, diagnosis techniques and prevention strategies, and determine the need for pre-emptive production of vaccine and other countermeasures for candidate high-risk viruses. The GVP can also provide further insights into viral pathogenicity and possible biosecurity methods in agriculture[15].
The Global Virome Project was supposed to be begin sampling wild animal populations in 2020 but were delayed due to the COVID-19 pandemic.[19]
Methods
[edit]Part of a series on |
DNA barcoding |
---|
By taxa |
Other |
Direct Metagenomics
[edit]Metagenomic analysis uses whole genome shotgun sequencing to characterize microbial diversity in clinical and environmental samples. Total DNA and/or RNA are extracted from the samples and are prepared on a DNA or RNA library for sequencing[20]. These methods have been used to sequence the whole genome of Epstein-Barr virus (EBV) and HCV, however, contaminating nucleic acids can affect the sensitivity to the target viral genome with the proportion of reads related to the target sequence often being low[21][22]. Due to the uncontrollable nature of environmental DNA samples, the most abundant organisms in the environmental sample are the highest represented in the sequencing data and require large samples to achieve full coverage. That being said, shotgun sequencing ensures that these organisms that would previously go unnoticed in culture dependent methods are represented by some sequence segments[23].
Metagenomics can be used for pathogen discovery or diagnosis with the proper bioinformatic tools and databases that can evaluate the possible pathogen. Metagenomics requires no prior knowledge of the viral genome as it does not require primer or probe design, allowing for rapid response to emerging threats[20].Because this method is agnostic to expected viral content of a sample, it can be used to identify new virus species or divergent members of known species. It therefore has a role in clinical diagnostics, such as identification of pathogens causing encephalitis or virus-associated cancers[20].
PCR Amplicon Enrichment
[edit]PCR amplicon enrichment enriches a portion of the viral genome prior to sequencing. This is done via PCR amplification of primers that are complementary to a known, highly conserved nucleotide sequence[20]. PCR amplicon enrichment is then followed by whole genome sequencing methods and has been used to track the Ebola virus[24], Zika Virus[25], and COVID-19[26] epidemics. PCR amplicon sequencing is more successful for whole genome sequencing of samples with low concentrations. However, with larger viral genomes and the heterogeneity of RNA viruses multiple overlapping primers may be required to cover the amplification of all genotypes. PCR amplicon sequencing requires knowledge of the viral genome prior to sequencing, appropriate primers, and is highly dependent on viral titers, however, PCR amplicon sequencing is a cheaper evaluation method than metagenomic sequencing when studying known viruses with relatively small genomes[20].
Target Enrichment
[edit]Target enrichment is a culture independent method that sequences viral genomes directly from clinical sample using small RNA or DNA probes complementary to the pathogens reference sequence. The probes, which can be bound to a solid phase and capture and pull down complementary DNA sequences in the sample[20]. The presence of overlapping probes increases the tolerance for primer mismatches but their design requires high cost and time so a rapid response is limited. DNA capture is followed by brief PCR cycling and shotgun sequencing. Success of this method is dependent available reference sequences to create the probes and is not suitable for characterization of novel viruses[20]. This method has been used to characterize large and small viruses such as HCV[22], HSV-1[27], and HCMV[28].
Applications
[edit]Agriculture
[edit]Plant viruses pose a global threat to crop production but through metagenomic sequencing and viral database creation, modified plant viruses can be used to aid in plant immunity as well as alter physical appearance[29]. Data obtained on plant virus genomes from metagenomic sequencing can be used to create clone viruses to inoculate the plant with to study viral components and biological characterization of viral agents with increased reproducibility. Engineered mutant virus strains have been used to alter the coloration and size of various ornamental plants and promote the health of crops[30].
Ecology
[edit]Viral metagenomics contributes to viral classification without the need of culture based methodologies and has provided vast insights on viral diversity in any system. Metagenomics can be used to study viruses effects on a given ecosystem and how they effect the microbiome as well as monitoring viruses in an ecosystem for possible spillover into human populations[1]. Within the ecosystems, viruses can be studied to determine how they compete with each other as well as viral effects on functions of the host. Viral metagenomics has been used to study unculturable viral communities in marine and soil ecosystems[2][9].
Infectious Disease Research
[edit]Viral metagenomics is readily used to discover novel viruses, with a major focus on those zoonotic or pathogenic to humans. Viral databases obtained from metagenomics provides quick response methods to determine viral infections as well as determine drug resistant variants in clinical samples[20]. The contributions of viral metagenomics to viral classification have aided pandemic surveillance efforts as well as made infectious disease surveillance and testing more affordable[18]. Since the majority of human pandemics are zoonotic in origin, metagenomic surveillance can provide faster identification of novel viruses and their reservoirs[31].
Medicine
[edit]Viral metagenomics has been used to test for virus related cancers and and difficult to diagnose cases in clinical diagnostics[32]. This method is most often used when conventional and advanced molecular testing cannot find a causative agent for disease. Metagenomic sequencing can also be used to detect pathogenic viruses in clinical samples and provide real time data for a pathogens presence in a population[31].
References
[edit]- ^ a b c d Sommers, Pacifica; Chatterjee, Anushila; Varsani, Arvind; Trubl, Gareth (29 September 2021). "Integrating Viral Metagenomics into an Ecological Framework". Annual Review of Virology. 8 (1): 133–158. doi:10.1146/annurev-virology-010421-053015. ISSN 2327-056X. PMID 34033501.
- ^ a b c Alavandi, S. V.; Poornima, M. (2012-08-14). "Viral Metagenomics: A Tool for Virus Discovery and Diversity in Aquaculture". Indian Journal of Virology. 23 (2): 88–98. doi:10.1007/s13337-012-0075-2. ISSN 0970-2822.
- ^ Zárate S, Taboada B, Yocupicio-Monroy M, Arias CF (November 2017). "Human Virome". Archives of Medical Research. 48 (8): 701–716. doi:10.1016/j.arcmed.2018.01.005. PMID 29398104.
- ^ Wilhelm, Steven W.; Suttle, Curtis A. (1999). "Viruses and Nutrient Cycles in the Sea". BioScience. 49 (10): 781–788. doi:10.2307/1313569. ISSN 1525-3244. JSTOR 1313569.
- ^ Kristensen, David M.; Mushegian, Arcady R.; Dolja, Valerian V.; Koonin, Eugene V. (2010). "New dimensions of the virus world discovered through metagenomics". Trends in Microbiology. 18 (1): 11–19. doi:10.1016/j.tim.2009.11.003. PMC 3293453. PMID 19942437.
- ^ Bernardo, P; Albina, E; Eloit, M; Roumagnac, P (May 2013). "Pathology and viral metagenomics, a recent history". Med Sci (Paris). (in French). 29 (5): 501–8. doi:10.1051/medsci/2013295013. PMID 23732099.
- ^ Angly FE; Felts B; Breitbart M; Salamon P; Edwards RA; Carlson C; Chan AM; Haynes M; Kelley S; Liu H; Mahaffy JM; Mueller JE; Nulton J; Olson R; Parsons R; Rayhawk S; Suttle CA; Rohwer F (2006). "The marine viromes of four oceanic regions". PLOS Biology. 4 (11): e368. doi:10.1371/journal.pbio.0040368. PMC 1634881. PMID 17090214.
{{cite journal}}
: CS1 maint: unflagged free DOI (link) - ^ Culley, A. I.; Lang, A. S.; Suttle, C. A. (2006). "Metagenomic analysis of coastal RNA virus communities". Science. 312 (5781): 1795–1798. Bibcode:2006Sci...312.1795C. doi:10.1126/science.1127404. PMID 16794078. S2CID 20194876.
- ^ a b Pratama, Akbar Adjie; van Elsas, Jan Dirk (August 2018). "The 'Neglected' Soil Virome – Potential Role and Impact". Trends in Microbiology. 26 (8): 649–662. doi:10.1016/j.tim.2017.12.004. ISSN 0966-842X. PMID 29306554. S2CID 25057850.
- ^ Simmonds P, Adams MJ, Benkő M, Breitbart M, Brister JR, Carstens EB, Davison AJ, Delwart E, Gorbalenya AE, Harrach B, Hull R, King AMQ, Koonin EV, Krupovic M, Kuhn JH, Lefkowitz EJ, Nibert ML, Orton R, Roossinck MJ, Sabanadzovic S, Sullivan MB, Suttle CA, Tesh RB, van der Vlugt RA, Varsani A, Zerbini FM (2017). "Consensus statement: Virus taxonomy in the age of metagenomics" (PDF). Nature Reviews Microbiology. 15 (3): 161–168. doi:10.1038/nrmicro.2016.177. PMID 28134265. S2CID 1478314.
{{cite journal}}
: CS1 maint: multiple names: authors list (link) - ^ Paez-Espino D, Chen AI, Palaniappan K, Ratner A, Chu K, Szeto E, Pillay M, Huang J, Markowitz VM, Nielsen T, Huntemann M, Reddy TBK, Pavlopoulos GA, Sullivan MB, Campbell BJ, Chen F, McMahon K, Hallam SJ, Denef V, Cavicchioli R, Caffrey SM, Streit WR, Webster J, Handley KM, Salekdeh GH, Tsesmetzis N, Setubal JC, Pope PB, Liu W, Rivers AR, Ivanova NN, Kyrpides NC (2016). "IMG/VR: A database of cultured and uncultured DNA Viruses and Retroviruses". Nucleic Acids Research. 45 (D1): D457–D465. doi:10.1093/nar/gkw1030. PMC 5210529. PMID 27799466.
{{cite journal}}
: CS1 maint: multiple names: authors list (link) - ^ Paez-Espino D, Roux S, Chen IA, Palaniappan K, Ratner A, Chu K, et al. (2018). "IMG/VR v.2.0: an integrated data management and analysis system for cultivated and environmental viral genomes". Nucleic Acids Res. 47 (D1): D678–D686. doi:10.1093/nar/gky1127. PMC 6323928. PMID 30407573.
- ^ Vernimmen, Tim (2020-04-16). "Infectious disease: Making — and breaking — the animal connection". Knowable Magazine | Annual Reviews. doi:10.1146/knowable-041620-1.
- ^ "Contact". Global Virome Project. Archived from the original on 2022-08-22. Retrieved 2022-08-22.
- ^ a b Carroll, Dennis; Daszak, Peter; Wolfe, Nathan D.; Gao, George F.; Morel, Carlos M.; Morzaria, Subhash; Pablos-Méndez, Ariel; Tomori, Oyewale; Mazet, Jonna A. K. (2018-02-23). "The Global Virome Project". Science. 359 (6378): 872–874. Bibcode:2018Sci...359..872C. doi:10.1126/science.aap7463. ISSN 0036-8075. PMID 29472471. S2CID 3543474.
- ^ a b "Ambitious Global Virome Project Could Mark End of Pandemic Era". 22 February 2018.
- ^ Zhang, Peter (2021-07-09). "Reproduction of 'The COVID-19 Pandemic and the $16 Trillion Virus'".
{{cite journal}}
: Cite journal requires|journal=
(help) - ^ a b Schmidt, Charles (2018-10-11). "The virome hunters". Nature Biotechnology. 36 (10): 916–919. doi:10.1038/nbt.4268. ISSN 1087-0156. PMC 7097093. PMID 30307913.
- ^ "Before the Next Pandemic, an Ambitious Push to Catalog Viruses in Wildlife".
- ^ a b c d e f g h Houldcroft, Charlotte J.; Beale, Mathew A.; Breuer, Judith (2017-01-16). "Clinical and biological insights from viral genome sequencing". Nature Reviews Microbiology. 15 (3): 183–192. doi:10.1038/nrmicro.2016.182. ISSN 1740-1526. PMC 7097211. PMID 28090077.
- ^ Depledge, Daniel P.; Palser, Anne L.; Watson, Simon J.; Lai, Imogen Yi-Chun; Gray, Eleanor R.; Grant, Paul; Kanda, Ravinder K.; Leproust, Emily; Kellam, Paul; Breuer, Judith (2011-11-18). Jhaveri, Ravi (ed.). "Specific Capture and Whole-Genome Sequencing of Viruses from Clinical Samples". PLoS ONE. 6 (11): e27805. doi:10.1371/journal.pone.0027805. ISSN 1932-6203. PMC 3220689. PMID 22125625.
{{cite journal}}
: CS1 maint: PMC format (link) CS1 maint: unflagged free DOI (link) - ^ a b Thomson, Emma; Ip, Camilla L. C.; Badhan, Anjna; Christiansen, Mette T.; Adamson, Walt; Ansari, M. Azim; Bibby, David; Breuer, Judith; Brown, Anthony; Bowden, Rory; Bryant, Josie; Bonsall, David; Da Silva Filipe, Ana; Hinds, Chris; Hudson, Emma (2016-10). "Comparison of Next-Generation Sequencing Technologies for Comprehensive Assessment of Full-Length Hepatitis C Viral Genomes". Journal of Clinical Microbiology. 54 (10): 2470–2484. doi:10.1128/jcm.00330-16. ISSN 0095-1137.
{{cite journal}}
: Check date values in:|date=
(help) - ^ Jarrod., Chapman, (2004-03-04). Community structure and metabolism through reconstruction of microbial genomes from the environment. Nature Publishing Group. OCLC 926320276.
{{cite book}}
: CS1 maint: extra punctuation (link) CS1 maint: multiple names: authors list (link) - ^ Quick, Josh (2019-09-25). "Ebola virus sequencing protocol v1". dx.doi.org. Retrieved 2022-11-30.
- ^ Vlachakis, Dimitrios; Papageorgiou, Louis; Megalooikonomou, Vasileios (2018-06-13), "Genetic and Geo-Epidemiological Analysis of the Zika Virus Pandemic; Learning Lessons from the Recent Ebola Outbreak", Current Topics in Zika, InTech, retrieved 2022-11-30
- ^ Charre, Caroline; Ginevra, Christophe; Sabatier, Marina; Regue, Hadrien; Destras, Grégory; Brun, Solenne; Burfin, Gwendolyne; Scholtes, Caroline; Morfin, Florence (2020-07-15). "Evaluation of NGS-based approaches for SARS-CoV-2 whole genome characterisation". dx.doi.org. Retrieved 2022-11-30.
- ^ Ebert, Katja; Depledge, Daniel P.; Breuer, Judith; Harman, Laura; Elliott, Gillian (2013-09-15). "Mode of Virus Rescue Determines the Acquisition of VHS Mutations in VP22-Negative Herpes Simplex Virus 1". Journal of Virology. 87 (18): 10389–10393. doi:10.1128/jvi.01654-13. ISSN 0022-538X.
- ^ Depledge, Daniel P.; Palser, Anne L.; Watson, Simon J.; Lai, Imogen Yi-Chun; Gray, Eleanor R.; Grant, Paul; Kanda, Ravinder K.; Leproust, Emily; Kellam, Paul; Breuer, Judith (2011-11-18). "Specific Capture and Whole-Genome Sequencing of Viruses from Clinical Samples". PLoS ONE. 6 (11): e27805. doi:10.1371/journal.pone.0027805. ISSN 1932-6203.
{{cite journal}}
: CS1 maint: unflagged free DOI (link) - ^ Brewer, Helen C.; Hird, Diane L.; Bailey, Andy M.; Seal, Susan E.; Foster, Gary D. (2018-02-06). "A guide to the contained use of plant virus infectious clones". Plant Biotechnology Journal. 16 (4): 832–843. doi:10.1111/pbi.12876. ISSN 1467-7644.
- ^ Pasin, Fabio; Menzel, Wulf; Daròs, José‐Antonio (2019-02-28). "Harnessed viruses in the age of metagenomics and synthetic biology: an update on infectious clone assembly and biotechnologies of plant viruses". Plant Biotechnology Journal. 17 (6): 1010–1026. doi:10.1111/pbi.13084. ISSN 1467-7644.
- ^ a b Roux, Simon; Matthijnssens, Jelle; Dutilh, Bas E. (2021), "Metagenomics in Virology", Encyclopedia of Virology, Elsevier, pp. 133–140, doi:10.1016/b978-0-12-809633-8.20957-6, ISBN 978-0-12-814516-6, PMC 7157462, retrieved 2022-12-01
{{citation}}
: CS1 maint: PMC format (link) - ^ Dutilh, Bas; Reyes, Alejandro; Hall, Richard; Whiteson, Katrine (September 2017). "Editorial: Virus Discovery by Metagenomics: The (Im)possibilities". Frontiers in Microbiology. 8 (1710): 1710. doi:10.3389/fmicb.2017.01710. PMC 5596103. PMID 28943867.