Current insights into fungal species diversity and perspective on naming the environmental DNA sequences of fungi

doi:10.1080/21501203.2019.1614106

Review

. 2019 May 7;10(3):127-140.

doi: 10.1080/21501203.2019.1614106. eCollection 2019.

Current insights into fungal species diversity and perspective on naming the environmental DNA sequences of fungi

Bing Wu ¹, Muzammil Hussain ¹, Weiwei Zhang ¹, Marc Stadler ², Xingzhong Liu ^{1

3}, Meichun Xiang ¹

Affiliations

PMID: 31448147
PMCID: PMC6691916
DOI: 10.1080/21501203.2019.1614106

Review

Current insights into fungal species diversity and perspective on naming the environmental DNA sequences of fungi

Bing Wu et al. Mycology. 2019.

. 2019 May 7;10(3):127-140.

doi: 10.1080/21501203.2019.1614106. eCollection 2019.

Authors

Bing Wu ¹, Muzammil Hussain ¹, Weiwei Zhang ¹, Marc Stadler ², Xingzhong Liu ^{1

3}, Meichun Xiang ¹

Affiliations

¹ State Key Laboratory of Mycology, Institute of Microbiology, Chinese Academy of Sciences, Beijing, China.
² Department Microbial Drugs, Helmholtz Centre for Infection Research, Braunschweig, Germany.
³ University of Chinese Academy of Sciences, Beijing, China.

PMID: 31448147
PMCID: PMC6691916
DOI: 10.1080/21501203.2019.1614106

Abstract

The global bio-diversity of fungi has been extensively investigated and their species number has been estimated. Notably, the development of molecular phylogeny has revealed an unexpected fungal diversity and utilisation of culture-independent approaches including high-throughput amplicon sequencing has dramatically increased number of fungal operational taxonomic units. A number of novel taxa including new divisions, classes, orders and new families have been established in last decade. Many cryptic species were identified by molecular phylogeny. Based on recently generated data from culture-dependent and -independent survey on same samples, the fungal species on the earth were estimated to be 12 (11.7-13.2) million compared to 2.2-3.8 million species recently estimated by a variety of the estimation techniques. Moreover, it has been speculated that the current use of high-throughput sequencing techniques would reveal an even higher diversity than our current estimation. Recently, the formal classification of environmental sequences and permission of DNA sequence data as fungal names' type were proposed but strongly objected by the mycologist community. Surveys on fungi in unusual niches have indicated that many previously regarded "unculturable fungi" could be cultured on certain substrates under specific conditions. Moreover, the high-throughput amplicon sequencing, shotgun metagenomics and a single-cell genomics could be a powerful means to detect novel taxa. Here, we propose to separate the fungal types into physical type based on specimen, genome DNA (gDNA) type based on complete genome sequence of culturable and uncluturable fungal specimen and digital type based on environmental DNA sequence data. The physical and gDNA type should have priority, while the digital type can be temporal supplementary before the physical type and gDNA type being available. The fungal name based on the "digital type" could be assigned as the "clade" name + species name. The "clade" name could be the name of genus, family or order, etc. which the sequence of digital type affiliates to. Facilitating future cultivation efforts should be encouraged. Also, with the advancement in knowledge of fungi inhabiting various environments mostly because of rapid development of new detection technologies, more information should be expected for fungal diversity on our planet.

Keywords: Fungi; biodiversity; fungal phylogeny; molecular methods; numbers of fungi.

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Conflict of interest statement

No potential conflict of interest was reported by the authors.

Figures

Figure 1.

Figure 1.

The regression relationship between time and described fungal species using Sigma State software.

See this image and copyright information in PMC

References

1. Adams RI, Miletto M, Taylor JW, Bruns TD.. 2013. Dispersal in microbes: fungi in indoor air are dominated by outdoor air and show dispersal limitation at short distances. ISME J. 7:1262–1273. - PMC - PubMed
1. Ahrendt SR, Quandt CA, Ciobanu D, Clum A, Salamov A, Andreopoulos B, Cheng JF, Woyke T, Pelin A, Henrissat B, et al. 2018. Leveraging single-cell genomics to expand the fungal tree of life. Nat Microbiol. 3:1417–1428. - PMC - PubMed
1. Allen TR, Millar T, Berch SM, Berbee ML.. 2003. Culturing and direct DNA extraction find different fungi from the same ericoid mycorrhizal roots. New Phytol. 160:255–272. - PubMed
1. Anslan S, Bahram M, Tedersoo L. 2016. Temporal changes in fungal communities associated with guts and appendages of Collembola as based on culturing and high-throughput sequencing. Soil Biol Biochem. 96:152–159.
1. Aptroot A. 2001. Lichenized and saprobic fungal biodiversity of a single Elaeocarpus tree in Papua New Guinea, with the report of 200 species of ascomycetes associated with one tree. Fungal Divers. 6:1–11.

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[1] Adams RI, Miletto M, Taylor JW, Bruns TD.. 2013. Dispersal in microbes: fungi in indoor air are dominated by outdoor air and show dispersal limitation at short distances. ISME J. 7:1262–1273. - PMC - PubMed

[2] Adams RI, Miletto M, Taylor JW, Bruns TD.. 2013. Dispersal in microbes: fungi in indoor air are dominated by outdoor air and show dispersal limitation at short distances. ISME J. 7:1262–1273. - PMC - PubMed

[3] Ahrendt SR, Quandt CA, Ciobanu D, Clum A, Salamov A, Andreopoulos B, Cheng JF, Woyke T, Pelin A, Henrissat B, et al. 2018. Leveraging single-cell genomics to expand the fungal tree of life. Nat Microbiol. 3:1417–1428. - PMC - PubMed

[4] Ahrendt SR, Quandt CA, Ciobanu D, Clum A, Salamov A, Andreopoulos B, Cheng JF, Woyke T, Pelin A, Henrissat B, et al. 2018. Leveraging single-cell genomics to expand the fungal tree of life. Nat Microbiol. 3:1417–1428. - PMC - PubMed

[5] Allen TR, Millar T, Berch SM, Berbee ML.. 2003. Culturing and direct DNA extraction find different fungi from the same ericoid mycorrhizal roots. New Phytol. 160:255–272. - PubMed

[6] Allen TR, Millar T, Berch SM, Berbee ML.. 2003. Culturing and direct DNA extraction find different fungi from the same ericoid mycorrhizal roots. New Phytol. 160:255–272. - PubMed

[7] Anslan S, Bahram M, Tedersoo L. 2016. Temporal changes in fungal communities associated with guts and appendages of Collembola as based on culturing and high-throughput sequencing. Soil Biol Biochem. 96:152–159.

[8] Anslan S, Bahram M, Tedersoo L. 2016. Temporal changes in fungal communities associated with guts and appendages of Collembola as based on culturing and high-throughput sequencing. Soil Biol Biochem. 96:152–159.

[9] Aptroot A. 2001. Lichenized and saprobic fungal biodiversity of a single Elaeocarpus tree in Papua New Guinea, with the report of 200 species of ascomycetes associated with one tree. Fungal Divers. 6:1–11.

[10] Aptroot A. 2001. Lichenized and saprobic fungal biodiversity of a single Elaeocarpus tree in Papua New Guinea, with the report of 200 species of ascomycetes associated with one tree. Fungal Divers. 6:1–11.

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Current insights into fungal species diversity and perspective on naming the environmental DNA sequences of fungi

Affiliations

Current insights into fungal species diversity and perspective on naming the environmental DNA sequences of fungi

Authors

Affiliations

Abstract

Conflict of interest statement

Figures

References

Publication types

LinkOut - more resources

Full Text Sources