key: cord-011053-gza05hsv
authors: Tiew, Pei Yee; Mac Aogain, Micheál; Ali, Nur A’tikah Binte Mohamed; Thng, Kai Xian; Goh, Karlyn; Lau, Kenny J. X.; Chotirmall, Sanjay H.
title: The Mycobiome in Health and Disease: Emerging Concepts, Methodologies and Challenges
date: 2020-01-01
journal: Mycopathologia
DOI: 10.1007/s11046-019-00413-z
sha: 
doc_id: 11053
cord_uid: gza05hsv

Fungal disease is an increasingly recognised global clinical challenge associated with high mortality. Early diagnosis of fungal infection remains problematic due to the poor sensitivity and specificity of current diagnostic modalities. Advances in sequencing technologies hold promise in addressing these shortcomings and for improved fungal detection and identification. To translate such emerging approaches into mainstream clinical care will require refinement of current sequencing and analytical platforms, ensuring standardisation and consistency through robust clinical benchmarking and its validation across a range of patient populations. In this state-of-the-art review, we discuss current diagnostic and therapeutic challenges associated with fungal disease and provide key examples where the application of sequencing technologies has potential diagnostic application in assessing the human ‘mycobiome’. We assess how ready access to fungal sequencing may be exploited in broadening our insight into host–fungal interaction, providing scope for clinical diagnostics and the translation of emerging mycobiome research into clinical practice.

Fungal disease affects over 300 million people worldwide causing over 1.6 million deaths annually [1] . Despite their natural environmental abundance, few fungi are human pathogens, and while fulminant fungal infection is uncommon in the healthy individuals, invasive fungal disease is a concern in the immuno-compromised host with significant associated morbidity and mortality [2] . Increasing numbers of patients are at risk of invasive fungal disease including those with human immunodeficiency virus (HIV), malignancy and transplant recipients on immunosuppressive or immunomodulatory therapies, each contributing to the rising global trend of fungal infections among susceptible populations. Global warming and climate change also have significant impacts on the pathogenicity and survival of fungi [3] . Acclimatisation to higher temperatures increases their ability to replicate in the human body with high basal temperature, resulting in increased pathogenic potential even for species previously reported as nonpathogenic [3] . This impacts fungal distribution where increases in heat-resistant species facilitate human interaction, infection and transmission through skin contact, inhalation and/or ingestion [3] . Fungal infection therefore can manifest as superficial infections of the skin, nail, hair and mucous membranes, by dermatophytes and Candida spp. or as invasive disease caused by opportunistic and endemic mycoses [4] . Superficial disease is generally mild and easily diagnosed with readily available treatment. However, in the immuno-compromised individual, such infections may progress to invasive disease. Opportunistic fungal disease is primarily seen in the immunocompromised with aspergillosis, candidiasis and cryptococcosis most commonly reported. The annual incidence ranges from 200,000 to 1 million, with high and variable mortality rates ranging from 20 to 90% [5] . Table 1 and Fig. 1 summarise the most common invasive fungal diseases and the anatomical sites involved. Endemic fungal diseases occur in distinct geographic regions, apparently driven by environment and climate. Irrespective of underlying host immunity, individuals residing in endemic regions are at higher risk of life-threatening disease. Blastomycosis and histoplasmosis are endemic in the Midwestern United States (US), coccidioidomycosis in the Southwestern US, paracoccidioidomycosis in Brazil and talaromycosis in Southeast Asia [5] . Worryingly, endemic fungal disease continues to propagate even expanding beyond traditional accepted boundaries, again driven at least in part by climate change, urbanisation, land development and ease of travel [6] . A key example is the outbreak of Cryptococcus gattii at Vancouver Island and the Pacific Northwest of the USA [7] . This poses significant and emerging challenges for diagnosis, which in turn delays treatment initiation with adverse clinical consequence.

The early diagnosis and initiation of therapy for fungal infection is critical, influencing outcome and mortality, particularly in the immuno-compromised [8] [9] [10] . Current available diagnostic modalities lack sensitivity and specificity, and therefore the diagnosis of invasive fungal disease relies on a combined clinical, microbiological and radiological approach with empirical treatment often initiated based on clinical judgment alone pending diagnostic confirmation [11] . Patient characteristics including the presence or absence of neutropenia or use of antifungal prophylaxis impact the diagnostic accuracy of tests, adding additional uncertainty [12] [13] [14] . The ability to distinguish infection from colonisation poses an additional and important clinical challenge. Conventional culture methods provide species-level identification and information on antifungal susceptibility. However, culture-based methods are poorly sensitive and delay time to diagnosis [15] [16] [17] . Their accuracy is contingent on sample source, type of fungus, as well as disease and host immune status. For instance, Pneumocystis species are unable to grow on culture media [18, 19] and isolation of Aspergillus in blood is uncommon and ineffective for the diagnosis of invasive aspergillosis [16, 20] . In addition, positive cultures obtained from non-sterile body sites may not be representative and should be interpreted with caution. Direct microscopic examination is useful in providing rapid and more accurate diagnosis of fungal infection allowing differentiation by their morphology and staining [21] . However, as with culture, the diagnostic yield is contingent on several factors and exhibits variable accuracy [22] . Non-culture-based techniques are increasingly employed to aid the diagnosis of invasive fungal disease. For example, detection of b-glucan, a component of the fungal cell wall, identifies patients with invasive disease with sensitivities ranging from 50-100% and specificities of 44-98% [15, 23, 24] . The high false positive rate, however, limits the usefulness of this approach particularly in high-risk patient groups including patients with haematological malignancy, stem cell and lung transplant recipients, where co-existing bacterial infection is present and in those receiving haemodialysis [25] [26] [27] . While b-glucan is a useful diagnostic target, it is not specific to any single fungal Table 1 Review of major invasive fungal disease with organ involvement, disease manifestation, susceptibility, diagnosis and management [251] species and may be detectable across a range of fungal infections including invasive aspergillosis, candidiasis, and cryptococcosis. Galactomannan (GM) is another commonly used marker for the diagnosis of invasive aspergillosis in patients with haematological malignancy and/or neutropenia with sensitivities and specificities of 79-96% and 74-99%, respectively [23] . However, sensitivity decreases with use of antifungal agents and among non-neutropenic patients [12, 24] . Serological testing is another option available for a range of fungal infections including candidiasis, cryptococcosis and endemic mycoses with diagnostic accuracies varying based on the type of fungal organism and sample source. While providing a good diagnostic yield for histoplasmosis and coccidioidomycosis, it is not particularly useful for the diagnosis of invasive aspergillosis [22, 28] . Polymerase chain reaction (PCR) provides an alternative, more rapid and accurate diagnostic tool for the detection of fungal infection [29] . Numerous PCR assays are described with variations in primer sequence, DNA extraction method, positivity thresholds and assay performance, which coupled with limited multi-centre clinical validation, has curtailed widespread adoption [28] [29] [30] [31] . Importantly, false positive results are common as fungi are ubiquitous and contamination possible at various sample processing stages necessitating rigorous and costly quality control processes [32] . Next-generation sequencing (NGS) is increasingly used in epidemiological studies and during infectious disease outbreaks for resolution of species, virulence and antibiotic resistance, to assist infection control and its management [33] [34] [35] . In addition, NGS may be employed in the resolution of cryptic epidemiological cases where it has demonstrated superiority to traditional diagnostic methods in the detection of rare infections [36] [37] [38] . However, demonstration of its utility within the medical diagnostic setting is currently limited. Low abundance of fungi in relation to the overall microbial community (B 0.1%) poses challenges to their detection via metagenomic sequencing in human samples, necessitating targeted amplicon sequencing approaches, which are still in their infancy [29, 39, 40] . Further refinement and standardisation of reproducible wet-lab and bioinformatic workflows coupled to automated and scalable user-friendly reporting systems remain key challenges for the field, which unless addressed, will continue to impede widespread adoption and translation into clinical practice [41] [42] [43] .

Four distinct classes of antifungal drugs are currently prescribed: the polyenes, flucytosines, azoles and echinocandins. Despite treatment, mortality rates for invasive fungal disease remain high with factors contributing to poor prognosis including delayed diagnosis and initiation of antifungal treatment, host factors, site of infection, emerging antifungal resistance and drug toxicity. Clinical presentation of fungal infection is largely non-specific, and therefore a high index of suspicion is necessary for early diagnosis and initiation of treatment, particularly in the immunocompromised population. Host factors of relevance include underlying comorbidities and long-term medications that interact with antifungal treatment. This is most marked in concomitant antifungal and antiviral treatments in HIV-related cryptococcus infection, which results in life-threatening inflammation secondary to immune reconstitution. The available tissue concentrations of antifungals also differ according to their chemical and pharmacokinetic properties leading to sub-optimal concentrations, therapeutic failure and the development of resistance in many settings, highlighting the importance of infection site to the appropriate selection of antifungal agent [44] . Drug toxicity is a further consideration as treatment is often prolonged and, in those with other comorbidities, increases the risk of drug-drug interactions [45] . Antifungal resistance is emerging rapidly, both intrinsic resistance and that driven by the widespread use of antifungal and environmental fungicides [46] . Resistance, however, varies based on geographic location, patient demographics and prior drug exposure [47, 48] . Azole resistance in Candida and Aspergillus spp. ranges from 2.3-40 to 0.85-28%, respectively [47, [49] [50] [51] [52] . Resistance to echinocandins-first-line antifungal agents for invasive candidiasis-is also described in invasive Candida glabrata infections [48, 51, [53] [54] [55] . The development of new antifungals with decreased toxicity and broad-spectrum coverage is urgently required to reduce mortality rates, and a better understanding of host-fungal interaction is necessary to facilitate future therapeutic development pipelines. Furthermore, advances in NGS enable identification of antifungal resistance genes, informing our understanding of the resistome and guiding antifungal drug development [56] [57] [58] . In the following sections, we aim to describe our current understanding of the mycobiome in the context of recent NGS advances and the methodological challenges and barriers that exist in terms of its clinical implementation.

Sample processing including storage conditions and various DNA extraction protocols may inadvertently introduce confounders that affect experimental results (Fig. 2) . To date, studies comparing various methodologies of sample processing demonstrate conflicting results and varying efficacies, with implications for cross-comparisons of published mycobiome research. Freezing samples within 12 h to prevent overgrowth by fast-growing fungi and avoiding multiple freezethaw cycles has been advocated [59, 60] . The addition of RNAlater decreases the relative abundance of certain fungal taxa particularly in faecal samples suggesting possible introduction of bias in relative abundance assessments [61] . Nevertheless, taxonomic diversity generally remains assessable and largely unaffected by the freezing process [61] [62] [63] . When extracting fungal DNA for mycobiome sequencing, the highly rigid fungal cell wall, rich in glucans, chitin, mannans and glycoproteins, has necessitated additional steps that involve rigorous bead-beating or enzymatic lysis prior to DNA extraction [61, 62, [64] [65] [66] [67] . Notably, enzymatic lysis provides an alternative option for increasing DNA yields [68] [69] [70] . The harsher bead-beating method, however, is observed to have conflicting efficacies likely due to DNA degradation [71] . Various DNA extraction methods also significantly affect fungal DNA yield and quality with phenol/chloroform extraction often outperforming the various available commercial kits ( Fig. 2) [61, 62, 65, 70, 71] . This loss of DNA using commercial kits is likely related to use of silica column purification [71] . DNA extraction kits illustrate inconsistent results when performed with different sample types and produce variable fungal DNA yields [70, 72] . While extraction methods affect DNA yield and quality, their impact on mycobiome composition and diversity appears minor [62, 65, 71] . However, recent work from our group, using spontaneous induced sputum, has demonstrated more consistent amplification of the ITS region from samples subjected to mechanical disruption as compared to enzymatic lysis [40] . This was observed despite higher overall DNA yields achieved by enzymatic lysis suggesting preferential liberation of fungal DNA by mechanical lysis [40] . Extraction methods are critical and must be applied consistently and carefully both within and between mycobiome studies. Ultimately, sample-specific mycobiome protocols are required and a need exists to incorporate specific methods adjusted to sample type or disease-specific application, importantly, with validation for routine use in future mycobiome research.

In contrast to high-throughput sequencing (HTS) of the bacterial microbiome, taxonomic classification and primer choice are not well established for the fungal mycobiome ( Fig. 2) [60, 73] . As amplicon sequencing is well recognised to be subject to selective amplification bias, careful consideration of primer selection is crucial [74] . Key factors include taxonomic resolution, coverage, accuracy and amplicon length [74] . The ITS region, located between genes encoding ribosomal subunits 18S and 23S, has been proposed as the universal genetic fungal barcode, primarily because these regions have high evolutionary rates and are flanked by highly conserved regions serving as suitable target sites for universal primers [60, 73, 75, 76] . The ITS region typically spans 500-700 bps, and consists of two sub-regions, ITS1 and ITS2, which are separated by the conserved 5.8S region [77] . Although primers targeting ITS1 (i.e. ITS1F and ITS2) have been used for decades in several large-scale microbiome projects, to date, it is still unclear which ITS fragment is optimal. Recent findings demonstrate that these primers suffer from primer bias, amplification bias and fail to accurately profile mock communities analysed, leading to inconsistent representation of synthetic fungal communities of known taxonomic abundance [40, 74, [78] [79] [80] [81] [82] . Based on these observations, Nilsson and colleagues provide a list of fungus specific, HTS-oriented primers for amplification of ITS region, and recommend targeting the ITS2 sub-region by using degenerate forward primers gITS7ngs and the reverse primer ITS4ng owing to their superior coverage of the fungal kingdom [60] . Advantages of the ITS2 sub-region include a more universal primer site and lower length variation, leading to less taxonomic bias compared to ITS1 [60, 83, 84] . While this primer set (gITS7ngs and ITS4ng) has a superior coverage of fungal kingdoms, its accurate taxonomic resolution has yet to be evaluated experimentally [82] . Further confirmatory studies are required before the field can advance and eventually reach consensus on methodology for targeted amplicon sequencing of the mycobiome, as has been the case for 16 s rRNA sequencing of bacterial microbiomes. In addition to primer choice, care must be taken to yield fewer compromised amplicon sequences. These include careful consideration of number of PCR cycles and dilution of DNA samples where possible (Fig. 2) [85, 86] . High fidelity proofreading PCR polymerase with low GC content bias is also necessary to reduce chimeras and random errors that accumulate in later cycles [85, 86] . It is also essential to include appropriate negative controls and a mock community into the analysis. The former indicates sources of potential contamination, while the latter allows assessment of chimera formation, quantification of index switching and operational 

An alternative approach to targeted amplicon sequencing is the use of whole-genome shotgun (WGS) metagenomics to study the mycobiome. This entails the sequencing of all extracted DNA in a given sample without the use of targeted PCR amplification of the ITS or other specific target sequences. Here, all DNA from resident microbes and host cells present in a sample is assessed. Sequence reads are processed and classified relative to a reference database through either assembly-based or assembly-free methods [89] . Analysis will usually also include steps for removal of host DNA sequences, which may contribute to a significant proportion of sequence data if removal of human cells is not attempted prior to DNA extraction [90] . While, in principle, metagenomic sequencing should provide a superior, unbiased assessment of the mycobiome, studies to date employing WGS metagenomics highlight the low abundance of fungi relative to bacterial DNA across a variety of human samples (Fig. 2) [39] . This represents a significant cost barrier given the sequencing depth therefore required to detect fungi in samples where bacteria predominate while lower sequencing coverage also hinders assembly-based analysis of fungi [89] . Currently, it appears that low fungal abundance in human samples hinders the widespread application of metagenomic WGS in human samples, a finding that appears unrelated to DNA extraction methods and reflects a genuinely low overall in vivo fungal abundance [63] .

The development of tools for the analysis of ITSderived amplicon sequences is still a nascent area of research, and many options are available for the analysis of metabarcoding amplicon data sets [29] . While the field still has no consensus on standards and best practices, further studies are clearly required, and no optimal, broadly applicable protocol has been yet established. Further, it is probable that amplicon sequencing and its accompanying analysis largely depend on the samples under investigation due to variable primer coverage, as demonstrated for comparable bacterial microbiome analysis targeting the 16 s rRNA gene [91] . The increased variability of the fungal ITS region exacerbates this problem in the case of mycobiome research, and this requires careful consideration when interpreting ITS-derived mycobiome profiles. A further analytic hurdle of mycobiome metagenomic analyses remains the sparsely populated fungal databases on which read classifications are based (Fig. 2) . This leads to large numbers of unclassified reads or unidentified operational taxonomic units (OTUs), which may be addressed by generation of more high-quality metagenomic and whole-fungal genome assemblies [63, 92] . Major fungal ITS reference databases include the INSDC, UNITE and Warcup ITS [60] . Although accurate species-level classification is not possible using the ITS regions, there are currently no known alternate markers offering comparable lineage separation, while reported taxonomic thresholds for filamentous fungal identification at the genus, family, order and class levels are estimated at 94.3%, 88.5%, 81.2% and 80.9%, respectively [60, 93] . The increased accessibility of third-generation long-read sequencing offers promise in this regard as the large stretches of repetitive and non-coding DNA as well as introncontaining genes found in fungal genomes can be resolved by these technologies which may also be applied to targeted sequencing of the ITS [60, 63] . Although the literature on fungal metagenomics is lacking, two key studies (Nash et al. and Donovan et al.) represent the most in-depth assessment to date in terms of metagenomic identification of fungi in human samples [63, 94] . Nash et al. performed a large assessment of gut samples from the human microbiome project, performing both metagenomic analysis and comparative ITS sequencing. Importantly, they showed that DNA extraction methods did not have appreciable effects on the levels of fungi detected, reaffirming the apparent low abundance of fungi in these samples. Secondly, they performed a comparative analysis of ITS and 18 s targeted sequencing protocols demonstrating that ITS2-targeting primers showed greater resolution of low-abundance taxa [63] . The work of Donovan and colleagues is notable for their bioinformatic dissection of the challenges inherent to analysis of the fungal metagenome. They present a solution in the form of the 'FindFungi' pipeline, which highlights the challenges of fungal metagenomic analysis including false positive detection, for which they developed an important step to identify uneven read distribution across reference genomes indicating spurious fungal detection [94] . Finally, an additional challenge that remains is the implementation of these bioinformatic pipelines, which, necessitates execution on high-performance computing clusters due to the requirement to hold large genomic databases in memory (Fig. 2) . Such computation requires domain expertise that may not be widely available to fungal research laboratories and remains an operational and logistical challenge.

Culture-based methods of detection require a priori selection of fungal growth conditions and are susceptible to bacterial overgrowth hindering the proliferation of selected fungi leading to bias. In addition, culture-based methods are prone to cross-contamination of spore-producing fungi, which can be minimised by the use of horizontal laminar flow clean bench [95, 96] . While the addition of antibiotics to culture media is commonly employed to prevent bacterial contamination, its drawbacks include limited antibacterial spectrum, and its potential inhibitory effect on fungi [97] [98] [99] . Results from culture methods may be difficult to cross compare with the existing literature given heterogeneity of methodology and study designs as well as sample pre-processing protocols, thereby requiring a standardised protocol for detecting key fungal pathogens [100, 101] . However, culture-based methods do allow for an assessment of antifungal susceptibilities and the isolates obtained by culture provides scope for further molecular characterisation. Numerous culture-independent approaches have been developed to overcome the limitations of culture-based methodology but are not without their disadvantages. Internal transcribed spacer-polymerase chain reaction (ITS-PCR) approaches could be used to detect mixed infections; however, careful target selection is necessary [76, [102] [103] [104] . In some cases, ITS-PCR may appear even less reliable than culture for fungal detection [95] . Multiplex PCR assays allow for greater efficiency but require strict primer design [101] . However, PCR-based approaches are susceptible to falsenegative results where sub-optimal sample storage or DNA extraction methods are employed or where PCR inhibitors are present. The use of oligonucleotide array platforms represents a possible alternative but is expensive and subject to batch effects [101] . Arguably, sequencing of individual amplified ITS regions remains the gold standard for fungal identification, allowing for sensitive detection of unculturable or low-abundance fungi but may not be practical for all laboratories [105] . The use of mycobiome profiling as an alternative to culture-based and molecular diagnostic detection methods represents potentially valuable applications for this technology, but one that requires further validation and research [95] .

The term mycobiome is used to describe the fungal component of the microbiome. It is yet unclear whether a core mycobiome, analogous to the bacteriome, exists in humans [106] . Relative to the bacteriome ([ 99% of the total microbiota), the human mycobiome is less diverse (generally \ 20 OTUs per sample) and present at a lower abundance (B 0.1% of the total microbiota) [39, 63] . Targeted sequencing approaches reveal that infants are colonised by fungi shortly after birth, predominantly by members of the genera Candida, Saccharomyces, Cladosporium, Cryptococcus and Malassezia [107, 108] . Where correlated, stool mycobiomes from healthy adults reveal profiles predominated by Saccharomyces, Malassezia and Candida suggesting that these genera are the key constituents of a healthy mycobiome throughout life. Critically, however, and in contrast to human bacteriome studies, little correlation with host phenotype metadata is firmly established in healthy individuals and, as such, our knowledge of fungal mycobiome-host interaction remains limited to that in fungal colonisation and/or disease. It is clear from existing studies and their subsequent molecular analysis that intricate immunological systems have evolved to regulate fungal homoeostasis and, when perturbed, lead to infection or other pathologies [109] . Immunity to fungi is underpinned by innate signalling pathways recognising both spores and fungal cell wall components and include adaptive T cell responses that orchestrate tolerance and appropriate immune surveillance of ubiquitous fungi encountered daily [109, 110] . Immune responses to fungi are protective when functioning, however, where over-zealous, can manifest as allergy. Consequently, the evolution of immuno-regulatory mechanisms in vivo is perturbed across a range of fungal-driven allergy. Given the parallels with the human bacteriome, where host immunity acts as gatekeeper, it is arguable that similar ecological interactions occur with fungi [111] . Perhaps the strongest evidence for a conserved human mycobiome is evidenced by the restricted numbers of fungi that actually inhabit the human body, suggestive of niche specialisation [112] . Despite over 50 described bacterial phyla, the human bacteriome is characterised by four: Actinobacteria, Bacteroidetes, Firmicutes and Proteobacteria. In corollary, fungal taxa exhibit lower diversity in vivo compared to that seen environmentally and associations between fungi and specific body sites indicate the likely existence of selection and adaptation [113, 114] . Given the limited available data, formal meta-analysis of clinical mycobiome studies, while important, is currently challenging to perform. However, emerging associations based on culture-independent mycobiome studies in humans are summarised in Fig. 1 .

While fungal lung disease is now widespread and a growing global concern, the lack of dedicated mycobiome studies assessing the effects of fungi in chronic lung disease is hampering the field. In this particular organ system, the prior presupposition of sterility in a healthy lung puts back microbiome studies in this area for a number of years, and consequently, our understanding of the respiratory microbiome lags significantly behind that at other anatomical sites [115] . The advent of culture-independent sequencing technologies has uncovered the diversity of organisms inhabiting the lung, including that in the healthy state [116, 117] . Through the use of internal transcribed spacer (ITS) sequencing, it was reported that Ceriporia lacerata, Saccaromyces cerevisiae and Penicillium brevicompactum were possible pulmonary fungi, with the main pathogen being Aspergillus fumigatus [118, 119] . Lung-dwelling microbiota include bacteria, fungi and viruses, which together maintain a crosskingdom ecological network [120] . Interactions between lung and gut microbiomes, through the lung-gut axis, have further immunological consequence, and changes in the gut mycobiome can influence allergic airway disease [121] [122] [123] [124] [125] . The healthy lung mycobiome differs from that observed in patients suffering with chronic inflammatory respiratory disease such as asthma, chronic obstructive pulmonary disease (COPD), cystic fibrosis (CF) and bronchiectasis [126, 127] . The lungs in asthma, COPD and CF all exhibit lower fungal diversity, which in turn is linked to poorer lung function postulated to be influenced by fungal overgrowth and/or loss of some fungal species [128] . In asthma, higher loads with increase percentages of Psathyrella candolleana, Malassezia pachydermatis, Termitomyces clypeatus and Grifola sordulenta and a greater fungal diversity were observed compared to that of a healthy airway [129, 130] . In children with severe asthma, a higher abundance of Rhodosporidium, Pneumocystis, Leucosporidium and Rhodotorula was detected when compared to those without asthma [131] . Bronchiectasis, a permanent and irreversible dilatation of airways, places patients at the higher risks of fungal acquisition and colonisation [132] . This is reflected by airway mycobiomes demonstrating a higher abundance of potentially pathogenic taxa including Aspergillus, Penicillium and Cryptococcus and the detection, in many patients, of an unfavourable allergic sensitisation and immune response profile associated with Aspergillus [117, 133] . In view of the dysfunctional mucociliary clearance inherent in bronchiectasis, the airway is susceptible to inhaled airborne fungi and therefore colonisation [134] . In COPD, Aspergillus spp. has been isolated in 17% of patients and particular fungal taxa such as Pneumocystis jirovecii associated with a COPD airway have also been found in HIV and COPD-associated HIV suggestive of immunological predisposition [135, 136] . The overrepresentation of Pneumocystis and other fungal species in HIV-related COPD further illustrates the relationship between fungal communities in the lung and corresponding lung function and homoeostasis, warranting more detailed investigation by culture-independent sequencing [137] . Significant fungal variability is seen in cystic fibrosis (CF), a genetic disease caused by abnormal Cystic Fibrosis Transmembrane conductance Regulator (CFTR) function, where fungal colonisation and infection for A. fumigatus range between 6 and 60% [138] . While dedicated CF mycobiome research is nascent, a number of groups have nevertheless started to characterise its main components. Stable fungal communities are detected and exist in parallel to the more ephemeral fungal species that remain transient when assessed longitudinally [95, 127, 128, [139] [140] [141] [142] [143] . Targeted sequencing studies of the CF mycobiome reveal that in addition to the fungi detected by mycological culture alone, that (unculturable) fungal taxa are also present [95, 139, 142] . Overall, an increased abundance of Aspergillus species (particularly A. fumigatus), C. albicans, C. parapsilosis and Malassezia is identified [127] . In both asthma and CF, an allergic response may be induced when Aspergillus is encountered, with the key form being allergic bronchopulmonary aspergillosis (ABPA) [144] . The application of mycobiome sequencing approaches to the lung has started to gain significant traction and research interest with the transition from smaller pilotscale optimisation studies to a more detailed and comprehensive assessment in well-phenotyped cohorts of patients with respiratory disease [117, 139, 145, 146] .

Efforts to examine gut mycobiomes have largely focused on gastrointestinal (GI)-associated disease, and key findings echo trends of mycobiome alteration in other non-GI diseased states. In inflammatory bowel disease (IBD), for instance, initial work using 18S rRNA and rDNA sequencing showed an increased fungal diversity in Crohn's disease (CD) but not ulcerative colitis (UC) [147, 148] . Further differences were also identified between inflamed and noninflamed tissue [147] . More recently, however, application of ITS2 sequencing has found distinct fungal microbial dysbiosis in IBD with increased Basidiomycota/Ascomycota ratios accompanied by higher proportions of C. albicans but reduced levels of S. cerevisiae [149] . In CD, ITS2 pyrosequencing also confirms increases to overall fungal load during disease flares and a higher prevalence of the Cystofilobasidiaceae family and C. glabrata species. In correlation, the application of ITS1 sequencing in another study revealed an increased Candida tropicalis in CD as compared to non-CD relatives [150] . Interestingly, S. cerevisiae and Filobasidium uniguttulatum are associated with non-inflamed tissue in CD [151] . Malassezia restricta was found to increase CD severity in a subset of patients with CARD9 polymorphisms, suggesting that the targeting of specific fungi in certain patient phenotypes may have value [152] . It is further demonstrated that antifungal drugs lead to increases in colitis severity in animal models where ITS1 amplicon sequencing revealed gut fungal dysbiosis characterised by a reduction in Candida spp. and concurrent increase in Aspergillus, Wallemia and Epicoccum spp. [153] . Similarly, antibiotics influence gut inflammation through modification of the gut bacteriome with a consequential impact on fungal colonisation [154] . Here, alteration in Enterobacteriaceae modulates fungal colonisation and colitis severity [154] . Although the mouse gut mycobiome does not fully represent that in humans, these findings lend support to the implication of fungal dysbiosis in IBD. Paediatric IBD has also been assessed providing insight into potential age-associated effects, and 18S rDNA pyrosequencing illustrates Basidiomycota dominance [155] . In other paediatric IBD works, ITS1 pyrosequencing reveals high Candida burdens and a reduced fungal diversity [156] . While dedicated study of the healthy gut mycobiome is limited and much required, Nash et al. observed the healthy human gut mycobiome to be lacking in diversity and dominated by yeast genera such as Saccharomyces, Malassezia and Candida, albeit with significant interand intra-individual variability [63] . This suggests active and dynamic change to the gut mycobiome over time, further influenced by host immunity, even in the absence of disease. In Irritable Bowel Syndrome (IBS), a functional gastrointestinal disease, ITS1based metabarcoding of faecal samples reveals a gut mycobiome dysbiosis with a significant loss of diversity. Saccharomyces and Candida were dominant in IBS and healthy controls, but higher proportions were observed in the former [157] . Visceral hypersensitivity is linked to IBS with fungi implicated in animal models, suggesting that targeted manipulation of the mycobiome may provide scope for therapeutic intervention [158, 159] . Mycobiome signatures clearly differ between hypersensitive and normally sensitive IBS [158] . While these findings are clearly of clinical interest, more compelling evidence and biological validation is required to further clarify mechanistic underpinnings of these early observations [157] . Interestingly, in the oncological setting, antifungal treatment is associated with decreased tumour progression in pancreatic ductal carcinoma, while posttherapeutic repopulation by Malassezia accelerates tumour growth [160] . In addition, an increased abundance of Malassezia is described in colorectal cancer by faecal shotgun metagenomic sequencing, along-with Moniliophthtora, Rhodotorula, Acremonium, Thielaviopsis and Pisolithus, while a higher abundance of Basidiomycota is associated with more advance disease [161, 162] . The gut mycobiome may additionally influence other organ systems such as the lung and central nervous system through their respective axes, but the precise mechanisms are poorly understood. In particular, the lung-gut axis, which includes the mycobiome, is highlighted as a key and emerging player in determining susceptibility to chronic lung disease, and the gut microbiome composition in itself has also been independently associated with several chronic inflammatory lung diseases [118] . For instance, the presence of C. albicans in the gut influences Th17-related immune pathways, which in turn has implications for Aspergillus-associated pathology in chronic airways disease supporting a role for lung-gut cross-talk in the pathogenesis of respiratory disease [124] . Gut mycobiome dysbiosis is reported in multiple neurological disorders, where a higher abundance of Candida occurs in schizophrenia, autism and Rett Syndrome [163] [164] [165] [166] . This has prompted the investigation of gut fungi in the microbiome-gut-brain axis, an emerging biological concept already firmly established with respect to bacteria [167] . While recent studies describe associations between fungal dysbiosis and IBS, the association with neurological symptoms such as anxiety and depression in IBS sufferers is intriguing, results that further support the role of gut fungi in the microbiome-gut-brain axis [168] . While these findings remain speculative at present requiring more study to explain clearer biological mechanism, they nevertheless do illustrate the importance and emergence of the fungal mycobiome in human disease.

The skin remains a key organ and provides barrier protection against pathogens but is also home to resident fungi [169, 170] . Different skin components demonstrate differing fungal patterns, and fungal species also vary by age and gender. For instance, children have greater numbers and variety of fungi on their skin compared to adults, who are dominated by lipophilic Malassezia [115, 171] . This is likely explained by the changes in sebum composition and sebaceous gland activation [171] . Most work reveals that healthy skin (across many body sites) is characterised by Malassezia, which produces an aryl hydrocarbon receptor (Ahr) ligand beneficial for epithelial cell health and UV protection [114, 115, 172] . Diverse domains of the skin mycobiome interact with one another, promoting connectivity and providing network stability. Comparable to lung mycobiomes, the communities in skin mycobiomes help maintain ecological network structure [120] . As with other organ systems and their microbiomes, the skin mycobiome associates with skin disease: Malassezia, when in higher abundance or where an inappropriate immune response is observed is seen in association with seborrhoeic or atopic dermatitis [115, 173] . Conversely in psoriasis, which involves the multiplication of skin cells at much higher rates, patients had a lower abundance of Malassezia when compared to healthy skin despite Malassezia remaining the dominant phylum in both groups [174] . Relationships between the skin mycobiome and systemic diseases demonstrating dermatological manifestations are established: for example, the role of fungi in systemic sclerosis (SSc), an autoimmune disease characterised by skin thickening where Rhodotorula glutinis is highly abundant. Average R. glutinis abundance in normal subjects compared to SSc patients was 0.02 and 5.04 per million reads, respectively, supporting this association [175] . Tinea versicolor (Pityriasis versicolor), a skin fungal infection, attributed to Malassezia and a consequence of Malassezia protein-induced melanocyte apoptosis and UV exposure has also been the subject of multiple investigations [115] . Affected lesions illustrate high burdens of M. globosa, M. sympodialis and M. furfur, and mycelial fungal forms predominate in contrast to yeast forms commonly seen in healthy skin [176] . A role for the mycobiome has been established in seborrhoeic dermatitis, a condition where scaly patches, red skin and persistent dandruff ensue. While Ascomycota and Basidiomycota are prevalent in both healthy and dandruff-affected human scalps, the latter illustrates higher densities of Acremonium, Penicillium and Malassezia [176, 177] . Malassezia restricta and Malassezia globosa are identified in seborrhoeic dermatitis, and the presence of new colonising strains when compared to the healthy scalp is indicative of disease onset [173] . Malassezia may also more directly cause dandruff as antifungal agents are particularly effective as treatment [176] . Atopic dermatitis (AD) (eczema) is another important skin condition with established mycobiome associations: significant intra-and inter-individual variation is observed in AD where taxonomic diversity has been examined. However, consistently, as is the case in other skin conditions, M. sympodialis, M. sloofiae and M. dermatis all characterise disease and sometimes exacerbate it. AD patients demonstrate circulating IgE to Malassezia and on closer examination, secreted Malassezia vesicles from AD patients differ in their RNA content when compared to healthy individuals [115, 176, [178] [179] [180] . In addition, Malassezia may induce cutaneous inflammation via a Th-17 response, with increased CCR6 ? Th17 memory T cells (M. specific) observed in AD [181] . While Malassezia is a key AD correlate, it is important to recognise that non-Malassezia fungi are also described [179] . Different methodologies have been employed to characterise and describe skin mycobiomes: ion-torrent sequencing has been used in AD, while other approaches include targeted amplicon sequencing of various fungal regions, such as the fungal 28S rRNA large subunit D1/D2 and the 18S rRNA, internal transcribed spacer (ITS) regions ITS1 and ITS2 [108, 114, 171, 173, 175, 176, 179, [182] [183] [184] .

Increasing evidence suggests the importance of the microbiome in neurological disease. Changes to gut bacteria are linked to multiple sclerosis (MS), a neuroinflammatory disease characterised by demyelination and neurodegeneration, suggesting cross-talk via gutbrain microbiota in its pathogenesis [185] [186] [187] [188] [189] [190] . Higher abundance of Candida, Malassezia and Trichosporon by targeted ITS1 sequencing is reported in MS compared to control brain tissue [187] . Similarly, metagenomic analyses of cerebrospinal fluid (CSF) from MS patients reveal that the presence of Malassezia, Ascomycota, Funneliformis, Glomus, Cladosporium, Candida and Alternaria, however as concluded by these works, likely reflects environmental contaminants [191] . In contrast, Jovel et al. using CSF from MS patients did not report any detection of fungal reads [192] . In Alzheimer's disease, fungal cells are detected in neurons through immunohistochemistry and confocal microscopy within brain tissue and these fungal species are further identified by nested PCR, where Candida, Cladosporium, Malassezia, Neosartorya, Phoma and Sacharomyces are detected [193] . Using targeted amplicon sequencing, Alternaria and Malassezia are higher in Alzheimer's compared to normal brain tissue [194] . In other works, brain tissue from individuals with amyotrophic lateral sclerosis (ALS), a neurodegenerative disease with progressive motor neuron dysfunction, contains an increased abundance of Candida, Malassezia, Fusarium, Botrytis, Trichoderma and Cryptococcus [185, 195] . The strong association between seborrhoeic dermatitis and Parkinson disease (PD) also raises the suspicion of specific Malassezia contribution to both disease states. Importantly, genetic polymorphisms associated with PD and levodopa use are known to promote Malassezia growth and invasiveness, and hence this fungal association is of clinical relevance [196] . Collectively, these studies implicate fungi in the pathogenesis of several neurological diseases underlining the importance of fungal biology and host-microbe interaction to overall human health and the inter-organ axis communication networks posited to promote disease onset.

Fungi are ubiquitous and present in indoor (built) and outdoor environments [197] . While indoor and outdoor fungal communities are similar, indoor fungal particles are passively distributed and dominated by spores, hyphal fragments and other dormant fungi [198] . Fungi from indoor air may originate from outdoor air with air exchanges when windows are opened [199] . Outdoor airborne fungal composition is affected by location, temperature and humidity, with large numbers of fungi identified by metagenomic sequencing, with consequent and significant impact on indoor fungal communities [200] . Other sources of indoor fungi include humans, pets, plants, plumbing systems, heating ventilation and air conditioning systems (HVAC), and also dust re-suspension [201, 202] . Exposure to indoor fungi and fungal particles is linked to health-related outcomes including allergies, fatigue and asthma [197, 203] . In addition, damp dwellings pose an additional health risk due to fungal exposure [204] . The built mycobiome is therefore of interest from microbiological, environmental and clinical perspectives. Traditionally, morphology-based studies of fungal cultures and their spores, derived from indoor sampling, have recognised many common indoor fungal species; however, with the application of high-throughput sequencing in the built environment, the much larger scale and depth of the indoor fungal diversity have been demonstrated [203, 205] [206, 207] . In other works, 986 fungal OTUs were detected in a homogeneous set of houses in a Californian family housing complex [199] . Considering culture-dependent and culture-independent approaches (including next-generation sequencing; NGS), substantial fungal diversity is now associated with the built environment. These indoor fungi, whether persistent residents or transient visitors, likely hold clues to the increasing numbers of human allergies and other health problems observed globally in previously healthy individuals [208] . One such example is 'sick building syndrome': associated with poor indoor air quality and fungal exposure and experienced by building occupants, with symptoms including headache, dizziness, nausea, eye, nose or throat irritation [209] [210] [211] . As part of the effort in reducing harmful exposure of indoor fungi, sourcetracking of airborne fungi is necessary to locate and eliminate contaminated building surfaces that may serve as potential reservoirs, a major challenge given the highly dynamic movement of aerosols. Fungal growth on building surfaces may also be invisible to the naked eye, and it is impractical to swab all surfaces for examination. Therefore, future studies must instead attempt source-tracking by swabbing potential source surfaces in homes, classrooms and offices to compare them against air samples using probabilistic models [201, 212] . Some early works have reported mould and yeasts from the genera Alternaria, Aspergillus, Cladosporium, Penicillium, Rhodotorula and Wallemia, where Rhodotorula mucilaginosa generally dominate moist spaces such as toilets, A. fumigatus in drier spaces such as the living rooms and Cladosporium in almost every living space [212, 213] . Besides source-tracking, engineered building materials and surface coatings that prevent or minimise fungal colonisation are another area of active research [214, 215] . These solutions, however, are expensive, and it is almost impossible to maintain sterility in a built environment unless medically warranted, for example, in the intensive care units of healthcare facilities, which in themselves poses a challenge [216] . Alternatively, buildings should be constructed using sustainable fungal-resistant materials complemented with architectural designs that consider operating factors such as heating, ventilation and air conditioning (HVAC) systems for controlling indoor temperature and relative humidity, as well as plumbing designs with accessible sites for addressing water leaks, all of which can contribute to a safer indoor environment, minimal fungal contamination and potentially improved human health outcomes.

The number of reported microbiome-related publications has increased exponentially in recent years and now includes numerous studies of the mycobiome [94, 185] . In parallel, a better understanding of the role of microbes in health and disease has emerged with studies increasingly investigating the importance of the mycobiome and its contribution to disease [117, 124, 133, [217] [218] [219] . It is likely that these organisms co-exist in the same environment and that interaction between bacterial, fungal and viral microbiomes achieves homoeostasis among healthy individuals, while dysbiosis leads to disease. Although increasingly investigated in association with pathological states, it is still too early to make conclusions about the true clinical importance and relevance of the mycobiome. Several challenges do remain including the validation and standardisation of robust sampling and analytic methodologies, which must be examined in larger-scale studies. Currently, there is no standardised method in mycobiome sequencing with variation in DNA extraction methods, primer selection, sequencing, reference databases and analytical pipelines (Fig. 2) , precluding robust meta-analysis of clinical studies performed to date, which continue to increase, but remain limited in number. Nevertheless, the field of mycobiome research is evolving and the rapid adoption of sequencing and computational technologies may overcome current limitations and allow a better definition of the mycobiome from a clinical context [29] . With an improved understanding of resident mycobiomes and their interaction with host immunity, as correlated with disease at difference stages, this potentially opens avenues for early diagnosis and more targeted therapeutic approaches. Moreover, the use of NGS to characterise resistome pathways may have relevance for surveillance, antifungal stewardship and the development of new antifungal drug approaches. Newer treatment approaches may emerge from better patient stratification based on mycobiome profiles, while manipulating or restoring a 'healthy' mycobiome also represents a potentially viable approach for precision medicine. These technological advancements combined with sequencing and analysis may be simplified and evolve into point of care diagnostics for fungal disease in the future.

The number of microbiome studies focused on bacteria far exceeds that of the fungal mycobiome (and virome). This is largely attributed to pioneering efforts towards the standardisation of methodologies for bacterial 16 s rRNA gene sequencing and analysis, allowing scalability. A standardised and reliable method of mycobiome sequencing combined with more comprehensive fungal database coverage is crucial to achieve similar scalability for fungal microbiomes [29, 92] . Despite known interaction between various microbes, studies integrating bacterial microbiomes, fungal mycobiomes, viromes and parasites are limited. Interaction between members of microbial kingdoms likely results in an alteration of function and behaviour of individual microbes, which in turn play important roles for disease pathogenesis. Microbes housed at key body sites exhibit cross-talk and interaction with host immunity resulting in systemic manifestations of disease outside the initial site of dysbiosis. Dysregulation of intestinal microbiome has been implicated in allergic airways disease, with increased intestinal Clostridium spp. in asthmatics and an emerging role for the gut mycobiome in regulating fungal airway responses through the lunggut axis [118, 124, [220] [221] [222] . Such insight provides explanations for clinical phenomena including how disruption of the healthy intestinal mycobiome composition with oral antifungals can lead to exacerbations of allergy airway disease [173] . Changes in the composition of intestinal microbiota are also implicated in diseases of the central nervous system including autism spectrum disorder, Parkinson disease and schizophrenia, further substantiating the key role of microbiome cross-talk, which is likely to include major fungal in addition to established bacterial players [165, 223, 224] . To better understand the precise role of the mycobiome and its contribution to disease pathogenesis, future studies must assess interactions between the various microbial kingdoms in tandem with host immunity across multiple body sites in a holistic systems-based approach. Across such complex and interlinked microbial systems, the mycobiome is clearly a recognised and emerging factor that contributes to a range of diseases and their pathogenesis, which if harnessed appropriately can represent an opportunity, one that improves disease prognosis and future approaches to precision medicine using the microbiome.

Stop neglecting fungi

Global and multi-national prevalence of fungal diseases-estimate precision

Global warming will bring new fungal diseases for mammals

An overview of fungal infections

An official American Thoracic Society clinical practice guideline: the clinical utility of bronchoalveolar lavage cellular analysis in interstitial lung disease

An epidemic of coccidioidomycosis in Arizona associated with climatic changes

Molecular evidence that the range of the Vancouver Island outbreak of Cryptococcus gattii infection has expanded into the Pacific Northwest in the United States

The global problem of antifungal resistance: prevalence, mechanisms, and management

Fungal infections in HIV/AIDS

Early diagnosis of fungal infection in immunocompromised patients

Revised definitions of invasive fungal disease from the European Organization for Research and Treatment of Cancer/Invasive Fungal Infections Cooperative Group and the National Institute of Allergy and Infectious Diseases Mycoses Study Group (EORTC/MSG) Consensus Group

Diagnostic value of galactomannan antigen test in serum and bronchoalveolar lavage fluid samples from patients with nonneutropenic invasive pulmonary aspergillosis

Serum galactomannan-based early detection of invasive aspergillosis in hematology patients receiving effective antimold prophylaxis

Use of bronchoalveolar lavage to detect galactomannan for diagnosis of pulmonary aspergillosis among nonimmunocompromised hosts

Finding the ''missing 50%'' of invasive candidiasis: how nonculture diagnostics will improve understanding of disease spectrum and transform patient care

What is the clinical significance of positive blood cultures with Aspergillus sp. in hematopoietic stem cell transplant recipients? A 23 year experience

Diagnosis of invasive septate mold infections. A correlation of microbiological culture and histologic or cytologic examination

The challenge of Pneumocystis carinii culture

Inability to culture Pneumocystis jirovecii

The mechanism for low yield of blood culture in invasive aspergillosis; the clinical importance of antigen detection tests revisited

British Society for Medical M. British Society for Medical Mycology proposed standards of care for patients with invasive fungal infections

Clinical approach and management for selected fungal infections in pulmonary and critical care patients

Approach to the diagnosis of invasive aspergillosis and candidiasis

Diagnosis and management of Aspergillus diseases: executive summary of the 2017 ESCMID-ECMM-ERS guideline

The (1,3){beta}-D-glucan test as an aid to early diagnosis of invasive fungal infections following lung transplantation

Diagnostic performance of the (1 ? 3)-beta-D-glucan assay for invasive fungal disease

Difficulties in using 1,3-{beta}-D-glucan as the screening test for the early diagnosis of invasive fungal infections in patients with haematological malignancies-high frequency of falsepositive results and their analysis

Molecular and nonmolecular diagnostic methods for invasive fungal infections

Recent trends in molecular diagnostics of yeast infections: from PCR to NGS

Clinical practice guideline for the management of candidiasis: 2016 update by the Infectious Diseases Society of America

Determining the analytical specificity of PCR-based assays for the diagnosis of IA: What is Aspergillus?

PCR-based diagnosis of human fungal infections

Tracking a hospital outbreak of carbapenem-resistant Klebsiella pneumoniae with wholegenome sequencing

High-throughput whole-genome sequencing to dissect the epidemiology of Acinetobacter baumannii isolates from a hospital outbreak

An outbreak of colistinresistant Klebsiella pneumoniae carbapenemase-producing Klebsiella pneumoniae in the Netherlands

Actionable diagnosis of neuroleptospirosis by next-generation sequencing

Identification of prosthetic joint infection pathogens using a shotgun metagenomics approach

Chronic meningitis investigated via metagenomic next-generation sequencing

A human gut microbial gene catalogue established by metagenomic sequencing

Optimisation and benchmarking of targeted amplicon sequencing for mycobiome analysis of respiratory specimens

Bacterial genome sequencing in the clinic: bioinformatic challenges and solutions

Engineering bioinformatics: building reliability, performance and productivity into bioinformatics software

Accelerating in silico research with workflows: a lesson in simplicity

Tissue penetration of antifungal agents

Drug-drug interactions of antifungal agents and implications for patient care

Azole resistance in Aspergillus fumigatus: a side-effect of environmental fungicide use?

Triazole resistance in Aspergillus spp.: a worldwide problem

Antifungal resistance: current trends and future strategies to combat

Species identification and antifungal susceptibility testing of Candida bloodstream isolates from population-based surveillance studies in two U.S. cities from

Risk factors for fluconazole-resistant invasive candidiasis in intensive care unit patients: an analysis from the China Survey of Candidiasis study

Epidemiology of candidemia and antifungal susceptibility in invasive Candida species in the Asia-Pacific region

Azole resistance in Aspergillus fumigatus: can we retain the clinical use of mold-active antifungal azoles?

Epidemiology and risk factors for echinocandin nonsusceptible Candida glabrata bloodstream infections: data from a large multisite population-based candidemia surveillance program

Increasing echinocandin resistance in Candida glabrata: clinical failure correlates with presence of FKS mutations and elevated minimum inhibitory concentrations

FKS mutant Candida glabrata: risk factors and outcomes in patients with candidemia

Whole genome sequencing of Candida glabrata for detection of markers of antifungal drug resistance

Identification of genetic markers of resistance to echinocandins, azoles and 5-fluorocytosine in Candida glabrata by next-generation sequencing: a feasibility study

Next-generation sequencing offers new insights into the resistance of Candida spp. to echinocandins and azoles

Implications of multiple freezethawing on respiratory samples for culture-independent analyses

Mycobiome diversity: highthroughput sequencing and identification of fungi

Combined bacterial and fungal intestinal microbiota analyses: impact of storage conditions and DNA extraction protocols

The fungal frontier: a comparative analysis of methods used in the study of the human gut mycobiome

The gut mycobiome of the Human Microbiome Project healthy cohort

Comparison of six extraction techniques for isolation of DNA from filamentous fungi

Effect of DNA extraction methods and sampling techniques on the apparent structure of cow and sheep rumen microbial communities

The fungal cell wall: structure, biosynthesis, and function. Microbiology spectrum

Cell wall dynamics in yeast

Improving molecular detection of fungal DNA in formalin-fixed paraffin-embedded tissues: comparison of five tissue DNA extraction methods using panfungal PCR

Enzymatic treatment of specimens before DNA extraction directly influences molecular detection of infectious agents

Evaluating the impact of DNA extraction method on the representation of human oral bacterial and fungal communities

Evaluation of oral cavity DNA extraction methods on bacterial and fungal microbiota

Comparison of six DNA extraction methods for recovery of fungal DNA as assessed by quantitative PCR

Forgotten fungi-the gut mycobiome in human health and disease

Improved selection of internal transcribed spacer-specific primers enables quantitative, ultra-high-throughput profiling of fungal communities

Current state and perspectives of fungal DNA barcoding and rapid identification procedures

Nuclear ribosomal internal transcribed spacer (ITS) region as a universal DNA barcode marker for Fungi

Shotgun metagenomes and multiple primer pairbarcode combinations of amplicons reveal biases in metabarcoding analyses of fungi

Different amplicon targets for sequencing-based studies of fungal diversity

Mycobiome: approaches to analysis of intestinal fungi

ITS as an environmental DNA barcode for fungi: an in silico approach reveals potential PCR biases

Comparison and validation of some ITS primer pairs useful for fungal metabarcoding studies

Fungal identification biases in microbiome projects

Complementary amplicon-based genomic approaches for the study of fungal communities in humans

New primers to amplify the fungal ITS2 region-evaluation by 454-sequencing of artificial and natural communities

A fungal mock community control for amplicon sequencing experiments

A comprehensive benchmarking study of protocols and sequencing platforms for 16S rRNA community profiling

Reagent and laboratory contamination can critically impact sequence-based microbiome analyses

FUNGuild: an open annotation tool for parsing fungal community datasets by ecological guild

Shotgun metagenomics, from sampling to analysis

Improving saliva shotgun metagenomics by chemical host DNA depletion. Microbiome

Selection of primers for optimal taxonomic classification of environmental 16S rRNA gene sequences

Myco-pathologiaGENOMES: the New 'Home' for the Publication of Fungal Genomes

Large-scale generation and analysis of filamentous fungal DNA barcodes boosts coverage for kingdom fungi and reveals thresholds for fungal species and higher taxon delimitation

Identification of fungi in shotgun metagenomics datasets

Fungal and Bacterial Diversity of Airway Microbiota in Adults with Cystic Fibrosis: concordance Between Conventional Methods and Ultra-Deep Sequencing, and Their Practical use in the Clinical Laboratory

Aseptic technique for cell culture

Activity of antibiotics against Fusarium and Aspergillus

Bacterial inhibition of fungal growth and pathogenicity. Microbial Ecol Health Dis

A handy method to remove bacterial contamination from fungal cultures

Toward the standardization of mycological examination of sputum samples in cystic fibrosis: results from a French multicenter prospective study. Mycopathologia

Challenges in laboratory detection of fungal pathogens in the airways of cystic fibrosis patients

Molecular and phenotypic data supporting distinct species statuses for Scedosporium apiospermum and Pseudallescheria boydii and the proposed new species Scedosporium dehoogii

The sections of Alternaria: formalizing species-group concepts

Identification of pathogenic dematiaceous fungi and related taxa based on large subunit ribosomal DNA D1/D2 domain sequence analysis

Culture-independent molecular methods for detection of antifungal resistance mechanisms and fungal identification

Human Microbiome Project C. Structure function and diversity of the healthy human microbiome

Bacterial and fungal viability in the preterm gut: NEC and sepsis

Development of the human mycobiome over the first month of life and across body sites. mSystems

Immunity to fungal infections

Aspergillus fumigatus morphology and dynamic host interactions

Cultivating our ''frienemies'': viewing immunity as microbiome management

The human microbiome: at the interface of health and disease

Dimensions of biodiversity in the Earth mycobiome

Topographic diversity of fungal and bacterial communities in human skin

Commensal fungi in health and disease

Characterization of the oral fungal microbiome (mycobiome) in healthy individuals

Immunological corollary of the pulmonary mycobiome in bronchiectasis: the CAMEB study

Functional effects of the microbiota in chronic respiratory disease

The emerging importance and challenges of the human mycobiome

Fungi stabilize connectivity in the lung and skin microbial ecosystems. Microbiome

The lung microbiome: key to respiratory Ills?

Response to fungal dysbiosis by gut-resident CX3CR1 ? mononuclear phagocytes aggravates allergic airway disease

Expansion of commensal fungus Wallemia mellicola in the gastrointestinal mycobiota enhances the severity of allergic airway disease in mice

Human anti-fungal Th17 immunity and pathology rely on cross-reactivity against Candida albicans

Development of allergic airway disease in mice following antibiotic therapy and fungal microbiota increase: role of host genetics, antigen, and interleukin-13

Mycobiome in the lower respiratory tract-a clinical perspective

The lung mycobiome: an emerging field of the human respiratory microbiome

The lung mycobiome in the next-generation sequencing era

Corticosteroid treatment is associated with increased filamentous fungal burden in allergic fungal disease

Differences in fungi present in induced sputum samples from asthma patients and nonatopic controls: a community based case control study

Lower airway microbiota and mycobiota in children with severe asthma

Geographic variation in the aetiology, epidemiology and microbiology of bronchiectasis

Distinct 'immuno-allertypes' of disease and high frequencies of sensitisation in non-cystic-fibrosis bronchiectasis

Fungi in bronchiectasis: a concise review

The potential impact of the pulmonary microbiome on immunopathogenesis of Aspergillus related lung disease

The respiratory microbiome of HIV-infected individuals

Topographic diversity of the respiratory tract mycobiome and alteration in HIV and lung disease

The changing microbial epidemiology in cystic fibrosis

The airway microbiota in cystic fibrosis: a complex fungal and bacterial community-implications for therapeutic management

Use of denaturing high-performance liquid chromatography (DHPLC) to characterize the bacterial and fungal airway microbiota of cystic fibrosis patients

Characterization and quantification of the fungal microbiome in serial samples from individuals with cystic fibrosis

Global analysis of the fungal microbiome in cystic fibrosis patients reveals loss of function of the transcriptional repressor Nrg1 as a mechanism of pathogen adaptation

Cohort Study of Airway Mycobiome in Adult Cystic Fibrosis Patients: differences in Community Structure between Fungi and Bacteria Reveal Predominance of Transient Fungal Elements

The human lung and Aspergillus: You are what you breathe in?

Mycobiome sequencing and analysis applied to fungal community profiling of the lower respiratory tract during fungal pathogenesis

Characterizing the human mycobiota: a comparison of small subunit rRNA, ITS1, ITS2, and large subunit rRNA genomic targets

Dysbiosis of gut fungal microbiota is associated with mucosal inflammation in Crohn's disease

Fungi and inflammatory bowel diseases: alterations of composition and diversity

Fungal microbiota dysbiosis in IBD

Bacteriome and mycobiome interactions underscore microbial dysbiosis in familial Crohn's disease

Fungal dysbiosis in mucosa-associated microbiota of Crohn's disease patients

Malassezia is associated with Crohn's disease and exacerbates colitis in mouse models

Immunological consequences of intestinal fungal dysbiosis

Enterobacteriaceae are essential for the modulation of colitis severity by fungi. Microbiome

The fungal microbiota of de-novo paediatric inflammatory bowel disease

Fungal signature in the gut microbiota of pediatric patients with inflammatory bowel disease

The potential role of gut mycobiome in irritable bowel syndrome

Intestinal fungal dysbiosis is associated with visceral hypersensitivity in patients with irritable bowel syndrome and rats. Gastroenterology

Reversal of visceral hypersensitivity in rat by Menthacarin Ò , a proprietary combination of essential oils from peppermint and caraway, coincides with mycobiome modulation

The fungal mycobiome promotes pancreatic oncogenesis via activation of MBL

Enteric fungal microbiota dysbiosis and ecological alterations in colorectal cancer

Dysbiosis of fungal microbiota in the intestinal mucosa of patients with colorectal adenomas

Gastrointestinal inflammation and associated immune activation in schizophrenia

Candida albicans exposures, sex specificity and cognitive deficits in schizophrenia and bipolar disorder

Altered gut microbiota in Rett syndrome

New evidences on the altered gut microbiota in autism spectrum disorders

The microbiome-gut-brain axis in health and disease

Dysfunctional cognitions, anxiety and depression in irritable bowel syndrome

Staged development of long-lived T-cell receptor alphabeta TH17 resident memory T-cell population to Candida albicans after skin infection

Invasive candidiasis: from mycobiome to infection, therapy, and prevention

Diverse human skin fungal communities in children converge in adulthood

Redefining the chronic-wound microbiome: fungal communities are prevalent, dynamic, and associated with delayed healing

Immunity to commensal fungi: detente and disease

The role of the skin and gut microbiome in psoriatic disease

High Rhodotorula sequences in skin transcriptome of patients with diffuse systemic sclerosis

Topographical and physiological differences of the skin mycobiome in health and disease

Characterization of the fungal microbiota (mycobiome) in healthy and dandruff-afflicted human scalps

Extracellular nanovesicles released from the commensal yeast Malassezia sympodialis are enriched in allergens and interact with cells in human skin

Analysis of the skin mycobiome in adult patients with atopic dermatitis

Identification of small RNAs in extracellular vesicles from the commensal yeast Malassezia sympodialis

The skin commensal yeast malassezia triggers a type 17 response that coordinates anti-fungal immunity and exacerbates skin inflammation

The microbiomes of a XVIII century mummy from the castle of Krásna Hôrka (Slovakia) and its surrounding environment

Skin fungal community and its correlation with bacterial community of urban Chinese individuals

Effect of an emollient on the mycobiome of atopic dermatitis patients

A fungal world: could the gut mycobiome be involved in neurological disease?

The gut microbiome in human neurological disease: a review

Multiple sclerosis and mixed microbial infections. Direct identification of fungi and bacteria in nervous tissue

Alterations of the human gut microbiome in multiple sclerosis

Gut microbiota composition and relapse risk in pediatric MS: a pilot study

Gut microbiota in early pediatric multiple sclerosis: a case-control study

Metagenomic analysis of cerebrospinal fluid from patients with multiple sclerosis

Cerebrospinal fluid in a small cohort of patients with multiple sclerosis was generally free of microbial DNA

Different brain regions are infected with fungi in Alzheimer's disease

Infection of fungi and bacteria in brain tissue from elderly persons and patients with Alzheimer's disease

Fungal infection in neural tissue of patients with amyotrophic lateral sclerosis

Malassezia and Parkinson's disease

Larenas-Linnemann D, Phipatanakul W. Exposure and health effects of fungi on humans

Submicron fungal fragments as another indoor biocontaminant in elementary schools

Dispersal in microbes: fungi in indoor air are dominated by outdoor air and show dispersal limitation at short distances

Microbial communities in the tropical air ecosystem follow a precise diel cycle

Sources of airborne microorganisms in the built environment

Ecological succession of the microbial communities of an air-conditioning cooling coil in the tropics

Annotating public fungal ITS sequences from the built environment according to the MIxS-Built Environment

Fundamentals of mold growth in indoor environments and strategies for healthy living

Taxonomic annotation of public fungal ITS sequences from the built environment -a report from an

Indoor fungal composition is geographically patterned and more diverse in temperate zones than in the tropics

Utilizing pyrosequencing and quantitative PCR to characterize fungal populations among house dust samples

Fungi and allergic lower respiratory tract diseases

Correlation between the prevalence of certain fungi and sick building syndrome

Studies on the role of fungi in Sick Building Syndrome

Indoor biological contaminants and symptoms of sick building syndrome in office buildings in Mauritius

City-scale distribution and dispersal routes of mycobiome in residences

The diversity and distribution of fungi on residential surfaces

Building materials with antifungal efficacy enriched with silver nanoparticles

Antifungal efficiency assessment of the TiO2 coating on facade paints

Ten questions concerning the microbiomes of buildings

Role of the mycobiome in human acute graft-versus-host disease

Interactions between commensal fungi and the C-type lectin receptor Dectin-1 influence colitis

The mammalian mycobiome: a complex system in a dynamic relationship with the host

Mode and place of delivery, gastrointestinal microbiota, and their influence on asthma and atopy

Allergy development and the intestinal microflora during the first year of life

The role of the microbiome in asthma: the gut(-)lung axis

Intestinal dysbiosis and yeast isolation in stool of subjects with autism spectrum disorders. Mycopathologia

Gut microbiota regulate motor deficits and neuroinflammation in a model of Parkinson's disease

Neglected endemic mycoses

ESCMID and ECMM joint clinical guidelines for the diagnosis and management of mucormycosis 2013

Brazilian guidelines for the clinical management of paracoccidioidomycosis

Hidden killers: human fungal infections

Pulmonary aspergillosis: a clinical review

Practice guidelines for the diagnosis and management of aspergillosis: 2016 update by the Infectious Diseases Society of America

Isavuconazole treatment for rare fungal diseases and for invasive aspergillosis in patients with renal impairment: challenges and lessons of the VITAL trial

Fungal infections of the central nervous system

A retrospective series of gut aspergillosis in haematology patients

Cutaneous aspergillosis

Changes in incidence and antifungal drug resistance in candidemia: results from populationbased laboratory surveillance in Atlanta and Baltimore

Excess mortality, hospital stay, and cost due to candidemia: a case-control study using data from population-based candidemia surveillance

Candida and invasive mould diseases in nonneutropenic critically ill patients and patients with haematological cancer

Ocular manifestations of candidemia

Clinical practice guidelines for the management of cryptococcal disease: 2010 update by the infectious diseases society of america

Epidemiology and outcome of zygomycosis: a review of 929 reported cases

Mucormycosis in immunochallenged patients

Pulmonary mucormycosis: a case report and review of the literature

Cutaneous mucormycosis

Gastrointestinal mucormycosis in immunocompromised hosts

ECIL guidelines for treatment of Pneumocystis jirovecii pneumonia in non-HIV-infected haematology patients

Extrapulmonary pneumocystosis

Pneumocystis carinii infection of the small intestine

Blastomycosis mortality rates

Clinical manifestations and treatment of blastomycosis

Clinical practice guidelines for the management of blastomycosis: 2008 update by the Infectious Diseases Society of America

Hospitalizations for endemic mycoses: a population-based national study

Clinical perspectives in the diagnosis and management of histoplasmosis

Clinical practice guidelines for the management of patients with histoplasmosis: 2007 update by the Infectious Diseases Society of America

Infectious Diseases Society of America (IDSA) clinical practice guideline for the treatment of coccidioidomycosis

Coccidioidomycosis and the skin: a comprehensive review

Coccidioidomycosis of bone and joints

Disseminated coccidioidomycosis with multifocal musculoskeletal disease involvement. Radiol Case Rep

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Acknowledgements The authors would like to acknowledge The Academic Respiratory Initiative for Pulmonary Health (TARIPH) for collaboration support. 

Conflict of interest The authors declare that they have no conflict of interest.