AUTHOR=McTaggart Lisa R. , Copeland Julia K. , Surendra Anuradha , Wang Pauline W. , Husain Shahid , Coburn Bryan , Guttman David S. , Kus Julianne V. 

TITLE=Mycobiome Sequencing and Analysis Applied to Fungal Community Profiling of the Lower Respiratory Tract During Fungal Pathogenesis

JOURNAL=Frontiers in Microbiology

VOLUME=10

YEAR=2019

URL=https://www.frontiersin.org/journals/microbiology/articles/10.3389/fmicb.2019.00512

DOI=10.3389/fmicb.2019.00512

ISSN=1664-302X

ABSTRACT=<p>Invasive fungal infections are an increasingly important cause of human morbidity and mortality. We generated a next-generation sequencing (NGS)-based method designed to detect a wide range of fungi and applied it to analysis of the fungal microbiome (mycobiome) of the lung during fungal infection. Internal transcribed spacer 1 (ITS1) amplicon sequencing and a custom analysis pipeline detected 96% of species from three mock communities comprised of potential fungal lung pathogens with good recapitulation of the expected species distributions (Pearson correlation coefficients <italic>r</italic> = 0.63, <italic>p</italic> = 0.004; <italic>r</italic> = 0.71, <italic>p</italic> &lt; 0.001; <italic>r</italic> = 0.62, <italic>p</italic> = 0.002). We used this pipeline to analyze mycobiomes of bronchoalveolar lavage (BAL) specimens classified as culture-negative (<italic>n</italic> = 50) or culture-positive (<italic>n</italic> = 39) for <italic>Blastomyces dermatitidis/gilchristii</italic>, the causative agent of North America blastomycosis. Detected in 91.4% of the culture-positive samples, <italic>Blastomyces</italic> dominated (&gt;50% relative abundance) the mycobiome in 68.6% of these culture-positive samples but was absent in culture-negative samples. To overcome any bias in relative abundance due to between-sample variation in fungal biomass, an abundance-weighting calculation was used to normalize the data by accounting for sample-specific PCR cycle number and PCR product concentration data utilized during sample preparation. After normalization, there was a statistically significant greater overall abundance of ITS1 amplicon in the <italic>Blastomyces</italic>-culture-positive samples versus culture-negative samples. Moreover, the normalization revealed a greater biomass of yeast and environmental fungi in several <italic>Blastomyces</italic>-culture-positive samples than in the culture-negative samples. Successful detection of <italic>Coccidioides</italic>, <italic>Scedosporium</italic>, <italic>Phaeoacremonium</italic>, and <italic>Aspergillus</italic> in 6 additional culture-positive BALs by ITS1 amplicon sequencing demonstrates the ability of this method to detect a broad range of fungi from clinical specimens, suggesting that it may be a potentially useful adjunct to traditional fungal microbiological testing for the diagnosis of respiratory mycoses.</p>