Your search keyword '"DeRisi JL"' showing total 4 results

1. Genomic and serologic characterization of enterovirus A71 brainstem encephalitis

Author

Leon KE, Schubert RD, Casas-Alba D, Hawes IA, Ramachandran PS, Ramesh A, Pak JE, Wu W, Cheung CK, Crawford ED, Khan LM, Launes-Montana C, Sample HA, Zorn KC, Cabrerizo M, Valero-Rello A, Langelier C, Munoz-Almagro C, DeRisi JL, and Wilson MR

Abstract

OBJECTIVE: In 2016, Catalonia experienced a pediatric brainstem encephalitis outbreak caused by enterovirus A71 (EV-A71). Conventional testing identified EV in the periphery but rarely in CSF. Metagenomic next-generation sequencing (mNGS) and CSF pan-viral serology (VirScan) were deployed to enhance viral detection and characterization. METHODS: RNA was extracted from the CSF (n = 20), plasma (n = 9), stool (n = 15), and nasopharyngeal samples (n = 16) from 10 children with brainstem encephalitis and 10 children with meningitis or encephalitis. Pathogens were identified using mNGS. Available CSF from cases (n = 12) and pediatric other neurologic disease controls (n = 54) were analyzed with VirScan with a subset (n = 9 and n = 50) validated by ELISA. RESULTS: mNGS detected EV in all samples positive by quantitative reverse transcription polymerase chain reaction (qRT-PCR) (n = 25). In qRT-PCR-negative samples (n = 35), mNGS found virus in 23% (n = 8, 3 CSF samples). Overall, mNGS enhanced EV detection from 42% (25/60) to 57% (33/60) (p-value = 0.013). VirScan and ELISA increased detection to 92% (11/12) compared with 46% (4/12) for CSF mNGS and qRT-PCR (p-value = 0.023). Phylogenetic analysis confirmed the EV-A71 strain clustered with a neurovirulent German EV-A71. A single amino acid substitution (S241P) in the EVA71 VP1 protein was exclusive to the CNS in one subject. CONCLUSION: mNGS with VirScan significantly increased the CNS detection of EVs relative to qRT-PCR, and the latter generated an antigenic profile of the acute EV-A71 immune response. Genomic analysis confirmed the close relation of the outbreak EV-A71 and neuroinvasive German EV-A71. A S241P substitution in VP1 was found exclusively in the CSF.

Published

2020

2. Chronic Meningitis Investigated via Metagenomic Next-Generation Sequencing

Author

Wilson, MR, O'Donovan, BD, Gelfand, JM, Sample, HA, Chow, FC, Betjemann, JP, Shah, MP, Richie, MB, Gorman, MP, Hajj-Ali, RA, Calabrese, LH, Zorn, KC, Chow, ED, Greenlee, JE, Blum, JH, Green, G, Khan, LM, Banerji, D, Langelier, C, Bryson-Cahn, C, Harrington, W, Lingappa, JR, Shanbhag, NM, Green, AJ, Brew, BJ, Soldatos, A, Strnad, L, Doernberg, SB, Jay, CA, Douglas, V, Josephson, SA, and DeRisi, JL

Subjects

Adult, Male, Adolescent, Cryptococcal, Aspergillus oryzae, Histoplasma, HIV Infections, Neurocysticercosis, Young Adult, Taenia solium, Genetics, Animals, Humans, Meningitis, Child, Histoplasmosis, Candida, Neuroaspergillosis, Candidiasis, Neurosciences, High-Throughput Nucleotide Sequencing, Middle Aged, Emerging Infectious Diseases, Infectious Diseases, Chronic Disease, HIV-1, Cryptococcus neoformans, RNA, Metagenome, Female, Metagenomics, Infection, Sequence Analysis

Abstract

Importance:Identifying infectious causes of subacute or chronic meningitis can be challenging. Enhanced, unbiased diagnostic approaches are needed. Objective:To present a case series of patients with diagnostically challenging subacute or chronic meningitis using metagenomic next-generation sequencing (mNGS) of cerebrospinal fluid (CSF) supported by a statistical framework generated from mNGS of control samples from the environment and from patients who were noninfectious. Design, Setting, and Participants:In this case series, mNGS data obtained from the CSF of 94 patients with noninfectious neuroinflammatory disorders and from 24 water and reagent control samples were used to develop and implement a weighted scoring metric based on z scores at the species and genus levels for both nucleotide and protein alignments to prioritize and rank the mNGS results. Total RNA was extracted for mNGS from the CSF of 7 participants with subacute or chronic meningitis who were recruited between September 2013 and March 2017 as part of a multicenter study of mNGS pathogen discovery among patients with suspected neuroinflammatory conditions. The neurologic infections identified by mNGS in these 7 participants represented a diverse array of pathogens. The patients were referred from the University of California, San Francisco Medical Center (n = 2), Zuckerberg San Francisco General Hospital and Trauma Center (n = 2), Cleveland Clinic (n = 1), University of Washington (n = 1), and Kaiser Permanente (n = 1). A weighted z score was used to filter out environmental contaminants and facilitate efficient data triage and analysis. Main Outcomes and Measures:Pathogens identified by mNGS and the ability of a statistical model to prioritize, rank, and simplify mNGS results. Results:The 7 participants ranged in age from 10 to 55 years, and 3 (43%) were female. A parasitic worm (Taenia solium, in 2 participants), a virus (HIV-1), and 4 fungi (Cryptococcus neoformans, Aspergillus oryzae, Histoplasma capsulatum, and Candida dubliniensis) were identified among the 7 participants by using mNGS. Evaluating mNGS data with a weighted z score-based scoring algorithm reduced the reported microbial taxa by a mean of 87% (range, 41%-99%) when taxa with a combined score of 0 or less were removed, effectively separating bona fide pathogen sequences from spurious environmental sequences so that, in each case, the causative pathogen was found within the top 2 scoring microbes identified using the algorithm. Conclusions and Relevance:Diverse microbial pathogens were identified by mNGS in the CSF of patients with diagnostically challenging subacute or chronic meningitis, including a case of subarachnoid neurocysticercosis that defied diagnosis for 1 year, the first reported case of CNS vasculitis caused by Aspergillus oryzae, and the fourth reported case of C dubliniensis meningitis. Prioritizing metagenomic data with a scoring algorithm greatly clarified data interpretation and highlighted the problem of attributing biological significance to organisms present in control samples used for metagenomic sequencing studies.

Published

2018

3. Acute West Nile Virus Meningoencephalitis Diagnosed Via Metagenomic Deep Sequencing of Cerebrospinal Fluid in a Renal Transplant Patient

Author

Wilson, MR, Zimmermann, LL, Crawford, ED, Sample, HA, Soni, PR, Baker, AN, Khan, LM, and DeRisi, JL

Subjects

Graft Rejection, basic (laboratory) research/science, diagnostic techniques and imaging, infection and infectious agents, Kidney Disease, Adolescent, viruses, infectious disease, kidney transplantation/nephrology, kidney (allograft) function/dysfunction, Kidney Function Tests, clinical research/practice, Medical and Health Sciences, West Nile [viral], Vaccine Related, Kidney Failure, Immunocompromised Host, Rare Diseases, Clinical Research, Meningoencephalitis, Risk Factors, Biodefense, genomics, Humans, Epstein-Barr Virus [viral], genetics, Chronic, Prevention, Graft Survival, Neurosciences, High-Throughput Nucleotide Sequencing, Prognosis, Kidney Transplantation, Vector-Borne Diseases, Emerging Infectious Diseases, Infectious Diseases, Orphan Drug, Good Health and Well Being, Female, Surgery, Metagenomics, Infection, West Nile virus, West Nile Fever, Immunosuppressive Agents, Glomerular Filtration Rate

Abstract

© 2016 The Authors. American Journal of Transplantation published by Wiley Periodicals, Inc. on behalf of American Society of Transplant Surgeons Solid organ transplant patients are vulnerable to suffering neurologic complications from a wide array of viral infections and can be sentinels in the population who are first to get serious complications from emerging infections like the recent waves of arboviruses, including West Nile virus, Chikungunya virus, Zika virus, and Dengue virus. The diverse and rapidly changing landscape of possible causes of viral encephalitis poses great challenges for traditional candidate-based infectious disease diagnostics that already fail to identify a causative pathogen in approximately 50% of encephalitis cases. We present the case of a 14-year-old girl on immunosuppression for a renal transplant who presented with acute meningoencephalitis. Traditional diagnostics failed to identify an etiology. RNA extracted from her cerebrospinal fluid was subjected to unbiased metagenomic deep sequencing, enhanced with the use of a Cas9-based technique for host depletion. This analysis identified West Nile virus (WNV). Convalescent serum serologies subsequently confirmed WNV seroconversion. These results support a clear clinical role for metagenomic deep sequencing in the setting of suspected viral encephalitis, especially in the context of the high-risk transplant patient population.

Published

2017

4. Programmable Microfluidic Synthesis of Over One Thousand Uniquely Identifiable Spectral Codes

Author

Nguyen, HQ, Baxter, BC, Brower, K, Diaz-Botia, CA, DeRisi, JL, Fordyce, PM, and Thorn, KS

Subjects

Lanthanides, Spectral Encoding, Optical Physics, Materials Engineering, Microparticles, Electrical and Electronic Engineering, Multiplexing, Biotechnology

Abstract

Encoded microparticles have become a powerful tool for a wide array of applications, including high-throughput sample tracking and massively parallel biological multiplexing. Spectral encoding, where particles are encoded with distinct luminescence spectra, provides a particularly appealing encoding strategy because of the ease of reading codes and assay flexibility. To date, spectral encoding has been limited in the number of codes that can be accurately resolved. Here, we demonstrate an automated 5-dimensional spectral encoding scheme using lanthanide nanophosphors that is capable of producing isotropic spherical microparticles with up to 1,100 unique codes, which we term MRBLEs (Microspheres with Ratiometric Barcode Lanthanide Encoding). We further develop a quantitative framework for evaluating global ability to distinguish codes and demonstrate that for six different sets of MRBLEs ranging from 106 to 1,101 codes in size, > 98% of MRBLEs can be assigned to a code with 99.99% confidence. These > 1,000 code sets represent the largest spectral code libraries built to date. We expect that these MRBLEs will enable a wide variety of novel multiplexed assays.

Published

2017