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Validation of Metagenomic Next-Generation Sequencing Tests for Universal Pathogen Detection
Identifier
026766
Type of Spiritual Experience
Background
A description of the experience
Arch Pathol Lab Med. 2017 Jun;141(6):776-786. doi: 10.5858/arpa.2016-0539-RA. Epub 2017 Feb 7.
Validation of Metagenomic Next-Generation Sequencing Tests for Universal Pathogen Detection.
Schlaberg R1, Chiu CY1, Miller S1, Procop GW1, Weinstock G1; Professional Practice Committee and Committee on Laboratory Practices of the American Society for Microbiology1; Microbiology Resource Committee of the College of American Pathologists1.
Abstract
CONTEXT:
- Metagenomic sequencing can be used for detection of any pathogens using unbiased, shotgun next-generation sequencing (NGS), without the need for sequence-specific amplification. Proof-of-concept has been demonstrated in infectious disease outbreaks of unknown causes and in patients with suspected infections but negative results for conventional tests. Metagenomic NGS tests hold great promise to improve infectious disease diagnostics, especially in immunocompromised and critically ill patients.
OBJECTIVE:
- To discuss challenges and provide example solutions for validating metagenomic pathogen detection tests in clinical laboratories. A summary of current regulatory requirements, largely based on prior guidance for NGS testing in constitutional genetics and oncology, is provided.
DATA SOURCES:
- Examples from 2 separate validation studies are provided for steps from assay design, and validation of wet bench and bioinformatics protocols, to quality control and assurance.
CONCLUSIONS:
- Although laboratory and data analysis workflows are still complex, metagenomic NGS tests for infectious diseases are increasingly being validated in clinical laboratories. Many parallels exist to NGS tests in other fields. Nevertheless, specimen preparation, rapidly evolving data analysis algorithms, and incomplete reference sequence databases are idiosyncratic to the field of microbiology and often overlooked.
PMID:
28169558
DOI:
10.5858/arpa.2016-0539-RA