Sequencing by Binding rivals error-corrected Sequencing by Synthesis technology for accurate detection and quantification of minor (<0.1%) subpopulation variants.

Allender, Christopher J; Wike, Candice; Ellis, Dean; Lemmer, Darrin; Porter, Tanner; Pond, Stephanie J K; Engelthaler, David M

Allender, Christopher J; Wike, Candice; Ellis, Dean; Lemmer, Darrin; Porter, Tanner; Pond, Stephanie J K; Engelthaler, David M.

Afiliación

Allender CJ; Translational Genomics Research Institute.
Wike C; Translational Genomics Research Institute.
Ellis D; Translational Genomics Research Institute.
Lemmer D; Translational Genomics Research Institute.
Porter T; Translational Genomics Research Institute.
Pond SJK; Translational Genomics Research Institute.
Engelthaler DM; Translational Genomics Research Institute.

Res Sq ; 2024 May 21.

Article en En | MEDLINE | ID: mdl-38826386

ABSTRACT

ABSTRACT

Detecting very minor (< 1%) subpopulations using next-generation sequencing is a critical need for multiple applications including detection of drug resistant pathogens and somatic variant detection in oncology. To enable these applications, wet lab enhancements and bioinformatic error correction methods have been developed for 'sequencing by synthesis' technology to reduce its inherent sequencing error rate. A recently available sequencing approach termed 'sequencing by binding' claims to have higher base calling accuracy data "out of the box." This paper evaluates the utility of using 'sequencing by binding' for the detection of ultra-rare subpopulations down to 0.001%.

Palabras clave

NGS benchmarking; heteroresistance; sequencing by binding (SBB); sequencing by synthesis (SBS); single molecule overlapping reads (SMOR); tuberculosis (TB); ultra-rare mutation detection

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