A theoretical and generalized approach for the assessment of the sample-specific limit of detection for clinical metagenomics

基因组 计算生物学 背景(考古学) 极限(数学) 生物 灵敏度(控制系统) 样本量测定 k-mer公司 病毒 检出限 基因组 计算机科学 统计 数学 基因 病毒学 遗传学 数学分析 古生物学 电子工程 工程类
作者
Arnt Ebinger,Susanne Fischer,Dirk W. Höper
出处
期刊:Computational and structural biotechnology journal [Elsevier]
卷期号:19: 732-742 被引量:20
标识
DOI:10.1016/j.csbj.2020.12.040
摘要

Metagenomics is a powerful tool to identify novel or unexpected pathogens, since it is generic and relatively unbiased. The limit of detection (LOD) is a critical parameter for the routine application of methods in the clinical diagnostic context. Although attempts for the determination of LODs for metagenomics next-generation sequencing (mNGS) have been made previously, these were only applicable for specific target species in defined samples matrices. Therefore, we developed and validated a generalized probability-based model to assess the sample-specific LOD of mNGS experiments (LODmNGS). Initial rarefaction analyses with datasets of Borna disease virus 1 human encephalitis cases revealed a stochastic behavior of virus read detection. Based on this, we transformed the Bernoulli formula to predict the minimal necessary dataset size to detect one virus read with a probability of 99%. We validated the formula with 30 datasets from diseased individuals, resulting in an accuracy of 99.1% and an average of 4.5 ± 0.4 viral reads found in the calculated minimal dataset size. We demonstrated by modeling the virus genome size, virus-, and total RNA-concentration that the main determinant of mNGS sensitivity is the virus-sample background ratio. The predicted LODmNGS for the respective pathogenic virus in the datasets were congruent with the virus-concentration determined by RT-qPCR. Theoretical assumptions were further confirmed by correlation analysis of mNGS and RT-qPCR data from the samples of the analyzed datasets. This approach should guide standardization of mNGS application, due to the generalized concept of LODmNGS.

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