Сравнение методов

Просматривайте выбранные методы рядом; строки с различиями подсвечены.

	Анализ временных рядов разнообразия микробиома ×	Анализ дифференциальной экспрессии РНК-сек (DE)×
Область	Биоинформатика	Биоинформатика
Семейство	Process / pipeline	Process / pipeline
Год появления≠	2010s (formalized with 16S amplicon sequencing era; expanded ~2012–2020)	2008–2010 (RNA-seq DE methodology established)
Автор метода≠	Developed iteratively through the microbiome research community; key contributions from Susan Holmes, Rob Knight, and colleagues	Multiple groups; foundational methods from Anders & Huber (DESeq, 2010), Robinson, McCarthy & Smyth (edgeR, 2010)
Тип≠	Longitudinal observational / bioinformatics pipeline	Quantitative genomics pipeline
Основополагающий источник≠	Callahan, B. J., McMurdie, P. J., Rosen, M. J., Han, A. W., Johnson, A. J. A., & Holmes, S. P. (2016). DADA2: High-resolution sample inference from Illumina amplicon data. Nature Methods, 13(7), 581–583. DOI ↗	Love, M. I., Huber, W., & Anders, S. (2014). Moderated estimation of fold change and dispersion for RNA-seq data with DESeq2. Genome Biology, 15(12), 550. DOI ↗
Другие названия	longitudinal microbiome diversity analysis, temporal microbiome analysis, repeated-measures microbiome diversity, time-course microbiome analysis	RNA-seq DE analysis, transcriptomic differential expression, bulk RNA-seq DE, DEA
Связанные≠	5	6
Сводка≠	Time-series microbiome diversity analysis tracks how the richness, evenness, and community composition of microbial communities change across multiple time points within the same subjects. By combining standard diversity metrics with longitudinal statistical models, it separates true temporal dynamics from inter-individual variation, identifying when and how perturbations such as diet changes, antibiotic treatment, or disease onset reshape the microbiome.	RNA-seq differential expression (DE) analysis identifies genes whose transcript abundance differs significantly between two or more biological conditions — for example, treated versus control, or diseased versus healthy tissue. Starting from raw sequencing reads, the pipeline moves through alignment, count-based normalization, statistical modeling of count dispersion, hypothesis testing, and multiple-testing correction to produce a ranked list of differentially expressed genes accompanied by fold-change estimates and adjusted p-values.
ScholarGateНабор данных ↗	v1 2 Источники PUBLISHED	v1 2 Источники PUBLISHED

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