Analysis and Interpretation of metagenomics data: an approach

Navgire, Gauri S; Goel, Neha; Sawhney, Gifty; Sharma, Mohit; Kaushik, Prashant; Mohanta, Yugal Kishore; Mohanta, Tapan Kumar; Al‐Harrasi, Ahmed

doi:10.1186/s12575-022-00179-7

Cited by 36 publications

(11 citation statements)

References 117 publications

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“…Researchers must weigh the trade-offs between DNA quantity and potential biases introduced by different kits. Differences in bacterial community composition and e ciency in lysis may signi cantly impact downstream applications, particularly in metagenomic studies, where accurate representation of microbial diversity is paramount (Navgire et al 2022). Hence, researchers should choose a kit that aligns with the goals and nuances of their speci c study design.…”

Section: Discussionmentioning

confidence: 99%

Comparative analysis of commercially available metagenomic kits for optimal DNA extraction from bovine fecal samples

PS,

Kumaresan,

et al. 2024

Preprint

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In the field of metagenomic research, the choice of DNA extraction methods plays a pivotal yet often underestimated role in shaping the reliability and interpretability of microbial community data. This study delves into the impact of five commercially available metagenomic DNA extraction kits on the analysis of bovine fecal microbiota. Recognizing the centrality of accurate DNA extraction in elucidating microbial community dynamics, we systematically assessed DNA yield, quality, and microbial composition across these kits. Notably, the FastDNA spin soil kit yielded the highest DNA concentration, while significant variations in quality were observed across kits. Furthermore, differential abundance analysis revealed kit-specific biases, impacting taxa representation. Microbial richness and diversity were significantly influenced by the choice of extraction kit, with QIAamp DNA stool minikit, QIAamp Power Pro, and DNeasy PowerSoil outperforming the Stool DNA Kit. Principal-coordinate analysis revealed distinct clustering based on DNA isolation procedures, particularly highlighting the unique microbial community composition derived from the Stool DNA Kit. Differential abundance analysis showcased kit-specific biases, influencing taxa representation. This study also addressed practical implications, demonstrating how kit selection influences the accurate identification of spiked bacteria. In essence, our research highlights the need for meticulous consideration of DNA extraction kits in metagenomic studies, offering valuable insights for researchers striving to advance the precision and depth of microbiota analyses in animals.

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Section: Discussionmentioning

confidence: 99%

Comparative analysis of commercially available metagenomic kits for optimal DNA extraction from bovine fecal samples

PS,

Kumaresan,

et al. 2024

Preprint

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“…Metagenomic analysis enables the analysis of DNA segments from multiple microorganisms without the need for culture and is carried out using either an amplicon or shotgun-based approach. 17 Previously, shortread sequencing of the bacterial 16S rRNA gene has been the standard method for microbiome profiling; however, recently long-read sequencing method has been employed to achieve a more comprehensive microbiome profiling. 18 Long-read methods offer higher detection confidence than short-read methods do.…”

Section: Discussionmentioning

confidence: 99%

Comparative evaluation of 16S rRNA metagenomic sequencing in the diagnosis and understanding of bacterial endophthalmitis

Asao,

Hashida,

Maruyama

et al. 2023

BMJ Open Ophth

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ObjectiveTo evaluate the usefulness of metagenomic analysis in the search for causative organisms of bacterial endophthalmitis.Methods and analysisTwenty-one consecutive treatment-naïve patients (13 men and 8 women; mean age, 60.8±19.8 years) with suspected endophthalmitis were recruited. Vitrectomy was performed to diagnose and treat endophthalmitis. Bacterial culture and metagenomic analysis of the vitreous body were performed. Extracted DNA was analysed using 16S rRNA sequences, and libraries were sequenced on an Illumina MiSeq sequencer. To compare the bacterial composition in each case, α and β diversities were determined.ResultsPatients were categorised into three groups: endophthalmitis cases with matching predominant organisms according to metagenomic analysis and bacterial culture, those with negative results for bacterial culture and those with negative results in both cases. In 7 of 15 culture-negative cases, results from metagenomic analysis could detect pathogens. The diversity of bacterial populations was significantly lower in the group with positive results for predominant bacteria according to culture and metagenomic analysis. All patients with uveitis were included in the group for which the causative pathogen could not be determined by culture or metagenomic analysis. The structures of bacterial populations significantly differed between the positive and negative groups by culture and metagenomic analysis.ConclusionsMetagenomic analysis could be useful for prompt detection of causative pathogens, for precise diagnosis of infection, and as a marker of inflammation processes such as uveitis.

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“…Metagenomics has enabled the identification of specific microbial species or groups that potentially benefit cereals (refer to Table 2 ). These studies provide valuable information on functional gene annotation within the cereal microbiome [ 91 ]. By comparing metagenomic sequences to reference databases, researchers can identify genes involved in various functions, such as nutrient cycling, plant growth promotion, disease suppression, and stress tolerance [ 92 ].…”

Section: Metagenomics: An Overviewmentioning

confidence: 99%

Exploring Cereal Metagenomics: Unravelling Microbial Communities for Improved Food Security

Masenya,

Manganyi,

Dikobe

2024

Microorganisms

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Food security is an urgent global challenge, with cereals playing a crucial role in meeting the nutritional requirements of populations worldwide. In recent years, the field of metagenomics has emerged as a powerful tool for studying the microbial communities associated with cereal crops and their impact on plant health and growth. This chapter aims to provide a comprehensive overview of cereal metagenomics and its role in enhancing food security through the exploration of beneficial and pathogenic microbial interactions. Furthermore, we will examine how the integration of metagenomics with other tools can effectively address the adverse effects on food security. For this purpose, we discuss the integration of metagenomic data and machine learning in providing novel insights into the dynamic interactions shaping plant-microbe relationships. We also shed light on the potential applications of leveraging microbial diversity and epigenetic modifications in improving crop resilience and yield sustainability. Ultimately, cereal metagenomics has revolutionized the field of food security by harnessing the potential of beneficial interactions between cereals and their microbiota, paving the way for sustainable agricultural practices.

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Analysis and Interpretation of metagenomics data: an approach

Cited by 36 publications

References 117 publications

Comparative analysis of commercially available metagenomic kits for optimal DNA extraction from bovine fecal samples

Comparative analysis of commercially available metagenomic kits for optimal DNA extraction from bovine fecal samples

Comparative evaluation of 16S rRNA metagenomic sequencing in the diagnosis and understanding of bacterial endophthalmitis

Exploring Cereal Metagenomics: Unravelling Microbial Communities for Improved Food Security

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