Bacterial meta-analysis of chicken cecal microbiota

Luis Alberto Chica Cardenas; Viviana Clavijo; Martha Vives; Alejandro Reyes

doi:10.7717/peerj.10571

Bacterial meta-analysis of chicken cecal microbiota

PeerJ. 2021 Jan 5:9:e10571. doi: 10.7717/peerj.10571. eCollection 2021.

Authors

Luis Alberto Chica Cardenas^{1

2}, Viviana Clavijo³, Martha Vives³, Alejandro Reyes^{1

2

4}

Affiliations

¹ Research Group on Computational Biology and Microbial Ecology, Department of Biological Sciences, Universidad de Los Andes, Bogotá, Colombia.
² Max Planck Tandem Group in Computational Biology, Universidad de Los Andes, Bogotá, Colombia.
³ Centro de Investigaciones Microbiológicas, Department of Biological Sciences, Universidad de Los Andes, Bogotá, Colombia.
⁴ The Edison Family Center for Genome Sciences and Systems Biology, Washington University School of Medicine, St. Louis, MO, USA.

Abstract

Poultry production is an industry that generates 90,000 metric tons of chicken meat worldwide. Thus, optimizing chicken growth and sustainable production is of great importance. A central factor determining not only production parameters, but also stability of the immune system and chicken health, is the diversity and variability of the microbiota present throughout the gastrointestinal tract. To date, several studies have investigated the relationship between bacterial communities and the gut microbiome, with limited data to compare. This study aims to create a bacterial meta-analysis based on studies using amplicon sequencing with Illumina sequencing technologies in order to build a baseline for comparison in future analyses of the cecal bacterial composition in chicken. A systematic literature review was performed (SYRF ID: e84f0468-e418-4eec-9da4-b517f1b4809d. Full project URL: https://app.syrf.org.uk/projects/e84f0468-e418-4eec-9da4-b517f1b4809d/detail). From all the available and analyzed manuscripts only nine contained full raw-sequence data available and the corresponding metadata. A total of 324 samples, comprising three different regions within the 16S rRNA gene, were analyzed. Due to the heterogeneity of the data, each region was analyzed independently and an effort for a joint analysis was performed as well. Taxonomic profiling revealed 11 phyla, with Firmicutes as the most prevalent phylum, followed by Bacteroidetes and Proteobacteria. At genus level, 109 genera were found. Shannon metric for alpha diversity showed that factors like type of chickens (Commercial or experimental) and 16S rRNA gene subregion have negligible effect on diversity. Despite the large number of parameters that were taken into account, the identification of common bacteria showed five genera to be common for all sets in at least 50% of the samples. These genera are highly associated to cellulose degradation and short chain fatty acids synthesis. In general, it was possible to identify some commonalities in the bacterial cecal microbial community despite the extensive variability and factors differing from one study to another.

Keywords: 16S rRNA sequencing; Bacterial diversity; Chicken microbiota; Meta-analysis.

Grants and funding

The authors received no funding for this work.