Whole genome sequencing of “Faecalibaculum rodentium” ALO17, isolated from C57BL/6J laboratory mouse feces

Interactions between animals and their intestinal microorganisms play a crucial role in host physiology [1‐3]. For example, perturbations of the intestinal microbiota have been associated with immunological, metabolic, and neurological diseases [4, 5]. The metabolic activities of intestinal microorganisms directly affect food digestion, absorption, and energy production [6, 7]. The composition of the intestinal microbiota is also related to ageing of the host [8‐10]. The gut microbiota changes dramatically between early and late stages of life, with a shift from Lactobacillus and Bifidobacterium to Bacteroidetes and Clostridia genera. This shift suggests a change from lactate metabolism to increased short-chain fatty acid (SCFA) production and carbohydrate metabolism as ageing progresses [8, 10‐12]. To date, multiple studies have investigated the human intestinal microbiome to understand the relationships between the gut microbiota and host ageing [6, 8, 9]. However, difficulties controlling experimental conditions, including diet, medications, and housing status in complex human systems has contributed to inconsistencies in results from such studies. Mouse studies of the relationships between the microbiome and host ageing have provided better-controlled systems with consistent results. Langile et al. [10] divided female C57BL/6J mice into three age groups based on murine frailty index (FI) scores and reported that Erysipelotrichaceae was one of the dominant bacterial families colonising the guts of middle-aged mice (589 days old). These data are consistent with our unpublished data from investigations of the microbial diversity in mice of different ages. We found the most abundant operational taxonomic units (OTU) of middle-aged mice (18–21 months old) were related to Allobaculum species [13] within the family Erysipelotrichaceae. Using fresh and anoxic mice faeces and anaerobic culture techniques [13, 14], we isolated a strain closely related (99 % 16S rRNA gene sequence similarity) to the most abundant OTUs from the feces of C57BL/6J mice, and designated it “Faecalibaculum rodentium” ALO17 [13]. However, the overall intestinal microbiota, including the dominant strains present in the guts of different aged mice, has not been investigated in precise detail. In this study, the whole genome sequence of “F. rodentium” ALO17 was generated using a PacBio instrument and compared in silico to the previously-reported genome sequence of Allobaculum stercoricanis DSM 13633^T.

The genome of “F. rodentium” ALO17 as assembled here consisted of a single circular DNA chromosome of 2,542,486 base pairs, a GC content of 54.0 %, and no plasmids. The genome contained 2583 predicted open reading frames (ORFs), 55 tRNAs, and 38 rRNAs. Analyses using SEED subsystem categorization and COG functional categorizations are shown in Fig. 1. SEED subsystem categorization predicted 1529 ORFs that encode known functional proteins, whereas 1054 ORFs were of unknown function. Among the ORFs with a predicted function, 274 were predicted to be for carbohydrate synthesis, 200 were predicted to be for amino acid synthesis, 191 for protein metabolism, 140 for RNA metabolism, 122 for DNA metabolism, and 78 for the production of cofactors, vitamins, prosthetic groups, and pigments. Additionally, 40 ORFs belonged to the fermentation category. There are five major roles for genes in this category. A total of 13 ORFs (32.5 %) were similar to genes responsible for the fermentation of acetyl-CoA to butyrate, 12 (30.0 %) were predicted to be involved in fermentations with mixed acids, 9 (22.5 %) in butanol biosynthesis, 4 (10.0 %) in lactate fermentation, and 2 (5.0 %) were predicted to be acetolactate synthase subunits. COG analyses assigned 1566 ORFs (91.0 % of all predicted ORFs) to functional categories. Among these, 815 ORFs (47.39 % of the COG-assigned ORFs) belonged to 5 primary categories: 204 ORFs belonged to Category L (replication, recombination, and repair), 182 to Category G (carbohydrate transport and metabolism), 146 to Category E (amino acid transport and metabolism), 142 to Category K (transcription), and 141 to Category J (translation, ribosomal structure and biogenesis). For comparative genomic analyses, two methods were used: ANI and 16S rRNA gene sequencing. Nine bacterial species with pairwise similarities >85 % for the 16S rRNA gene, compared to “F. rodentium” ALO17, were selected. Among those selected, whole genome sequences for four species were in the NCBI database. A phylogenetic tree was constructed based on the 16S rRNA gene sequences. ANI values calculated between ALO17, E. dolichum DSM3991^T, F. cylindroides ATCC 27803^T, H. biformis DSM 3989^T, A. stercoricanis DSM 13633^T, were 63.9, 65.8, 66.2 and 66.8 %, respectively. Strain ALO17 clustered with strain DSM 13633^T in the phylogenetic tree, which was supported by a high bootstrap value and ANI dendrogram (Fig. 2). Due to their high level of relatedness, additional detailed genomic analyses were performed between “F. rodentium” ALO17 and other 4 reference of A. stercoricanis DSM 13633^T, H. biformis DSM 3989^T, F. cylindroides ATCC 27803^T and E. dolichum DSM3991^T. This comparison of the fermentation related genes is summarised in Table 1. “F. rodentium” ALO17 had a single homologue predicted to encode a protein that stimulates sugar/maltose fermentation. Additionally, subsystems for acetolactate synthase subunits, the fermentation of acetyl-CoA to butyrate, butanol biosynthesis, lactate fermentation, and mixed acid fermentation were present in both “F. rodentium” ALO17 and A. stercoricanis DSM 13633^T genomes. The numbers of genes in “F. rodentium” ALO17 and A. stercoricanis DSM 13633^T predicted to be involved in fermentation subsystems were 40 and 23, respectively. “F. rodentium” ALO17 had more genes predicted to be involved in specific functions, compared to A. stercoricanis DSM 13633^T. Such genes were predicted to encode for 3-hydroxybutyryl-CoA dehydrogenase (EC 1.1.1.157), 3-hydroxybutyryl-CoA dehydrogenase (EC 1.1.1.157), electron transfer flavoprotein (alpha and beta subunit), 3-hydroxybutyryl-CoA dehydrogenase (EC 1.1.1.157), pyruvate formate-lyase (EC 2.3.1.54), L-lactate dehydrogenase (EC 1.1.1.27), pyruvate formate-lyase (EC 2.3.1.54), and pyruvate formate-lyase activating enzyme (EC1.97.1.4). These data suggest that this isolate has stronger fermentation activity than A. stercoricanis DSM 13633^T. To test this hypothesis, the lactic acid concentrations were measured in the growth medium of “F. rodentium” ALO17 and A. stercoricanis DSM 13633^T by high-performance liquid chromatography. After three days of incubation at 37 °C, the lactic acid concentrations were observed to be 9.5 ± 0.6 mM (strain ALO17) and 4.9 ± 0.8 mM (A. stercoricanis DSM 13633^T), respectively. Previous study of A. stercoricanis DSM 13633^T showed the level of lactic acid was 3.5 mM [24]. In summary, despite their phylogenetic clustering, “F. rodentium” ALO17 differed from A. stercoricanis DSM 13633^T in lactic acid production. We hypothesize that “F. rodentium” ALO17 is an obligate anaerobe that replaces Lactobacilli and Bifidobacterium in middle-aged mice. Lactobacilli and Bifidobacterium are primary lactic acid producers in young mice; however, as the gut becomes strictly anaerobic with age, “F. rodentium” may become dominant. Thus, dominance of lactate producers and lactate production in the animal gut might be inversely related to ageing [10].