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Long-term effects of early-life rumen microbiota modulation on dairy cow production performance and methane emissions
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Rumen microbiota modulation during the pre-weaning period has been suggested as means to affect animal performance later in life. In this follow-up study, we examined the post-weaning rumen microbiota development differences in monozygotic twin-heifers that were inoculated (T-group) or not inoculated (C-group) (n = 4 each) with fresh adult rumen liquid during their pre-weaning period. We also assessed the treatment effect on production parameters and methane emissions of cows during their 1st lactation period. The rumen microbiota was determined by the 16S rRNA gene, 18S rRNA gene, and ITS1 amplicon sequencing. Animal weight gain and rumen fermentation parameters were monitored from 2 to 12 months of age. The weight gain was not affected by treatment, but butyrate proportion was higher in T-group in month 3 (p = 0.04). Apart from archaea (p = 0.084), the richness of bacteria (p < 0.0001) and ciliate protozoa increased until month 7 (p = 0.004) and anaerobic fungi until month 11 (p = 0.005). The microbiota structure, measured as Bray–Curtis distances, continued to develop until months 3, 6, 7, and 10, in archaea, ciliate protozoa, bacteria, and anaerobic fungi, respectively (for all: p = 0.001). Treatment or age × treatment interaction had a significant (p < 0.05) effect on 18 bacterial, 2 archaeal, and 6 ciliate protozoan taxonomic groups, with differences occurring mostly before month 4 in bacteria, and month 3 in archaea and ciliate protozoa. Treatment stimulated earlier maturation of prokaryote community in T-group before month 4 and earlier maturation of ciliate protozoa at month 2 (Random Forest: 0.75 month for bacteria and 1.5 month for protozoa). No treatment effect on the maturity of anaerobic fungi was observed. The milk production and quality, feed efficiency, and methane emissions were monitored during cow’s 1st lactation. The T-group had lower variation in energy-corrected milk yield (p < 0.001), tended to differ in pattern of residual energy intake over time (p = 0.069), and had numerically lower somatic cell count throughout their 1st lactation period (p = 0.081), but no differences between the groups in methane emissions (g/d, g/kg DMI, or g/kg milk) were observed. Our results demonstrated that the orally administered microbial inoculant induced transient changes in early rumen microbiome maturation. In addition, the treatment may influence the later production performance, although the mechanisms that mediate these effects need to be further explored.
Title: Long-term effects of early-life rumen microbiota modulation on dairy cow production performance and methane emissions
Description:
Rumen microbiota modulation during the pre-weaning period has been suggested as means to affect animal performance later in life.
In this follow-up study, we examined the post-weaning rumen microbiota development differences in monozygotic twin-heifers that were inoculated (T-group) or not inoculated (C-group) (n = 4 each) with fresh adult rumen liquid during their pre-weaning period.
We also assessed the treatment effect on production parameters and methane emissions of cows during their 1st lactation period.
The rumen microbiota was determined by the 16S rRNA gene, 18S rRNA gene, and ITS1 amplicon sequencing.
Animal weight gain and rumen fermentation parameters were monitored from 2 to 12 months of age.
The weight gain was not affected by treatment, but butyrate proportion was higher in T-group in month 3 (p = 0.
04).
Apart from archaea (p = 0.
084), the richness of bacteria (p < 0.
0001) and ciliate protozoa increased until month 7 (p = 0.
004) and anaerobic fungi until month 11 (p = 0.
005).
The microbiota structure, measured as Bray–Curtis distances, continued to develop until months 3, 6, 7, and 10, in archaea, ciliate protozoa, bacteria, and anaerobic fungi, respectively (for all: p = 0.
001).
Treatment or age × treatment interaction had a significant (p < 0.
05) effect on 18 bacterial, 2 archaeal, and 6 ciliate protozoan taxonomic groups, with differences occurring mostly before month 4 in bacteria, and month 3 in archaea and ciliate protozoa.
Treatment stimulated earlier maturation of prokaryote community in T-group before month 4 and earlier maturation of ciliate protozoa at month 2 (Random Forest: 0.
75 month for bacteria and 1.
5 month for protozoa).
No treatment effect on the maturity of anaerobic fungi was observed.
The milk production and quality, feed efficiency, and methane emissions were monitored during cow’s 1st lactation.
The T-group had lower variation in energy-corrected milk yield (p < 0.
001), tended to differ in pattern of residual energy intake over time (p = 0.
069), and had numerically lower somatic cell count throughout their 1st lactation period (p = 0.
081), but no differences between the groups in methane emissions (g/d, g/kg DMI, or g/kg milk) were observed.
Our results demonstrated that the orally administered microbial inoculant induced transient changes in early rumen microbiome maturation.
In addition, the treatment may influence the later production performance, although the mechanisms that mediate these effects need to be further explored.
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