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Effect of chronic alcohol consumption on oral microbiota in rats with periodontitis

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Background The imbalance of oral microbiota can contribute to various oral disorders and potentially impact general health. Chronic alcohol consumption beyond a certain threshold has been implicated in influencing both the onset and progression of periodontitis. However, the mechanism by which chronic alcohol consumption affects periodontitis and its association with changes in the oral microbial community remains unclear. Objective This study used 16S rRNA gene amplicon sequencing to examine the dynamic changes in the oral microbial community of rats with periodontitis influenced by chronic alcohol consumption. Methods Twenty-four male Wistar rats were randomly allocated to either a periodontitis (P) or periodontitis + alcohol (PA) group. The PA group had unrestricted access to alcohol for 10 weeks, while the P group had access to water only. Four weeks later, both groups developed periodontitis. After 10 weeks, serum levels of alanine aminotransferase and aspartate aminotransferase in the rats’ serum were measured. The oral swabs were obtained from rats, and 16S rRNA gene sequencing was conducted. Alveolar bone status was assessed using hematoxylin and eosin staining and micro-computed tomography. Results Rats in the PA group exhibited more severe periodontal tissue damage compared to those in the periodontitis group. Although oral microbial diversity remained stable, the relative abundance of certain microbial communities differed significantly between the two groups. Actinobacteriota and Desulfobacterota were more prevalent at the phylum level in the PA group. At the genus level, Cutibacterium, Tissierella, Romboutsia, Actinomyces, Lawsonella, Anaerococcus, and Clostridium_sensu_stricto_1 were significantly more abundant in the PA group, while Haemophilus was significantly less abundant. Additionally, functional prediction using Tax4Fun revealed a significant enrichment of carbohydrate metabolism in the PA group. Conclusion Chronic alcohol consumption exacerbated periodontitis in rats and influenced the composition and functional characteristics of their oral microbiota, as indicated by 16S rRNA gene sequencing results. These microbial alterations may contribute to the exacerbation of periodontitis in rats due to chronic alcohol consumption.
Title: Effect of chronic alcohol consumption on oral microbiota in rats with periodontitis
Description:
Background The imbalance of oral microbiota can contribute to various oral disorders and potentially impact general health.
Chronic alcohol consumption beyond a certain threshold has been implicated in influencing both the onset and progression of periodontitis.
However, the mechanism by which chronic alcohol consumption affects periodontitis and its association with changes in the oral microbial community remains unclear.
Objective This study used 16S rRNA gene amplicon sequencing to examine the dynamic changes in the oral microbial community of rats with periodontitis influenced by chronic alcohol consumption.
Methods Twenty-four male Wistar rats were randomly allocated to either a periodontitis (P) or periodontitis + alcohol (PA) group.
The PA group had unrestricted access to alcohol for 10 weeks, while the P group had access to water only.
Four weeks later, both groups developed periodontitis.
After 10 weeks, serum levels of alanine aminotransferase and aspartate aminotransferase in the rats’ serum were measured.
The oral swabs were obtained from rats, and 16S rRNA gene sequencing was conducted.
Alveolar bone status was assessed using hematoxylin and eosin staining and micro-computed tomography.
Results Rats in the PA group exhibited more severe periodontal tissue damage compared to those in the periodontitis group.
Although oral microbial diversity remained stable, the relative abundance of certain microbial communities differed significantly between the two groups.
Actinobacteriota and Desulfobacterota were more prevalent at the phylum level in the PA group.
At the genus level, Cutibacterium, Tissierella, Romboutsia, Actinomyces, Lawsonella, Anaerococcus, and Clostridium_sensu_stricto_1 were significantly more abundant in the PA group, while Haemophilus was significantly less abundant.
Additionally, functional prediction using Tax4Fun revealed a significant enrichment of carbohydrate metabolism in the PA group.
Conclusion Chronic alcohol consumption exacerbated periodontitis in rats and influenced the composition and functional characteristics of their oral microbiota, as indicated by 16S rRNA gene sequencing results.
These microbial alterations may contribute to the exacerbation of periodontitis in rats due to chronic alcohol consumption.

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