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猪肠道微生物群中抗菌药物耐药性的多组学监测

Multi-omics surveillance of antimicrobial resistance in the pig gut microbiome.

作者信息

Guitart-Matas Judith, Vera-Ponce de León Arturo, Pope Phillip B, Hvidsten Torgeir R, Fraile Lorenzo, Ballester Maria, Ramayo-Caldas Yuliaxis, Migura-Garcia Lourdes

机构信息

Joint Research Unit IRTA-UAB in Animal Health, Animal Health Research Centre (CReSA), Autonomous University of Barcelona (UAB), Bellaterra, Catalonia, Spain.

Institute of Agrifood Research and Technology (IRTA), Animal Health Program (CReSA), WOAH Collaborating Centre for the Research and Control of Emerging and Re-Emerging Swine Diseases in Europe, Autonomous University of Barcelona (UAB), Bellaterra, Catalonia, Spain.

出版信息

Anim Microbiome. 2025 Jun 17;7(1):65. doi: 10.1186/s42523-025-00418-8.

Abstract

BACKGROUND

High-throughput sequencing technologies play an increasingly active role in the surveillance of major global health challenges, such as the emergence of antimicrobial resistance. The post-weaning period is of critical importance for the swine industry and antimicrobials are still required when infection occurs during this period. Here, two sequencing approaches, shotgun metagenomics and metatranscriptomics, have been applied to decipher the effect of different treatments used in post-weaning diarrhea on the transcriptome and resistome of pig gut microbiome. With this objective, a metagenome-assembled genome (MAG) catalogue was generated to use as a reference database for transcript mapping obtained from a total of 140 pig fecal samples in a cross-sectional and longitudinal design to study differential gene expression. The different treatments included antimicrobials trimethoprim/sulfamethoxazole, colistin, gentamicin, and amoxicillin, and an oral commercial vaccine, a control with water acidification, and an untreated control. For metatranscriptomics, fecal samples from pigs were selected before weaning, three days and four weeks post-treatment.

RESULTS

The final non-redundant MAGs collection comprised a total of 1396 genomes obtained from single assemblies and co-assemblies per treatment group and sampling time from the metagenomics data. Analysis of antimicrobial resistance genes (ARGs) at this assembly level considerably reduced the total number of ARGs identified in comparison to those found at the reads level. Besides, from the metatranscriptomics data, half of those ARGs were detected transcriptionally active in all treatment groups. Differential gene expression between sampling times after treatment found major number of differential expressed genes (DEGs) against the group treated continuously with amoxicillin, with DEGs being correlated with antimicrobial resistance. Moreover, at three days post-treatment, a high number of significantly downregulated genes was detected in the group treated with gentamicin. At this sampling time, this group showed an altered expression of ribosomal-related genes, demonstrating the rapid effect of gentamicin to inhibit bacterial protein synthesis.

CONCLUSIONS

Different antimicrobial treatments can impact differently the transcriptome and resistome of microbial communities, highlighting the relevance of novel sequencing approaches to monitor the resistome and contribute to a more efficient antimicrobial stewardship.

摘要

背景

高通量测序技术在监测全球重大健康挑战(如抗菌药物耐药性的出现)方面发挥着越来越积极的作用。断奶后时期对养猪业至关重要,在此期间发生感染时仍需要使用抗菌药物。在此,应用了两种测序方法,即鸟枪法宏基因组学和宏转录组学,以解读断奶后腹泻中使用的不同处理方法对猪肠道微生物组转录组和耐药组的影响。为此,构建了一个宏基因组组装基因组(MAG)目录,用作从总共140份猪粪便样本中获得的转录本映射的参考数据库,这些样本采用横断面和纵向设计,以研究差异基因表达。不同的处理方法包括抗菌药物甲氧苄啶/磺胺甲恶唑、黏菌素、庆大霉素和阿莫西林,一种口服商业疫苗,水酸化对照,以及未处理对照。对于宏转录组学,在断奶前、处理后三天和四周选择猪的粪便样本。

结果

最终的非冗余MAG集合总共包含1396个基因组,这些基因组是从每个处理组和宏基因组学数据的采样时间的单组装和共组装中获得的。与在 reads 水平上发现的相比,在此组装水平上对抗菌药物耐药基因(ARG)的分析大大减少了鉴定出的ARG总数。此外,从宏转录组学数据来看,这些ARG中有一半在所有处理组中都被检测到具有转录活性。处理后不同采样时间之间的差异基因表达发现,与持续用阿莫西林处理的组相比,差异表达基因(DEG)数量最多,且DEG与抗菌药物耐药性相关。此外,在处理后三天,庆大霉素处理组中检测到大量显著下调的基因。在这个采样时间,该组显示核糖体相关基因的表达发生了改变,表明庆大霉素抑制细菌蛋白质合成的快速作用。

结论

不同的抗菌药物处理对微生物群落的转录组和耐药组的影响不同,突出了新型测序方法在监测耐药组以及促进更有效抗菌药物管理方面的相关性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/bcdf/12172226/a67381cb8fc2/42523_2025_418_Fig1_HTML.jpg

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