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益生菌可刺激新生鼠肠道内肠细胞迁移和微生物多样性。

Probiotics stimulate enterocyte migration and microbial diversity in the neonatal mouse intestine.

机构信息

Texas Children's Hospital, Feigin Center, Ste. 830, 1102 Bates Ave., Houston, Texas 77030, USA.

出版信息

FASEB J. 2012 May;26(5):1960-9. doi: 10.1096/fj.10-177980. Epub 2012 Jan 20.

Abstract

Beneficial microbes and probiotics show promise for the treatment of pediatric gastrointestinal diseases. However, basic mechanisms of probiosis are not well understood, and most investigations have been performed in germ-free or microbiome-depleted animals. We sought to functionally characterize probiotic-host interactions in the context of normal early development. Outbred CD1 neonatal mice were orally gavaged with one of two strains of human-derived Lactobacillus reuteri or an equal volume of vehicle. Transcriptome analysis was performed on enterocyte RNA isolated by laser-capture microdissection. Enterocyte migration and proliferation were assessed by labeling cells with 5-bromo-2'-deoxyuridine, and fecal microbial community composition was determined by 16S metagenomic sequencing. Probiotic ingestion altered gene expression in multiple canonical pathways involving cell motility. L. reuteri strain DSM 17938 dramatically increased enterocyte migration (3-fold), proliferation (34%), and crypt height (29%) compared to vehicle-treated mice, whereas strain ATCC PTA 6475 increased cell migration (2-fold) without affecting crypt proliferative activity. In addition, both probiotic strains increased the phylogenetic diversity and evenness between taxa of the fecal microbiome 24 h after a single probiotic gavage. These experiments identify two targets of probiosis in early development, the intestinal epithelium and the gut microbiome, and suggest novel mechanisms for probiotic strain-specific effects.

摘要

有益微生物和益生菌有望用于治疗儿科胃肠道疾病。然而,益生菌的基本机制尚未得到很好的理解,并且大多数研究都是在无菌或微生物组耗尽的动物中进行的。我们试图在正常早期发育的背景下对益生菌-宿主相互作用进行功能表征。对经口给予两种人源乳杆菌(雷氏乳杆菌)菌株之一或等量载体的 CD1 新生小鼠进行外群处理。通过激光捕获微切割分离肠细胞 RNA 进行转录组分析。通过用 5-溴-2'-脱氧尿苷标记细胞来评估肠细胞的迁移和增殖,通过 16S 宏基因组测序来确定粪便微生物群落组成。益生菌摄入改变了涉及细胞运动的多个典型途径的基因表达。与给予载体的小鼠相比,DSM 17938 株显著增加了肠细胞迁移(3 倍)、增殖(34%)和隐窝高度(29%),而 ATCC PTA 6475 株增加了细胞迁移(2 倍)而不影响隐窝增殖活性。此外,两种益生菌株在单次益生菌灌胃后 24 小时增加了粪便微生物组中分类群之间的系统发育多样性和均匀度。这些实验确定了早期发育中益生菌的两个作用靶点,即肠道上皮和肠道微生物组,并提出了益生菌菌株特异性作用的新机制。

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