Gut Microbiota Dysbiosis in Suspected Food Protein Induced Proctocolitis-A Prospective Comparative Cohort Trial

被引:4
作者
Wurm, Philipp [1 ]
Stampfer, Laura [2 ]
Greimel, Theresa [2 ]
Leitner, Eva [3 ]
Zechner, Ellen L. [4 ,5 ]
Bauchinger, Sebastian [2 ]
Hauer, Almuthe C. [2 ]
Gorkiewicz, Gregor [1 ]
Hoegenauer, Christoph [6 ]
Hoffmann, K. Martin [3 ,7 ,8 ]
机构
[1] Med Univ Graz, Inst Pathol, Graz, Austria
[2] Med Univ Graz, Dept Pediat & Adolescent Med, Div Gen Pediat, Graz, Austria
[3] Med Univ Graz, Diagnost & Res Inst Hyg, Microbiol & Environm Med, Graz, Austria
[4] Karl Franzens Univ Graz, Inst Mol Biosci, Graz, Austria
[5] BioTechMed, Graz, Austria
[6] Med Univ Graz, Dept Internal Med, Div Gastroenterol & Hepatol, Graz, Austria
[7] Kinderarzte Zentrum Graz Raaba, Raaba Grambach, Austria
[8] Kinderarzte Zentrum Graz Raaba, Dr Auner Str 20-6, A-8074 Raaba Grambach, Austria
基金
奥地利科学基金会;
关键词
food protein induced proctocolitis; gut microbiota; hematochezia; infants; proctocolitis; INTESTINAL MICROBIOTA; ALLERGIC COLITIS; HUMAN-MILK; INFANTS; GUIDELINES; MANAGEMENT; DIAGNOSIS; BIFIDOBACTERIUM; CHILDREN; EUROPE;
D O I
10.1097/MPG.0000000000003789
中图分类号
R57 [消化系及腹部疾病];
学科分类号
摘要
Objectives: In infants with suspected food protein induced proctocolitis (sFPIP) only a minority of patients are finally diagnosed with the disease following diagnostic dietary intervention (DDI). There is a need for a pathophysiological explanation for the cause of hematochezia in the majority of sFPIP infants. Methods: We prospectively recruited infants with sFPIP and healthy controls. Fecal samples were collected at inclusion, week 4 (end of DDI in sFPIP), and week 8. For 16S rRNA sequencing (515F/806R) we used Illumina MiSeq sequencing system. Amplicon sequence variants were generated using Qiime2 and DADA2. Qiime diversity alpha and beta group comparisons and linear discriminant analysis effect size analysis was performed. For shotgun metagenomic analysis on species level we used KneadData and MetaPhlAn2. Results: Fourteen sFPIP infants were compared to 55 healthy infants. At inclusion overall microbial composition of sFPIP infants differed significantly from controls (weighted UniFrac; Pairwise PERMANOVA,P = 0.002, pseudo-F = 5.008). On genus level healthy infant microbiota was significantly enriched with Bifidobacterium (B) compared to sFPIP patients (linear discriminant analysis [LDA] = 5.5, P < 0.001, 31.3% vs 12.1%). sFPIP stool was significantly enriched by Clostridium sensu stricto 1 over controls (LDA = 5.3, P = 0.003, 3.5% vs 18.3%). DDI caused a significant and sustained increase of Bifidobacterium (LDA = 5.4, P = 0.048, 27.9%) in sFPIP infants. Species level analysis revealed significant reduction of abundance of B longum in sFPIP patients, which after DDI was reversed by B. species other than B longum. Conclusions: We revealed a gut microbiota dysbiosis phenomenon in sFPIP infants. DDI induces a microbiota composition comparable to that of healthy infants. In most sFPIP infants hematochezia might be triggered by a gut microbiota dysbiosis phenomenon.
引用
收藏
页码:31 / 38
页数:8
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