An optimization and refinement of the whole‐gut transit assay in mice

Author:

Schonkeren Simone L.1ORCID,Seeldrayers Saskia23ORCID,Thijssen Meike S.14ORCID,Boesmans Werend14ORCID,Langen Ramon C. J.35ORCID,Melotte Veerle16ORCID

Affiliation:

1. Department of Pathology, GROW School for Oncology and Reproduction Maastricht University Medical Center Maastricht The Netherlands

2. Central Animal Facilities Maastricht University Maastricht The Netherlands

3. Animal Welfare Body Maastricht University Maastricht The Netherlands

4. Biomedical Research Institute (BIOMED) Hasselt University Hasselt Belgium

5. Department of Respiratory Medicine, NUTRIM School for Nutrition, Toxicology and Metabolism Maastricht University Medical Center Maastricht The Netherlands

6. Department of Clinical Genetics Erasmus University Medical Center Rotterdam The Netherlands

Abstract

AbstractBackgroundGastrointestinal motility measurements in mice are currently performed under suboptimal conditions, as these nocturnal animals are measured during light conditions. In addition, other stressors, like individual housing, placement in a new cage during observation, and lack of bedding and cage enrichment cause animal discomfort and might contribute to higher variability. Here we aimed to develop a refined method of the widely‐used whole‐gut transit assay.MethodsWildtype mice (N = 24) were subjected to the standard or refined whole‐gut transit assay, either with or without a standardized slowing in gastrointestinal motility induced by loperamide. The standard assay consisted of a gavage with carmine red, observation during the light period and individual housing in a new cage without cage enrichment. For the refined whole‐gut transit assay, mice were gavaged with UV‐fluorescent DETEX®, observed during the dark period, while pairwise housed in their home cage with cage enrichment. Time until excretion of the first colored fecal pellet was assessed, and pellets were collected to assess number, weight, and water content.Key ResultsThe DETEX®‐containing pellets were UV‐detectable, allowing to measure the mice in their active period in the dark. The refined method caused less variation (20.8% and 16.0%) compared to the standard method (29.0% and 21.7%). Fecal pellet number, weight, and water content was significantly different between the standard and refined method.Conclusions & InferencesThis refined whole‐gut transit assay provides a reliable approach to measure whole‐gut transit time in mice in a more physiological context, with reduced variability compared to the standard method.

Funder

Nederlandse Organisatie voor Wetenschappelijk Onderzoek

Publisher

Wiley

Subject

Gastroenterology,Endocrine and Autonomic Systems,Physiology

Cited by 1 articles. 订阅此论文施引文献 订阅此论文施引文献,注册后可以免费订阅5篇论文的施引文献,订阅后可以查看论文全部施引文献

1. Circadian rhythm and whole gut transit in mice;Neurogastroenterology & Motility;2024-02-23

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