Animals and experimental design

The study was conducted at the Technical University of Denmark with ethical approval from the Danish Animal Experiment Inspectorate (permit number 2020-15-0201-00484). The in-house Animal Welfare Committee for Animal Care and Use oversaw the experiment, and the experiment was conducted in accordance with the ARRIVE guidelines (Percie du Sert et al., Reference Percie du Sert, Ahluwalia, Alam, Avey, Baker, Browne, Clark, Cuthill, Dirnagl, Emerson, Garner, Holgate, Howells, Hurst, Karp, Lazic, Lidster, MacCallum, Macleod and Würbel2020).

Twenty-four female Mouse Pathogen Free C57BL/6 mice, 7–8 weeks of age, were purchased from Taconic Biosciences (Ejby, Denmark). The software G*power 3 (Faul et al., Reference Faul, Erdfelder, Lang and Buchner2007) was used to estimate the necessary sample size for the experiment, with intestinal transit time as the main outcome. With a power of 0.80 and an alpha level of 0.05, the minimum group size for detecting differences in transit time between the four groups was estimated to be 6 animals per group. Upon arrival, the mice were allowed to acclimatize to the facilities for 11 days before starting the experiment. The mice were kept at a 12-hour light cycle in a constant environment with a relative humidity of 55 ± 5%, a temperature of 22 ± 1 °C, and an air change of 50 times per hour. The animals had ad libitum access to a regular chow diet (Altromin 1314, Brogaarden ApS, Denmark) and drinking water, also during transit time observations. The animals were single-housed during the entire study to limit stress-related effects on the transit time measurements, as expected to occur if the animals were moved from their cage mates during transit time observations.

On Day 1 of the experiment, the animals were allocated into four groups: control (saline), low loperamide dose (5 mg/kg), medium loperamide dose (7.5 mg/kg), and high loperamide dose (10 mg/kg). The animals were allocated to the four groups based on body weight, ensuring a similar average body weight in all groups. Loperamide/saline was administered to the animals through oral gavage for 1 week, starting from Day 3 of the study. Total intestinal time was measured at 4 different time points during the experiment, as described in the next section. Fresh faecal samples were collected on the morning of all days of the experiment, although samples could not be obtained from all animals on all days during the period of loperamide treatment due to constipation. The samples were kept on ice during collection and immediately transferred to −20 °C after collection. Bodyweight and food intake were monitored daily during the experiment. The experiment was terminated in the morning on Day 11, where all animals were anesthetised with hypnorm/midazolam (0.1 ml/10 g SC) and euthanized by cervical dislocation after collection of heart blood. The experimental design is illustrated in Figure 1A.

Figure 1. Overview of the study design (A) Minutes change in transit time between baseline observation (Day 2) and observations on Day 5, Day 8, and Day 10 for all groups (B) Differences between the groups were tested with a two-way ANOVA, followed by unpaired t-tests with FDR adjustment. *p < 0.05, **p < 0.01. Figure 1A was created in BioRender. Hjørne, A. (2023) BioRender.com/c29x987.

Oral administration and transit time estimation

In a pilot experiment (data not shown), we found that it was not possible to dissolve loperamide hydrochloride purchased from Sigma-Aldrich in saline or Tween, and the pure compound could not be used for oral administration. Instead, we used pulverised Imolope® tablets from Orifarm Generics, containing 2 mg of loperamide hydrochloride per tablet. The tablets were pulverized and dissolved in sterile saline in three different suspensions (0.05%, 0.075%, and 0.1% loperamide) to ensure similar dosing volumes for the three treatment groups. Dosing volume was calculated each day based on the body weight from the day before. Control animals received a volume of sterile saline corresponding to the volume of loperamide solution administered to animals of similar body weight, and dosing volumes ranged from 180–230 μL.

A solution of 6% carmine red (Sigma-Aldrich, C1022) and 0.05% methylcellulose (Sigma-Aldrich, M0262) was prepared the day before transit time measurements. The effect of the carmine red solution on the gut microbiome has already been tested in a previous animal study (Dey et al., Reference Dey, Wagner, Blanton, Cheng, Fontana, Haque, Ahmed and Gordon2015), which found no significant effects of the solution on the gut microbiome. On the morning of transit time measurements, the animals were moved to a clean cage with white absorbent paper covering the cage floor. All animals were administered 150 μL of the carmine red solution through oral gavage. On the days of co-administration of the loperamide and carmine solutions, loperamide was administered first, and faecal pellets were collected before administration. The time of carmine red gavage was recorded for each animal, and the animals were observed every 10–15 mins until the first red faecal pellet appeared. The transit time was calculated as the time between oral administration and the appearance of the first red pellet. The researcher observing the animals during transit time measurements was blinded to the treatment status of the animals.

In vitro test of direct drug effects on the gut microbiome

We performed an anaerobic batch fermentation experiment to test for any direct effects of the Imolope® solution on the gut microbiome. The experiment included three groups: control (saline), low loperamide (0.3 mg/l), and high loperamide (3 mg/l). The chosen loperamide concentrations were based on a paper from 1979 demonstrating that 70% of radiolabelled loperamide administered to rats was taken up in the liver or tissue (Miyazaki et al., Reference Miyazaki, Nambu, Matsunaga and Hashimoto1979), leaving 30% for transit through the colon before being excreted in the faeces. Thus, the 3 mg/ml corresponds to 30% of the 10 mg/kg body weight dosed to the high-dose mouse group in this study. The Imolope® solution was prepared as described for the animals above. Saline or Imolope® solution was added to 15 ml Falcon tubes containing pre-reduced-modified Gifu Anaerobic Medium (mGAM broth, Shimadzu, 05433-GBM-0100) with a pH of 7.3. A total volume of 5 ml was used for the fermentation, and all conditions were set up in triplicates. A faecal slurry was prepared by pooling faeces collected from all control animals on Day 4 of the experiment. Faecal pellets were homogenised in pre-reduced PBS (250 μL per pellet) inside an anaerobic chamber, and 50 μL of the faecal slurry was inoculated into the media with saline/Imolope®. The tubes were allowed to ferment while shaking for 72 hours in total, and 500 μL samples were collected every 24 hours. Immediately after collection, the samples were centrifuged at 10,000 g for 10 mins at 4 °C, the supernatant was removed, and the pellets were kept at -20 °C until DNA extraction. An overview of the fermentation experiment is provided in Supplementary Figure 10.

DNA extraction

The Qiagen Powersoil DNeasy kit (Qiagen) was used to extract DNA from mouse faecal samples (12–270 mg) and from the samples collected during the in vitro experiment. Before DNA extraction, faecal samples were suspended in 4x volumes of sterile Milli-Q, followed by centrifugation at 16,000 g for 10 mins. The supernatant was aspirated, and the pellet was used for DNA extraction. A blank DNA extraction control was included, and the manufacturer’s instructions were followed with a few adjustments, described in the following. Samples were homogenised by 10 mins of bead beating on a Retsch MM300 mixer mill (30/s) using the glass beads provided in the kit. In the first centrifugation step, samples were centrifuged at 16,000 g for 3 mins. In all other centrifugation steps, samples were centrifuged at 16,000 g for 1 min. DNA concentrations were measured using the Qubit 2.0 dsDNA High Sensitivity (Qubit HS) kit (Qiagen) and adjusted to 5 ng/μL for amplicon library preparation.

16S rRNA gene amplicon sequencing

PCR amplification and Ion Torrent GSS5 sequencing of the V3 region of the 16S rRNA were performed as previously described (Laursen et al., Reference Laursen, Dalgaard and Bahl2017). Briefly, a Mastermix of 10.4 μL PCR grade water, 4 μL HF-buffer, 0.4 μL dNTP (10 mM), 2 μL reverse primer (PBR 5′-trP1-adapter-ATTACCGCGGCTGCTGG-3′, 10 pmol/ μL), and 0.2 μL Phusion High-Fidelity Polymerase (Fisher Scientific, F-553 L) per sample was prepared. PCR was performed in a 20 μL reaction with 1 μL template DNA (5 ng/μL), 2 μL forward primer (PBU 5′-A-adapter-TCAG-barcode-CCTACGGGAGGCAGCAG-3′, 10 pmol/ μL), and 17 μL Mastermix. The forward and reverse primers were obtained from TAG Copenhagen A/S. Both primers were linked to adaptors necessary for ion torrent sequencing (A-adapter and trP1-adapter), while the forward primer also contained a barcode of 10 bp, unique for each sample. Primers were modified from Milani et al. (Reference Milani, Hevia, Foroni, Duranti, Turroni, Lugli, Sanchez, Martín, Gueimonde, van Sinderen, Margolles and Ventura2013). A Mock Community (ZymoBIOMICS™ Microbial Community DNA Standard, D6505) was included as a positive control, while PCR-grade water and a blank DNA extraction control were included as negative controls. The PCR was run on the following 45 mins program: (i) 30s denaturation at 98 °C, (ii) 24 cycles of 98 °C for 15 s, and 72 °C for 30s, (iii) 5 mins extension at 72 °C, and (iv) cooling to 4 °C. Randomly selected PCR products were quality-checked on a pre-made 2% agarose E-Gel Power Snap with SYBR-safe gel stain (Thermo Fisher Scientific). The PCR products were purified with HighPrep PCR Magnetic Beads (MAGBIO, AC-60005) using a 96-well magnet stand (MAGBIO, MyMag 96), following the manufacturer’s instructions. Final DNA concentrations were measured using the Qubit 2.0 dsDNA High Sensitivity (Qubit HS) kit (Qiagen), and samples were pooled in equimolar concentrations before Ion Torrent sequencing. Sequencing was performed on a 318-chip using the Ion OneTouch™ 200 bp Template Kit v2 DL.

Quantitative PCR measurement of total bacterial load

Quantitative PCR (qPCR) was performed to estimate the total faecal bacterial load, using the universal primers PBU (5′-CCTACGGGAGGCAGCAG-3′) and PBR (5′-ATTACCGCGGCTGCTGG-3′). A Mastermix of 6 μL PCR grade water, 1 μL forward primer (PBU, 4 μM), 1 μL reverse primer (PBR, 4 μM), and 10 μL SYBR Green Master Mix (Applied Biosystems, A25742) per sample was prepared. The PCR was performed in a 20 μL reaction with 18 μL Mastermix and 2 μL template DNA (5 ng/μL). A standard curve was generated from a 10-fold serial dilution (10³–10⁶ 16S rRNA copies/μL) of known concentrations of DNA from E. coli type strain (DSM18039). PCR-grade water was included as a negative control, and all reactions were performed in triplicates. The plate was run on the QuantStudio5™ Real-Time PCR system (Applied Biosystems) with the following program: (i) preincubation at 95 °C for 5 mins, (ii) 40 cycles of 95 °C for 10s, 60 °C for 15 s, and 72 °C for 45 s, (iii) a melting curve analysis of 95 °C for 5 s, 68 °C for 1 mins, and 98 °C for 15 s, and (iv) cooling to 4 °C. Data was analysed with the Design & Analysis software (v2.6.0, Applied Biosystems) and Excel. The qPCR data was used to estimate the absolute abundances of the microbial taxa by multiplying with the relative abundances obtained from the 16S rRNA gene amplicon sequencing.

Bioinformatic analysis

Raw 16S rRNA amplicon data was processed with an in-house pipeline (Mortensen, Reference Mortensen2023). Briefly, demultiplexing was performed with cutadapt (v. 4.1) (Martin, Reference Martin2011), denoising was performed with DADA2 (v. 1.22) (Callahan et al., Reference Callahan, McMurdie, Rosen, Han, Johnson and Holmes2016), and amplicon sequence variants (ASVs) were classified using the rdp_train_set_18 (Cole et al., Reference Cole, Wang, Fish, Chai, McGarrell, Sun, Brown, Porras-Alfaro, Kuske and Tiedje2014). Further processing and analysis of the data were done in R (v. 4.3.1).

Short-chain and branched-chain fatty acid extraction and analysis

Faecal and caecal water for SCFA and BCFA analysis was prepared by diluting the content in 4x volumes of sterile MiliQ, followed by 1–2 mins of vortexing. Samples were centrifuged at 16.000 g for 10 mins at 4 °C. The supernatant was transferred into 0.22 μm centrifuge filters (Costar Spin-X, centrifuge tube cellulose acetate filters) and filtered by centrifugation at 15.000 g for 10 mins at 4 °C.

Sample analysis was carried out by MS-Omics (Vedbæk, Denmark) as follows. Samples were acidified using hydrochloride acid, and deuterium-labelled internal standards were added. All samples were analysed in a randomized order. Analysis was performed using a high-polarity column (Zebron™ ZB-FFAP, GC Cap. Column 30 m × 0.25 mm × 0.25 μm) installed in a GC (7890B, Agilent) coupled with a time-of-flight MS (Pegasus® BT, LECO). The system was controlled by ChromaTOF® (LECO). Raw data was converted to netCDF format using Chemstation (Agilent), before the data was imported and processed in Matlab R2021b (Mathworks, Inc.) using the PARADISe software described by Johnsen and coworkers (Johnsen et al., Reference Johnsen, Skou, Khakimov and Bro2017).

Statistics

All statistical analyses were performed in R (v. 4.3.1). All p-values were adjusted for multiple comparisons using the False Discovery Rate (FDR) method. P-values below 0.05 after adjusting for multiple comparisons were considered significant. Appropriate parametric or non-parametric tests were applied for all analyses, depending on normality and variance tests. The tests applied for the specific comparisons are indicated in the figure legends. In all box plots, the border of the boxes indicates the interquartile range (IQR), horizontal lines represent the median, and the whiskers extend from the 25th and 75th percentiles to the furthest outlier within 1.5 times the IQR. The dots represent individual data points, and group means are visualised with a cross.

For beta diversity analysis, we first applied one-way ANOVA to identify possible group differences in beta dispersion, which can affect the interpretation of the following PERMANOVA (Warton et al., Reference Warton, Wright and Wang2012). A pairwise PERMANOVA within the Ecole package (Smith, Reference Smith2021) was performed for beta diversity analysis to test for differences between the animal groups on Day 9 and between the in vitro conditions at the three different time points.

The DAtest package (Russel et al., Reference Russel, Thorsen, Brejnrod, Bisgaard, Sorensen and Burmolle2018) was first used for the differential abundance analysis to find the best method for analysing the animal data. However, since the DAtest cannot be trusted when there is a separation associated with the predictor (in this case, treatment groups) (Russel et al., Reference Russel, Thorsen, Brejnrod, Bisgaard, Sorensen and Burmolle2018), the method identified in the DAtest was only used to screen the data for relevant taxa, i.e., taxa that appeared to differ in relative abundance between the treatment groups on Day 9 of the study. The relative distribution of the identified taxa was transformed into absolute abundances by multiplying with the bacterial load. Differences between the treatment groups in absolute abundances of the identified taxa were tested with appropriate statistical tests, as indicated in the figure legends. Moreover, the trajectories of the taxa were evaluated for all groups, and correlation analysis was used to evaluate associations between transit time and absolute abundances (transit time on Day 5 versus abundance on Day 5 and average transit time on Day 8/10 versus abundance on Day 9). The trajectories of relevant taxa were also evaluated for the different in vitro groups through appropriate statistical tests, as indicated in the figure legends.