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Effects of non-digestible carbohydrates on gut microbiota and microbial metabolites: a randomised, controlled dietary intervention in healthy individuals

Published online by Cambridge University Press:  04 November 2024

Fiona C. Malcomson Open the ORCID record for Fiona C. Malcomson [Opens in a new window] ,
Panayiotis Louca Open the ORCID record for Panayiotis Louca [Opens in a new window] ,
Andrew Nelson ,
Naomi D. Willis ,
Iain McCallum ,
Long Xie ,
Arthur C. Ouwehand ,
Julian D. Stowell Open the ORCID record for Julian D. Stowell [Opens in a new window] ,
Tom Preston  and
Douglas J. Morrison Open the ORCID record for Douglas J. Morrison [Opens in a new window]
...Show all authors
Fiona C. Malcomson
Affiliation:
Human Nutrition and Exercise Research Centre, Centre for Healthier Lives, Population Health Sciences Institute, Newcastle University, Newcastle upon Tyne NE2 4HH, UK Centre for Cancer, Population Health Sciences Institute, Newcastle University, Newcastle upon Tyne, UK
Panayiotis Louca
Affiliation:
Human Nutrition and Exercise Research Centre, Centre for Healthier Lives, Population Health Sciences Institute, Newcastle University, Newcastle upon Tyne NE2 4HH, UK
Andrew Nelson
Affiliation:
Department of Applied Science, Northumbria University, Newcastle upon Tyne NE1 8ST, UK
Naomi D. Willis
Affiliation:
Human Nutrition and Exercise Research Centre, Centre for Healthier Lives, Population Health Sciences Institute, Newcastle University, Newcastle upon Tyne NE2 4HH, UK
Iain McCallum
Affiliation:
Northumbria Healthcare NHS Foundation Trust, North Tyneside General Hospital, Rake Lane, North Shields NE29 8NH, UK
Long Xie
Affiliation:
Human Nutrition and Exercise Research Centre, Centre for Healthier Lives, Population Health Sciences Institute, Newcastle University, Newcastle upon Tyne NE2 4HH, UK
Arthur C. Ouwehand
Affiliation:
International Flavors & Fragrances, Kantvik 02460, Finland
Julian D. Stowell
Affiliation:
Sabri Ülker Foundation, Istanbul, Turkey
Tom Preston
Affiliation:
Scottish Universities Environmental Research Centre, College of Science and Engineering, University of Glasgow, Glasgow, UK
Douglas J. Morrison
Affiliation:
Scottish Universities Environmental Research Centre, College of Science and Engineering, University of Glasgow, Glasgow, UK
Seamus B. Kelly
Affiliation:
Northumbria Healthcare NHS Foundation Trust, North Tyneside General Hospital, Rake Lane, North Shields NE29 8NH, UK
D. Michael Bradburn
Affiliation:
Northumbria Healthcare National Health Service Foundation Trust, Ashington, UK
Nigel J. Belshaw
Affiliation:
University of East Anglia, Norwich Research Park, Norwich NR4 7TJ, UK
Ian T. Johnson
Affiliation:
Quadram Institute, Norwich Research Park, Norwich, Norfolk NR4 7UQ, UK
Bernard M. Corfe
Affiliation:
Human Nutrition and Exercise Research Centre, Centre for Healthier Lives, Population Health Sciences Institute, Newcastle University, Newcastle upon Tyne NE2 4HH, UK
Christopher J. Stewart
Affiliation:
Translational and Clinical Research Institute, Newcastle University, Newcastle upon Tyne NE2 4HH, UK
John C. Mathers*
Affiliation:
Human Nutrition and Exercise Research Centre, Centre for Healthier Lives, Population Health Sciences Institute, Newcastle University, Newcastle upon Tyne NE2 4HH, UK
*
Corresponding author: John C. Mathers; Email: [email protected]
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Abstract

The gut microbiome is impacted by certain types of dietary fibre. However, the type, duration and dose needed to elicit gut microbial changes and whether these changes also influence microbial metabolites remain unclear. This study investigated the effects of supplementing healthy participants with two types of non-digestible carbohydrates (resistant starch (RS) and polydextrose (PD)) on the stool microbiota and microbial metabolite concentrations in plasma, stool and urine, as secondary outcomes in the Dietary Intervention Stem Cells and Colorectal Cancer (DISC) Study. The DISC study was a double-blind, randomised controlled trial that supplemented healthy participants with RS and/or PD or placebo for 50 d in a 2 × 2 factorial design. DNA was extracted from stool samples collected pre- and post-intervention, and V4 16S rRNA gene sequencing was used to profile the gut microbiota. Metabolite concentrations were measured in stool, plasma and urine by high-performance liquid chromatography. A total of fifty-eight participants with paired samples available were included. After 50 d, no effects of RS or PD were detected on composition of the gut microbiota diversity (alpha- and beta-diversity), on genus relative abundance or on metabolite concentrations. However, Drichlet’s multinomial mixture clustering-based approach suggests that some participants changed microbial enterotype post-intervention. The gut microbiota and fecal, plasma and urinary microbial metabolites were stable in response to a 50-d fibre intervention in middle-aged adults. Larger and longer studies, including those which explore the effects of specific fibre sub-types, may be required to determine the relationships between fibre intake, the gut microbiome and host health.

Keywords

Non-digestible carbohydratesResistant starchPolydextroseGut microbiotaSCFARandomised controlled trialDietary interventionHumans
Type
Research Article
Information
British Journal of Nutrition , Volume 132 , Issue 11 , 14 December 2024 , pp. 1433 - 1445
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Creative Commons
Creative Common License - CCCreative Common License - BY
This is an Open Access article, distributed under the terms of the Creative Commons Attribution licence (https://creativecommons.org/licenses/by/4.0/), which permits unrestricted re-use, distribution and reproduction, provided the original article is properly cited.
Copyright
© The Author(s), 2024. Published by Cambridge University Press on behalf of The Nutrition Society

Dietary fibre has been defined as carbohydrate polymers with three or more monomeric units that are not hydrolysed by endogenous enzymes in the small intestine(Reference McKeown, Fahey and Slavin1). It reaches the large intestine and is fermented by resident gut bacteria to produce microbial metabolites such as short-chain fatty acids (SCFA) including acetate, propionate and butyrate. Observational data suggest that higher intakes of dietary fibre, when compared with the lowest consumers, are associated with reduced risk of non-communicable diseases, including colorectal cancer, diabetes and CVD(Reference Reynolds, Mann and Cummings2). The proposed mechanisms through which dietary fibres exert their beneficial health effects include modulation of the gut microbiota and synthesis of microbial metabolites, primarily SCFA.

Dietary fibres include a wide range of non-digestible carbohydrates that differ in terms of physiochemical properties such as solubility and physiological effects such as fermentability(Reference McKeown, Fahey and Slavin1). These non-digestible carbohydrates include resistant starch (RS; the sum of starch and products of starch digestion that are not absorbed in the small bowel(Reference Cummings and Stephen3)) and polydextrose (PD; a synthetic, soluble fibre and glucose polymer with sorbitol end groups developed as a low-energy sweetener with bulking properties(Reference Stowell, Rastall and Gibson4)). Further, five subtypes of RS exist according to the factors affecting their resistance to digestion in the colon: type 1 (physically inaccessible e.g. wholegrains), type 2 (ungelatinised resistant granules with type B crystallinity e.g. high-amylose maize starch, green bananas), type 3 (retrograded starch e.g. cooked then cooled potatoes), type 4 (chemically modified starches e.g. cross-linked starch in thickeners) and type 5 (amylose–lipid complexes, e.g. palmitic acid amylose complex, foods with high amylose content)(Reference Raigond, Dutt, Singh, Mérillon and Ramawat5). Some highly fermentable fibres, including fructooligosaccharides and inulin, exert prebiotic effects, i.e. selectively stimulate the growth or activity of one or a limited number of gut bacteria, and thus confer beneficial effects on host health(Reference Swanson, Gibson and Hutkins6). A recent systematic review and meta-analysis, spanning sixty-four studies and over 2000 participants, investigated the effects of dietary fibre interventions on gut microbiota composition in healthy adults and included eight randomised controlled studies which supplemented with RS and/or PD(Reference So, Whelan and Rossi7). In the meta-analysis, six studies reported Shannon diversity index and three reported total number of observed operational taxonomic units and showed no overall effect of dietary fibre supplementation on α-diversity compared with placebo or low-fibre comparators(Reference So, Whelan and Rossi7). Subgroup analysis of the effects of fibres classified as candidate prebiotics (which include RS and PD) on bacterial abundance demonstrated increased Bifidobacterium spp., but no effects on Lactobacillus spp. (the two most commonly reported taxa), compared with placebo or low-fibre controls(Reference So, Whelan and Rossi7). It is not only the type of dietary fibre that is important, but fibre subtypes (e.g. RS type 1 v. type 2) may have differential effects on the gut microbiota and on host health. The authors also explored effects of dietary fibre interventions on SCFA concentrations (but did not perform fibre type subgroup analyses) and reported an increase in fecal butyrate concentrations after dietary fibre interventions compared with placebo or low-fibre comparators (standard mean difference (95 % CI): 0·24 (0·00, 0·47), P = 0·05)(Reference So, Whelan and Rossi7). However, no effects on total fecal SCFA concentrations were observed(Reference So, Whelan and Rossi7).

The SCFA butyrate exerts chemoprotective and other health-promoting properties that may be beneficial in the prevention or management of diseases such as colorectal cancer, insulin resistance and hypercholesterolaemia(Reference Canani, Costanzo and Leone8). Chambers et al. have also shown that targeted delivery of propionate has positive effects on appetite regulation, body weight maintenance and adiposity, and modulated the gut microbiota and plasma metabolome(Reference Chambers, Byrne and Morrison9,Reference Chambers, Viardot and Psichas10) . In contrast, higher intakes of dietary fibre, particularly insoluble fibre, have been associated with lower concentrations of fecal branched-chain fatty acids (BCFA)(Reference Rios-Covian, Gonzalez and Nogacka11), end-products of protein decomposition, which may provide an additional chemoprotective effect as certain metabolites produced during this process are carcinogenic. For example, in healthy male volunteers, supplementation with PD or soluble maize fibre for 21 d reduced the production of putrefactive compounds, including fecal BCFA and ammonia(Reference Boler, Serao and Bauer12).

The aim of this study was to investigate the effects of supplementing healthy participants for 50 d with two types of non-digestible carbohydrates which fall within the definition of dietary fibre (RS: Hi-maize® 260 (Ingredion™, type 2 RS) and/or PD: Litesse® Ultra™ (International Flavors & Fragances™ Danisco®)) on the gut microbiota and on microbial metabolite concentrations, including SCFA and BCFA, in stool, plasma and urine in the Dietary Intervention Stem Cells and Colorectal Cancer (DISC) Study. This is a secondary analysis of samples and data from the DISC study. We have reported previously the effects of RS and PD on a range of outcomes including inflammatory markers, WNT pathway-related markers, colorectal crypt cell proliferative state and microRNA expression(Reference Malcomson, Willis and McCallum13Reference Malcomson, Willis and McCallum15).

Experimental methods

A flowchart of the study design and analytical pipeline is presented in Fig. 1.

Figure 1. Flow chart of DISC study design and analytical pipeline. ATIMA, Agile Toolkit for Incisive Microbial Analysis; DISC, Dietary Intervention Stem Cells and Colorectal Cancer; DMM, Dirichlet’s multinomial mixture; PD, polydextrose; RS, resistant starch; SCFA, short-chain fatty acids.

The DISC study

The DISC study was a double-blind, randomised, placebo controlled dietary intervention that supplemented seventy-five healthy participants with two types of non-digestible carbohydrates (RS and/or PD) or respective placebos in a 2 × 2 factorial design for 50 d(Reference Malcomson, Willis and McCallum13). Participants were recruited by the research team from gastroenterology out-patients departments at North Tyneside General Hospital and Wansbeck General Hospital in the North East of England between May 2010 and July 2011 using endoscopy patient lists. Potential participants were sent a study invitation letter with detailed information about the study at least 5 days prior to their hospital appointment. At endoscopy, potential study participants were screened for exclusion criteria, which included: aged < 16 or > 85 years, pregnant or planning to become pregnant, diabetes mellitus, familial adenomatous polyposis syndrome, Lynch syndrome, known colorectal tumour or prior colorectal cancer, prior colorectal resection, active colonic inflammation at endoscopy, iatrogenic perforation at endoscopy, incomplete left-sided examination, colorectal carcinoma discovered at endoscopy or histology, chemotherapy in the last 6 months, administering non-steroidal anti-inflammatories, anti-coagulants or immunosuppressive medication. Ethical approval for the DISC study was granted by the Newcastle and North Tyneside Research Ethics Committee on 10th December 2009 (REC No. 09/H0907/77) and Caldicott approval for the storage of data was provided by the Northumbria NHS Foundation Trust (C1792). All participants provided informed written consent. The clinical trial is registered with ClinicalTrials.gov (Identifier NCT01214681).

Habitual diet was assessed at baseline using a food frequency questionnaire adapted from that used in the EPIC- Norfolk study (version 6, CAMB/PQ/6/1205)(Reference Kroke, Klipstein-Grobusch and Voss16). Participants were asked to consume their normal diet throughout the study. At least 1 week after their baseline endoscopy procedure, participants were randomised to one of four groups by selecting a sealed, opaque envelope:

  • Double placebo (12 g Maltodextrin (RS placebo) + 23 g Amioca starch (PD placebo))

  • PD (12 g Litesse® Ultra™ (International Flavors & Fragances™ Danisco®)

  • RS (23 g Hi-maize® 260, Ingredion™, Food Innovation)

  • RS + PD (23 g Hi-maize® 260, Ingredion™, Food Innovation + 12 g Litesse® Ultra™, International Flavors & Fragances™ Danisco®)

The allocation codes were locked and participants and the research team were blinded.

The RS utilised in this study was Hi-maize® 260 (Ingredion™), a type 2 RS that is isolated from high-amylose corn hybrids and occurs in the natural granular form and is approximately 53 % RS, with the remaining 40 % comprising digestible starch. PD was given in the form of Litesse® Ultra™, a sugar-free soluble fibre developed as a sweetener. It is a glucose polymer produced from sorbitol, dextrose and citric acid, which are derived naturally from corn. The intervention agents were supplied in a white powdered form in foil sachets packed into boxes each containing a week’s worth of sachets. Participants consumed 35 g of intervention supplement per day divided into four sachets (two sachets of each intervention agent). Participants were asked to consume the powdered supplements by adding to cold food or liquids such as yoghurt, orange juice or water. Participants were asked to retain all their sachets, including those that were not consumed. To measure compliance, the number of consumed and not consumed sachets were counted for each participant.

Sample collection

Participants provided rectal mucosal biopsies, blood, spot urine, stool and buccal cell samples at baseline (day 0) and post-intervention (day 50). Participants who underwent colonoscopy (pre-intervention only) were fasted at the point of blood sample collection. Blood samples were collected in seven 4 ml BD Vacutainer® K3EDTA tubes (Becton Dickinson, UK) and one 5 ml BD Vacutainer® SST™ II Advance tube with gold hemogard closure (Becton Dickinson, UK). EDTA tubes were centrifuged for 5 min at 3100 g and 4°C and plasma extracted and stored at −80°C until analysis.

At the initial endoscopy appointment, participants were provided with equipment for the collection of urine and stool at home. Sample collection was performed prior to the first home visit, seven days post-endoscopy appointment, to minimise any effects of bowel preparation associated with the endoscopy procedures. Post-intervention samples were collected just prior to the participant’s repeat sigmoidoscopy. For each collection, participants were provided with a large sealable bucket pot, a disposable bedpan, two ice packs and a cool bag. Urine and stool samples were kept in cool bags containing ice packs until collected by a member of the research team (pre-intervention samples) or brought to the repeat study visit (post-intervention samples). Stool was processed within 3–18 h of defecation. Samples were divided into 5–6 aliquots and stored immediately at –80°C until analysis.

Gut microbiota sequencing

Gut microbiota analysis was performed ∼10 years after data/sample collection. DNA was extracted from 250 mg stool samples using the DNeasy® PowerLyzer® PowerSoil® kit (Qiagen, UK) and following the manufacturer’s instructions. Bacterial profiling of the variable region 4 (V4) of the 16S rRNA gene was carried out by NU-OMICS (Northumbria University) based on the Schloss wet-lab MiSeq SOP(Reference Kozich, Westcott and Baxter17). Briefly, PCR was carried out using 1x Accuprime Pfx Supermix, 0·5 µM each primer and 1 µl of template DNA under the following conditions: 95°C 2 min, 30 cycles 95°C 20 s, 55°C 15 s, 72°C 5 min with a final extension 72°C 10 min. One positive (Zymobiomics Microbial Mock community DNA standard) and one negative control sample were included in each 96-well plate and carried through to sequencing. PCR products were quantified using Quant-iT™ PicoGreen™ dsDNA Assay (Invitrogen), and each sample was normalised to 10 nM and then each 96-well plate was pooled. Each pool was quantified using fragment size determined by BioAnalyzer (Agilent Technologies) and concentration by Qubit (Invitrogen). Pools were combined in equimolar amounts to create a single library then denatured using 0·2N NaOH for 5 min and diluted to a final concentration of 5 pM, supplemented with 25 % PhiX and loaded onto a MiSeq V2 500 cycle cartridge. Fastq files were processed using Mothur (v1·48). Paired reads were merged and then filtered to remove contigs > 275 bp, homopolymer > 8 and any ambiguous base. The high- quality reads were dereplicated and aligned to the Silva reference alignment (v132). Chimeric sequences were removed using VSearch(Reference Rognes, Flouri and Nichols18) and taxonomy was assigned using the RDP database (v18), and non Bacterial sequences were removed.

Quantification of microbial metabolite concentrations in stool, urine and plasma

Microbial metabolite analyses were performed within 12–24 months after data/sample collection. The concentrations of microbial metabolites (SCFA, BCFA, volatile fatty acids and lactic acid) in stool were quantified by gas chromatography by International Flavors & Fragances Danisco®, Finland as described previously(Reference Peuranen, Tiihonen and Apajalahti19). Briefly, 1 ml of 20 mm pivalic acid and 5 ml of water were added to 1 g of fecal sample, mixed thoroughly and centrifuged at 5000 g for 5 min. 250 µl of saturated oxalic acid solution was added to 500 µl of the supernatant, and the mixture was incubated at 48°C for 60 min, before centrifugation at 16 000 g for 5 min. The supernatant fraction was used for analysis, with pivalic acid as the internal standard.

Plasma and urinary SCFA and BCFA concentrations were measured by Scottish Universities Environmental Research Centre, East Kilbride, UK, as described by Morrison et al.(Reference Morrison, Cooper and Waldron20). SCFA and BCFA were extracted and derivatised as tBDMS (tert-butyl dimethyl silyl) esters prior to deuterium dilution analysis by GCMS. An alkaline internal standard mix containing three deuterated SCFA, three deuterated BCFA and 3-methyl valerate was added to each sample. Plasma samples (0·3 ml) were mixed and deproteinised using an ultracentrifuge device (Amicon Ultra 0·5 ml 30 kDa, Merck). Urine samples (1 ml) were spiked with an alkaline internal standard mix, but not ultrafiltered. Both sample types were dried by vacuum centrifuge. Blank tubes, deuterium enriched SCFA standards and unenriched SCFA standards were also dried. Dry samples and standards were acidified with dilute HCl. A volume of methyl tert-butyl ether was added and mixed to extract the SCFA. A sub-sample of the upper methyl tert-butyl ether phase was pipetted into a GC vial, and a composite derivatisation reagent was added. The freshly mixed derivatisation reagent contained tBDMSIM (Merck Sigma, UK) in acetonitrile with a hexanoic acid spike to facilitate removal of an acetate reagent blank. The vials were capped. They were derivatised at 70°C for 60 min and cooled. Samples and standards were analysed by GCMS (Agilent MSD, UK) in selected monitoring mode. SCFA and BCFA concentrations were calculated by deuterium dilution analysis.

Statistical analyses

The DISC study was not subject to a formal power calculation, and a target of seventy-five participants – allowing for a 10 % dropout rate, was set based on our previous study(Reference Dronamraju, Coxhead and Kelly21).

Statistical analyses were performed using R version 4.3.1(22), and the Agile Toolkit for Incisive Microbial Analysis (https://atima.research.bcm.edu/) (23) developed by the Centre for Metagenomics and Microbiome Research at the Baylor College of Medicine. The R-based software, Agile Toolkit for Incisive Microbial Analysis, is a stand-alone tool for analysing and visualising trends in alpha and beta diversity and taxa abundance. The rarefaction depth was set to 13 428, at which all negative controls and sequencing negatives were removed from the dataset. At this depth, 31 % of reads were used (1 879 920/6 097 817 reads retained). Microbial abundances with < 10 % prevalence were removed. Using Agile Toolkit for Incisive Microbial Analysis, Mann–Whitney test was used to compare pre- v. post-intervention data according to intervention agent (RS, PD or respective placebos). Differences in beta-diversity (weighted Bray–Curtis distance) were assessed using PERMANOVA, including study ID as a nesting factor. We controlled for false discovery rate (FDR) using the Bejamini-Hochberg procedure(Reference Benjamini and Hochberg24) and an FDR < 0·05 was considered significant.

To cluster gut microbial community states and distinguish inter-individual variations in gut microbiome response to the intervention we conducted Dirichlet’s multinomial mixture modelling(Reference Holmes, Harris and Quince25). The Laplace approximation criterion was used to determine the optimal number of clusters.

The ANOVA general linear model was used to test for effects of RS and PD and for interactions between the two, on post-intervention SCFA concentrations, adjusting for pre-intervention measurement, age, sex, BMI, endoscopy procedure and smoking status as covariates. Additionally, we calculated and investigated (using the same approaches as above) changes in microbial abundance and SCFA concentrations. Changes in microbial abundance and SCFA concentrations were calculated as delta = post-intervention value – corresponding pre-intervention value. Delta abundances were quantile normalised prior to modelling(Reference Bliss, Greenwood and White26). Confounding variables included age, sex, BMI, procedure type (flexible sigmoidoscopy or colonoscopy), smoking status and baseline dietary factors (intakes of energy, fibre and alcohol). Spearman’s correlations were used to explore metabolite correlations, both pre- and post-intervention, across tissue types (stool, urine and plasma). We also utilised the MaAsLin2 R package to conduct mixed effect modelling and explore the links between gut microbiome composition and intervention response. Within mixed effect modelling, participant ID was modelled as a random effect, intervention and additional covariates were modelled as fixed effects.

Results

Participant characteristics

Fifty-eight DISC study participants, for whom paired stool samples (pre- and post-intervention) were available for analyses, were included in this study (Fig. 1), and their characteristics are summarised in Table 1. All participants identified as being White British. The mean age of participants across all groups was 53 (sd 12) years. Just over half of the included participants were female (55 %). Most participants (83 %) were classed as having overweight or obesity based on their BMI. Over two-thirds of participants underwent endoscopic examination by flexible sigmoidoscopy during the baseline (pre-intervention) study visit. Half of the participants were never smokers, 26 % were former smokers and 24 % were current smokers. The mean dietary fibre (assessed using the Englyst method(Reference Englyst, Quigley and Hudson27)) intake at baseline was 22·5 g/d (sd 10·9). At baseline, there were no significant differences between intervention groups in habitual intake of energy (0·987), dietary fibre (P = 0·942) or protein (P = 0·532).

Table 1. Characteristics of participants in the DISC study (Numbers and percentages; mean values and standard deviations)

RS, resistant starch; PD, polydextrose.

Data are presented as number and proportion of participants (n (%)) with the exception of age, BMI and dietary fibre intake presented as mean (sd). Dietary fibre estimated using Englyst method.

Bacterial profiles in stool at baseline from DISC study participants

Pre-intervention, the bacterial profiles in stool from the DISC study participants reflected those of healthy human adults, as reported by King and colleagues(Reference King, Desai and Sylvetsky28); Firmicutes and Bacteroidetes were the most dominant phyla, followed by Proteobacteria, Actinobacteria and Verrucomicrobia (data not shown). At the genus level, the most abundant genera were Bacteroides, Faecalibacterium, Prevotella, Alistipes and Roseburia. There were no differences in the relative abundance of these bacteria between the four intervention groups at baseline. However, at the genus level, the relative abundance of Streptococcus was lower in participants randomised to the double placebo arm (FDR < 0·05).

Effects of resistant starch and polydextrose on gut microbiota diversity

When investigating effects of the intervention on alpha-diversity metrics (observed operational taxonomic units (richness) and Shannon index), no effects were detected post-intervention on alpha-diversity for either RS (observed operational taxonomic units, P = 0·833; Shannon index, P = 0·867) or PD (observed operational taxonomic units, P = 0·77; Shannon index, P = 0·89) (Fig. 2).

Figure 2. Effects of supplementation with RS and PD on two metrics of alpha-diversity. Alpha-diversity is represented by both observed operational taxonomic units (OTU) and Shannon Diversity. Panels A and B show the impact of RS supplementation on α diversity measured by observed OTU and Shannon diversity, respectively. Panels C and D illustrate the effects of PD supplementation on the same α diversity metrics. Each point represents individual participants pre- and post-intervention. Lines are coloured if change was > 1 sd, red lines between paired points represent a decrease and blue lines an increase, black lines represent changes of < 1 sd. PD, polydextrose; RS, resistant starch.

We further tested the effect of the intervention on beta-diversity metrics using both weighted and unweighted Bray–Curtis distances and found no effect of supplementation with RS (weighted P = 0·995, Fig. 3; unweighted: P = 1, online Supplementary Fig. 1) or PD (weighted: P = 0·93, Fig. 3; unweighted: P = 0·998, online Supplementary Fig. 1) compared with placebo.

Figure 3. Principal coordinates analysis based on weighted Bray–Curtis distance metrics, illustrating microbial communities pre- and post-intervention in response to both interventions. (a) Impact of RS supplement intervention on microbial community composition. (b) Influence of PD supplement intervention on microbial community composition. PD, polydextrose; RS, resistant starch.

Effects of resistant starch and polydextrose on gut microbiota abundance

When investigating differences in relative abundance of bacteria at taxonomic levels, we detected no effects of either RS or PD compared with their respective placebos at the phylum or genus level (Fig. 4).

Figure 4. Effects of supplementation with RS (a and c) and PD (b and d) on the relative abundance of bacteria. Phyla and genera are ordered based on lowest P value. Boxes represent interquartile ranges, with lines denoting median. Abbreviations: PD, polydextrose; RS, resistant starch.

We further performed a sensitivity analysis to adjust for several confounders on the effects of dietary treatment on bacterial abundances, including, age, sex, BMI, endoscopy procedure, smoking status and baseline dietary factors (intakes of energy, fibre and alcohol). After adjusting for confounders and multiple testing (FDR > 0·05), we did not detect any effect of dietary supplements on microbiota abundances. Results were consistent when using the MaAsLin2 R package(Reference Mallick, Rahnavard and McIver29) to conduct mixed effect modelling; no significant associations were identified after adjusting for participant ID as a random effect and the covariates listed above as fixed effects.

Inter-individual response to intervention

Although no effects of the intervention on gut microbiota diversity were detected for the study participants as a whole, Fig. 2 and Fig. 3 show relatively large, inter-individual changes in diversity metrics. To identify participants who displayed consistent gut microbiota responses to the intervention, we performed DMM clustering. Microbiota profiles were clustered into three microbial ‘enterotypes’ (online Supplementary Fig. 2). Cluster 1 was composed mostly of Bacteroides, Faecalibacterium and unclassified Ruminococcaceae. Cluster 2 was driven by high relative abundances of Bacteroides, Faecalibacterium and unclassified Lachnospiraceae, while cluster 3 was driven by high relative abundance of Prevotella, Faecalibacterium and Bacteroides abundance.

In response to the intervention, most participants remained in their baseline enterotype (Fig. 5). However, five participants transitioned from one enterotype to another, four from the RS + PD arm and one participant from the RS arm (Fig. 5(a)). The participant from the RS arm that transitioned enterotypes went from enterotype 2 pre-intervention to enterotype 1 post-intervention. Two participants from the RS + PD group transitioned from enterotype 3 pre-intervention to enterotype 1 post-intervention; one participant went from enterotype 1 to enterotype 2 and one participant transitioned from enterotype 2 to enterotype 1 (Fig. 5(b)). The numbers switching enterotypes were not statistically significant between groups.

Figure 5. Dirichlet’s multinomial mixture clustering of participants. (a) Proportional bar plot summarising the number of participants whose enterotype was unchanged and those who changed gut microbial enterotype post-intervention. (b) Movement of participants between the identified clusters (enterotypes) between pre- and post-intervention. Thin lines represent individual participants. PD, polydextrose; RS, resistant starch.

Effects of resistant starch and polydextrose on metabolite concentrations in stool, plasma and urine

The results for the effects of RS and PD on fecal, plasma and urinary metabolite concentrations, including SCFA and branched-chain fatty acids (BCFA), are displayed in Table 2. Participants supplemented with PD had lower post-intervention fecal concentrations of isobutyrate (least square mean (sd) 1·28 (0·12) PD v. 1·67 (0·13) placebo, P = 0·042) and of valeric acid (least square mean (sd) 1·76 (0·17) PD v. 2·48 (0·17) placebo, P = 0·006). There were no effects of RS or PD, or an interaction between the two NDC, on the other fecal, plasma and urinary microbial metabolites measured.

Table 2. Effects of RS and PD on post-intervention microbial metabolite concentrations in stool, plasma and urine

2MB, 2-methylbutyrate; BCFA, branched-chain fatty acids; PD, polydextrose; RS, resistant starch; SCFA, short-chain fatty acids; VFA, volatile fatty acids.

Data are presented as least squares means (LSM) for post-intervention data adjusted for pre-intervention measurement, age, sex, endoscopy procedure, BMI and smoking status (ANOVA GLM). Standard error of the mean (sem) are included in parentheses. *Significant effect of the intervention (P < 0·05). P interaction: P value for interaction effect of RS * PD.

When using delta change in metabolite concentrations between pre and post-intervention as the outcome, and after adjusting for age, sex, BMI, procedure type, smoking status, baseline dietary factors (energy, fibre and alcohol) and multiple testing, we noted that PD elevated fecal butyrate concentrations following the intervention (β (95 % CI) = 5·15 (0·55, 9·76), P adj = 0·03).

We further investigated the correlations between metabolite concentrations derived from stool, plasma and urine samples pre- and post-intervention. We detected multiple significant intra-sample correlations between microbial metabolites; however, inter-sample correlations were scarcer (online Supplementary Fig. 3). Of note, there were relatively strong negative correlations between urinary acetate concentrations and fecal concentrations of isovaleric acid and 2-methyl-1-butanol at baseline (pre-intervention).

Associations between gut microbiota and short-chain fatty acid concentrations

We further explored the relationship between changes in gut microbiota abundance and changes in fecal SCFA concentrations post-intervention. After adjusting for potential confounders, we detected possible associations between changes in gut microbial taxa, including Hydrogenoanaerobacterium, Roseburia and Collinsella, and changes in acetate (online Supplementary Fig. 4), propionate (online Supplementary Fig. 5), and butyrate concentrations (online Supplementary Fig. 6). However, none of these associations reached statistical significance following correction for multiple testing (FDR < 0·05).

Discussion

To our knowledge, the DISC study is the first study to investigate the effects of both RS and PD, or their combination, on the diversity and composition of the gut microbiota, as well as on fecal, plasma and urinary metabolite concentrations, particularly SCFA, in healthy participants. Further, to our knowledge, this is the largest randomised controlled trial in which healthy participants have been supplemented with PD, and second largest which has supplemented with RS(Reference So, Whelan and Rossi7) – the study by Alfa et al. included 84 participants(Reference Alfa, Strang and Tappia30). The DISC study also had the longest duration of supplementation with PD(Reference So, Whelan and Rossi7), and second longest to supplement with RS (the longest trial duration being 72 d(Reference Alfa, Strang and Tappia30)).

After adjusting for multiple testing and for potential confounders, we observed no effects of supplementation with RS and/or PD for 50 d on alpha-diversity, beta-diversity or on the relative abundance of bacteria phyla and genera. However, using clustering-based approaches that grouped individuals into enterotypes, we detected shifts in composition of the gut microbiota for some individuals in response to the RS and RS and PD intervention. This includes one participant supplemented with RS only and four participants supplemented with RS + PD (Fig. 5). Importantly, individuals randomised to the double placebo or PD arm did not change enterotype. This suggests that both the type and amount of dietary fibre may influence responses to intervention with larger amounts of dietary fibre (RS + PD) provoking enterotype change in more participants. The findings are in line with our earlier results on markers of colorectal cancer risk in the same cohort, where an effect of RS only on crypt cell proliferation was observed(Reference Malcomson, Willis and McCallum14).

In addition, the type of RS administered may be important in determining effects on the gut microbiome. Martinez et al. investigated the effects of supplementation with either 33 g per day of RS type 2 (a native granular starch consisting of ungelatinised granules) or type 4 (chemically modified starch) in ten healthy participants over 3 weeks and noted significant differences in their effects on human fecal microbiota composition(Reference Martínez, Kim and Duffy31). The RS type 4 (given as Fibersym®) significantly decreased Firmicutes and increased Bacteroidetes and Actinobacteria, whereas RS type 2 (given as Hi-Maize 260) produced no changes at the phylum level(Reference Martínez, Kim and Duffy31). In agreement with the findings from the present study, which used RS type 2, they found no effects of either type of RS on α-diversity(Reference Martínez, Kim and Duffy31). In contrast, in a 3-months long randomised controlled trial in which eighty-two healthy participants were supplemented with a potato-derived RS type 2 or corn starch placebo, there were significant effects on two measures of α-diversity (Shannon diversity index and inverse Simpson index)(Reference Alfa, Strang and Tappia30). RS type 2, used in the DISC study, is present in intact starch granules that can be found in foods such as bananas (4–5 g/100 g in ripe bananas and ∼18 g/100 g in green, unripe bananas(Reference Phillips, McGinty and Couture32))(Reference Mathers33).

Only four other randomised controlled trials have explored the effects of supplementing healthy adults with PD on the gut microbiota(Reference Costabile, Fava and Röytiö34Reference Jie, Bang-Yao and Ming-Jie37). Boler and colleagues examined the effects of supplementation with PD compared with soluble maize fibre or no fibre control on three specific fecal bacterial species and reported significant differences in post-intervention abundance of Bifidobacterium spp., Lactobacillus spp and Escherichia coli in those given PD(Reference Boler, Serao and Bauer35). In a placebo-controlled, double-blind, crossover study of thirty-one participants, 8 g of PD daily for 3 weeks significantly increased α-diversity (Simpson’s index) and the abundance of butyrate-producing Ruminococcus intestinalis and bacteria of the Clostridium clusters I, II and IV(Reference Costabile, Fava and Röytiö34). These changes were associated with lower fecal water genotoxicity, suggesting a reduction in risk factors that may be associated with early stages of colorectal carcinogenesis(Reference Costabile, Fava and Röytiö34). There were no effects of supplementation with PD on fecal SCFA concentrations(Reference Costabile, Fava and Röytiö34). Beards and colleagues supplemented forty healthy participants with chocolate products containing different blends of sucrose replacers (RS, PD or maltitol) for 6 weeks and found a significant increase in numbers of lactobacilli, Clostridium histolyticum/perfringens populations, Bacteroides, E. rectale, R. flavefaciens and total bacteria(Reference Beards, Tuohy and Gibson36). Over the 6-week period, there was also a significant increase in fecal acetate, propionate and butyrate concentrations(Reference Beards, Tuohy and Gibson36). In healthy Chinese adults, supplementation with PD for 28 d increased Lactobacillus and Bifidobacterium species and decreased Bacteroides species(Reference Jie, Bang-Yao and Ming-Jie37). Higher doses of PD increased fecal concentrations of acetate, butyrate and isobutyrate, and, perhaps surprisingly, resulted in higher colonocyte proliferation(Reference Jie, Bang-Yao and Ming-Jie37). In contrast, in twenty-one healthy adult men with a low habitual dietary fibre intake (∼13–15 g/d), supplementation with 21 g/d of PD for 21 d resulted in lower fecal acetate, propionate and butyrate concentrations compared with soluble maize fibre or no fibre control(Reference Boler, Serao and Bauer35). In agreement with the findings of Boler and colleagues(Reference Boler, Serao and Bauer35), in the DISC study, lower fecal concentrations of butyrate and valeric acid SCFA and of the BCFA isobutyrate were observed in participants supplemented with PD compared with placebo. We did not observe significant effects of RS, compared with placebo, on fecal, urinary or plasma SCFA. Although there is evidence that RS is one of the most effective dietary fibres at modulating the gut microbiota to stimulate butyrate production(Reference Cummings, Macfarlane and Englyst38), our systematic dose–response studies in the rat model have shown that the extent to which SCFA patterns are driven towards high molar proportion of butyrate depends on RS dose with lower molar proportions of butyrate observed with higher RS doses(Reference Mathers, Smith and Carter39). Importantly, in humans, the effects of RS on large bowel SCFA patterns vary at the individual participant level,(Reference Venkataraman, Sieber and Schmidt40,Reference Baxter, Schmidt and Venkataraman41) and some studies have reported no effects on butyrate concentrations(Reference DeMartino and Cockburn42). In addition, the effects of RS on butyrate, and other SCFA, are influenced by RS type(Reference Teichmann and Cockburn43). For example, although potato dish supplementation (providing RS type 2 and/or 3) for 4 weeks increased the abundance of butyrate-producing Roseburia faecis in healthy adults, there were no significant effects on fecal SCFA concentrations(Reference DeMartino, Johnston and Petersen44). When healthy young adults were supplemented with different types of RS for 2 weeks, only that from potatoes, but not RS from maize, increased fecal butyrate concentrations(Reference Baxter, Schmidt and Venkataraman41).

The lack of consistency in observations between the present study and some other studies of RS and PD supplementation in humans reflects the heterogeneity in findings reported in the systematic review and meta-analysis of effects of dietary fibre on the gut microbiome by So and colleagues(Reference So, Whelan and Rossi7). In addition to heterogeneity in characteristics of the study participants, this lack of consistency in response to supplementation may be explained by several factors related to the protocols for the intervention studies with the most prominent differences being type and dose of dietary fibre, study duration, comparator treatment and study design (most studies to date have been crossover trials)(Reference Dobranowski and Stintzi45). For example, RS type 4 may lead to larger changes in the composition of the gut microbiota than other RS types(Reference Martínez, Kim and Duffy31). Between study differences in findings may also be due to differences in the methods used to analyse the gut microbiota and to quantify concentrations of SCFA and other microbial metabolites.

Strengths and limitations

A strength of this study is that it was an randomised controlled trial that investigated the effects of equal doses of two contrasting types of dietary fibres (RS and PD) given for 50 d, which is one of the largest and longest duration studies of the effects of dietary fibre on the gut microbiome(Reference So, Whelan and Rossi7). The doses used (12 g of PD and 23 g RS per day) were designed to provide similar quantities of additional dietary fibre i.e. 11–12 g per day. As adults (aged 19–64 years) in the UK are estimated to consume, on average, 19·7 g of dietary fibre (AOAC definition) per day(46), the doses given would enhance fibre intake to the recommended level i.e. 30 g/d(47). Further, the ingredients were chosen as intervention agents because they can be incorporated into foods conveniently to enhance dietary fibre intake. Although RS and PD did not change the composition of the gut microbiota in this study, dietary fibre has a range of other beneficial effects including improving gut motility and contributing to metabolic health. Gastrointestinal transit time is a major modulator of the gut microbiome and of microbial metabolites both in vitro (Reference Minnebo, Delbaere and Goethals48) and in vivo (Reference Asnicar, Leeming and Dimidi49). Whilst some dietary fibres may impact gastrointestinal transit time(Reference Muller-Lissner50Reference Muir, Yeow and Keogh52), there is much less evidence for a consistent effect of RS on transit time(Reference Mathers, Smith and Carter39,Reference Cummings, Beatty and Kingman53Reference Sharma, Yadav and Yadav55) . Since we did not observe significant effects of RS or PD on the measured outcomes, we do not anticipate any effects on transit time.

We also performed sensitivity analyses to adjust for several potential confounders i.e. age, sex, endoscopy procedure at baseline, baseline dietary fibre intake and BMI. The results from these sensitivity analyses were comparable to those from our initial analyses, confirming our findings.

Another strength is that, in addition to characterising changes in the gut microbiota, we investigated effects on SCFA and other microbial metabolites in three different sample types i.e. stool, plasma and urine. However, fecal concentrations of SCFA may not be fully representative of intraluminal SCFA. For example, autopsy study of sudden death victims showed that concentrations of SCFA fell from the proximal to the distal colon(Reference Cummings, Pomare and Branch56). However, concentration of total SCFA in faeces was similar to those in the sigmoid and rectum(Reference Cummings, Pomare and Branch56).

A limitation of our study is that it may have been underpowered given that a priori sample size calculations were not conducted and that this was a secondary analysis using available data and samples. Although the DISC study included seventy-five participants, for the current investigation, paired baseline and follow-up data were available for a subset of fifty-eight participants only which limited our statistical power to detect effects of the intervention. That said, this is one of the largest randomised controlled studies on the effects of RS and PD on gastrointestinal microbiota and their metabolites in humans. Further, given the considerable inter-individual variation observed both at baseline and in response to the dietary fibre supplementation, the study duration and size may not have been sufficient to detect intervention effects at a group level.

Another limitation of this study is that dietary data were self-reported, which can introduce self-report bias(Reference Penn, Boeing and Boushey57). The mean habitual dietary fibre intake at baseline in our study was 22·5 g per day (mean intake by adults in the UK is approximately 18 g/d), which may suggest recruitment of participants with relatively healthier diets, despite the majority of participants having obesity, or an over-estimation of dietary fibre intake. We asked participants to maintain their habitual diet, but changes in other lifestyle factors such as physical activity, with potential to influence the gut microbiota and/or their metabolism, may have occurred during the intervention period. Lastly, all fifty-eight participants in this study identified as White British, restricting the generalisability of our findings to wider, more ethnically diverse populations.

Conclusions

In the DISC study, supplementation with RS and/or PD for 50 d did not elicit changes in the gut microbiota of healthy adults. Larger and longer duration studies that supplement with higher doses of dietary fibre are required to further investigate the effects of dietary fibre on the gut microbiome and associated metabolites. Such studies should focus on the effects of different fibre subtypes (e.g. RS type 1 v. RS type 2), be conducted in participants with different health status (e.g. individuals with bacterial dysbiosis or patients with type 2 diabetes(Reference Ojo, Ojo and Zand58) may be more responsive to dietary intervention) and use alternate study designs, including repeated measures and cross-over studies.

Supplementary material

For supplementary material/s referred to in this article, please visit https://doi.org/10.1017/S000711452400271X

Acknowledgements

We acknowledge the staff at the gastroenterology units at Wansbeck and North Tyneside General Hospitals for their help and support with participant recruitment and study visits. We are very grateful to Ingredion™, formerly National Starch, Food Innovation, USA and DuPont™ (International Flavors & Fragances™) Danisco®, Finland for supplying the RS and PD, respectively. We also thank the DISC study participants without whom this study would have been impossible. We are very grateful to Sinéad Ahearn-Ford for her help in training in DNA extractions from fecal samples.

This research was supported by an award from the Newcastle University Wellcome Trust-funded ISSF Small Grant Scheme to F. C. M, B. M. C., C. J. S. and J. C. M. The DISC study was funded by the BBSRC Diet and Health Research Industry Club (DRINC) (grant no. BB/H005013/1) to J. C. M., I. T. J., N. J. B. and S. K. P.L is supported by Newcastle University.

Designed research: F. C. M., N. D. W., S. B. K., M. B., N. J. B., I. T. J., B. M. C., C. J. S. and J. C. M. Conducted research: F. C. M., A. N., N. D. W., I. M., L. X., T. P., D. J. M. and C. J. S. Provided essential reagents or materials: A. N., N. D. W., I. M., A. C. O., J. D. S., T. P., D. J. M., C. J. S. and J. C. M. Analysed data or performed statistical analysis: F. C. M., P. L., C. J. S., Wrote paper: F. C. M., P. L., J. C. M. Had primary responsibility for final content: F. C. M., P. L., B. M. C., C. J. S. and J. C. M. All authors have read and approved the final manuscript.

The authors declare that they have no competing interests.

Metadata are available at: Malcomson, FC (2023), ‘DISC study Microbiota and SCFA data’, Mendeley Data, V2, DOI:10·17632/859pyzsxsg

Footnotes

These authors are co-first authors.

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Figure 0

Figure 1. Flow chart of DISC study design and analytical pipeline. ATIMA, Agile Toolkit for Incisive Microbial Analysis; DISC, Dietary Intervention Stem Cells and Colorectal Cancer; DMM, Dirichlet’s multinomial mixture; PD, polydextrose; RS, resistant starch; SCFA, short-chain fatty acids.

Figure 1

Table 1. Characteristics of participants in the DISC study (Numbers and percentages; mean values and standard deviations)

Figure 2

Figure 2. Effects of supplementation with RS and PD on two metrics of alpha-diversity. Alpha-diversity is represented by both observed operational taxonomic units (OTU) and Shannon Diversity. Panels A and B show the impact of RS supplementation on α diversity measured by observed OTU and Shannon diversity, respectively. Panels C and D illustrate the effects of PD supplementation on the same α diversity metrics. Each point represents individual participants pre- and post-intervention. Lines are coloured if change was > 1 sd, red lines between paired points represent a decrease and blue lines an increase, black lines represent changes of < 1 sd. PD, polydextrose; RS, resistant starch.

Figure 3

Figure 3. Principal coordinates analysis based on weighted Bray–Curtis distance metrics, illustrating microbial communities pre- and post-intervention in response to both interventions. (a) Impact of RS supplement intervention on microbial community composition. (b) Influence of PD supplement intervention on microbial community composition. PD, polydextrose; RS, resistant starch.

Figure 4

Figure 4. Effects of supplementation with RS (a and c) and PD (b and d) on the relative abundance of bacteria. Phyla and genera are ordered based on lowest P value. Boxes represent interquartile ranges, with lines denoting median. Abbreviations: PD, polydextrose; RS, resistant starch.

Figure 5

Figure 5. Dirichlet’s multinomial mixture clustering of participants. (a) Proportional bar plot summarising the number of participants whose enterotype was unchanged and those who changed gut microbial enterotype post-intervention. (b) Movement of participants between the identified clusters (enterotypes) between pre- and post-intervention. Thin lines represent individual participants. PD, polydextrose; RS, resistant starch.

Figure 6

Table 2. Effects of RS and PD on post-intervention microbial metabolite concentrations in stool, plasma and urine

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