What this is
- The review discusses the role of the gut microbiome in enhancing the efficacy of () in cancer therapy.
- It highlights how the microbiome can serve as a predictive biomarker and a therapeutic target.
- Current biomarkers for have limitations, and the integration of microbiome data may improve patient outcomes.
Essence
- The gut microbiome plays a crucial role in modulating immune responses to , potentially serving as both a biomarker and a therapeutic target. Its integration into cancer treatment strategies could enhance efficacy and mitigate adverse effects.
Key takeaways
- have transformed cancer treatment, but only ~13% of patients benefit from them. The gut microbiome's influence on immunity may help identify which patients are likely to respond.
- Higher microbial diversity correlates with improved responses to , suggesting that the gut microbiome could be a valuable biomarker for predicting treatment outcomes.
- () shows promise in enhancing ICI efficacy, with response rates of 20–30% observed in early-phase clinical trials.
Caveats
- Methodological heterogeneity in microbiome studies limits reproducibility and the generalizability of findings across different populations.
- Current clinical applications of microbiome-based strategies are still in early stages, requiring more rigorous trials to establish their efficacy and safety.
Definitions
- Immune checkpoint inhibitors (ICIs): Therapeutic agents that block proteins that inhibit immune responses, enhancing the body's ability to fight cancer.
- Fecal microbiota transplantation (FMT): A procedure that transfers fecal material from a healthy donor to a recipient to restore gut microbiome diversity and function.
AI simplified
1. Introduction
The approval of immune checkpoint inhibitors (ICIs) in the 2010s marked a paradigm shift in cancer therapy. Used as monotherapy or in combination, ICIs have produced unprecedented outcomes and are now the standard of care across several solid tumors. However, a substantial proportion of patients derive limited benefit, and efficacy can vary even among patients with the same cancer type and comparable biomarkers [1,2].
In parallel, the gut microbiome has emerged as a key regulator of host immunity. Accumulating evidence suggests that the microbiome may serve as both a predictive biomarker of ICI response and as a therapeutic target to enhance efficacy. Incorporating microbiota-based strategies into ICI therapy, therefore, represents a promising approach to improving clinical outcomes [3].
This review aims to provide practicing medical oncologists with a practical overview of how the gut microbiome affects antitumor immunity and influences the efficacy of ICIs. The following sections outline the limitations of current ICI biomarkers and describe how the microbiome is acquired and interacts with the host immune system. The discussion then covers the analytical methods used to study gut microbiota in relation to ICI response, microbial features associated with treatment outcomes, and therapeutic strategies targeting the gut microbiome. The review concludes by highlighting key challenges that future research must address for successful clinical application.
2. Current Biomarkers of ICIs and Their Limitations
ICIs have delivered long-term, durable responses in metastatic cancer and increased cure rates in early-stage disease. Despite this success, it is estimated that only ~13% of cancer patients are eligible and derive benefit from ICI therapy [4]. Currently, several biomarkers are used in clinical practice to guide ICI use, including programmed death-ligand 1 (PD-L1) expression, mismatch repair (MMR) or microsatellite instability (MSI) status, and tumor mutational burden (TMB). Other promising markers include POLE/POLD1 mutation and tumor-infiltrating lymphocytes (TILs). Despite extensive validation across tumor types, no single biomarker reliably predicts response to ICIs in all settings. Their performance is context-dependent and limited by assay heterogeneity, tumor evolution, and sampling bias. A summary of their methods, advantages, and limitations is presented in Table 1.
The limitations of these current ICI biomarkers justify the search for integrative models that incorporate host factors, including the gut microbiome, to better predict treatment outcomes.
| Biomarker | Methods | Advantages | Limitations |
|---|---|---|---|
| Programmed death-ligand 1 (PD-L1) [] [5] | immunohistochemistry (IHC) | widely available;quick turnaround; validated in several cancer types | multiple FDA-approvedcompanion assays (22C3, 28-8, SP142, SP263) with different score cut-off for ICIs and cancer types; subject to tumor heterogeneity and sampling bias |
| Mismatch repair (MMR) [,,] [6] [7] [8] | PCR or next-generation sequencing (NGS) for MSI status;IHC for MMR proteins (MLH1, PMS2, MSH2, MSH6) | FDA-approved MSI-high (MSI-H) or dMMR status as a tissue-agnostic biomarker; strong predictive value | rare in solid tumors (~3–16%);limited availability of validated MSI assays in some centers |
| Tumor mutational burden (TMB) [,] [9] [10] | NGS | FDA-approved TMB ≥ 10 mut/Mb by FoundationOne CDx as a tissue-agnostic biomarker for pembrolizumab; reflects overall neoantigen landscape | expensive and longer turnaround time; optimal cut-off may vary across cancer types; lack ofstandardized assessment methods |
| POLE/POLD1mutations [,] [11] [12] | NGS | associated with anultra-hypermutatedphenotype and exceptionally high TMB | not FDA-approved; rare in solid tumors (~4%) |
| Tumor-infiltrating lymphocytes (TILs) [] [13] | H&E pathology slide evaluation | reflects the actual immuneresponse within the tumor;assessable on routinepathology slides | not FDA-approved; lackstandardized scoring; subject to spatial and temporal heterogeneity |
3. The Microbiome: A Key Environmental Factor in Immunity
The human immune responses vary considerably across individuals, shaped by a combination of intrinsic host factors and external environmental influences. Host factors such as genetic background, age, and sex are known to affect immune cell composition and antitumor surveillance [14,15,16]. However, evidence from twin studies suggests that environmental factors, including the gut microbiome, infections, and medications (notably antibiotics and immunomodulatory drugs), are the dominant drivers, accounting for 24–77% of the variability in human immune traits [17,18].
3.1. Acquisition and Distribution
The gut microbiome is highly individualized down at the strain level [19,20], with environmental factors dominating over genetics in shaping its composition in adults [21,22,23]. Microbial colonization begins at birth via maternal transmission and evolves throughout life in response to interactions with other humans and animals, diet, antibiotic exposure, and the surrounding environment [24]. Microbial communities are found throughout the gastrointestinal tract, but their composition varies significantly by location due to differences in oxygen levels, pH, and transit time [25,26]. The large intestine hosts the most abundant and diverse community, making it the primary focus for biomarker discovery and therapeutic modulation.
3.2. How the Gut Microbiome Modulates Antitumor Immunity
The gastrointestinal tract houses one of the body’s largest immune compartments [27]. The gut microbiome modulates both innate and adaptive immune responses through two primary mechanisms: direct stimulation via microbial components (e.g., lipopolysaccharides activating Toll-like receptors) and indirect signaling via production of bioactive metabolites (e.g., short-chain fatty acids and secondary bile acids). Table 2 summarizes key microbiome-mediated mechanisms that affect both innate and adaptive immunity, including interactions across the cancer-immunity cycle. Figure 1 presents an integrated schematic of how these microbial processes influence antigen release, immune activation, T-cell trafficking, and tumor cell killing.
The gut microbiome is not a passive bystander but an active modulator of systemic immunity, with the potential to either enhance or suppress antitumor immune responses. Its ability to influence every step of the cancer-immunity cycle makes it a powerful biomarker and a promising therapeutic target in oncology.
Examples of microbiome interaction across the cancer-immunity cycle. The gut microbiome modulates antitumor immunity through multiple steps of the cancer–immunity cycle. () Microbial components and toxins can induce DNA damage and generate neoantigens. () Microbial antigens cross-react with tumor antigens and stimulate dendritic cell maturation via Toll-like receptor (TLR) signaling, enhancing antigen presentation and T-cell priming. () Microbiota-derived metabolites and cytokines regulate chemokine expression and myeloid-derived suppressor cell (MDSC) activity, facilitating T-cell trafficking and infiltration into the tumor microenvironment. () Within tumors, microbial signals can enhance HLA class I expression and modulate immune checkpoint molecules, promoting T-cell–mediated tumor killing. Abbreviations: CTL, cytotoxic T lymphocyte; DC, dendritic cell; IFN, interferon; IL, interleukin. Created with BioRender.com/0bwtrk8 (accessed on 9 November 2025). A B C D
| Innate Immunity | |
|---|---|
| - Maintenance of intestinal mucosal integrity and homeostasis through production of mucins and metabolites []. [28] - Bacterial components (e.g., LPS and flagellin) activate pattern recognition receptors (e.g., TLRs), promoting maturation of dendritic cells (DCs), polarization of M1 macrophages, and activation of NK cells []. [29] - Bacterial metabolites enhance the function of innate lymphoid cells []. [30] | |
| Examples of microbiome interactions across the cancer-immunity cycle | |
| Release of cancer cell antigens | - Microbial toxins can induce DNA damage, generating neoantigens [] [31] - The microbiota can influence tumor-associated antigens presentation and immunogenic cell death [] [32] |
| Antigen Presentation by Immune Cells & T-cell Activation and Priming | - Cross-reactivity between microbial and tumor antigens [,] [33] [34] - Promotes DC activation and maturation via TLR signaling [] [35] - Enhanced cytokine production (e.g., IL-1, IL-12) by dendritic cells [] [36] - Microbiota-derived SCFAs (butyrate and propionate) modulate DC function and T-cell differentiation by histone deacetylases (HDAC) inhibition [,,] [37] [38] [39] - Microbiota-derived inosine boosts IFN-γ production in CD8+T cells via adenosine receptor (A2A) signaling [] [40] |
| T-cell Trafficking & T-cell Infiltration into the Tumor | - Regulation of chemokines and cytokines influencing T-cell trafficking (e.g., TNF-α, CXCL9, CXCL10) [,] [41] [42] - Modulation of immunosuppressive cells like Myeloid-Derived Suppressor Cells (MDSCs) [,] [43] [44] |
| Cancer Cell Recognition by T cells & Tumor Cell Killing | - Influences the expression of immune checkpoint molecules (e.g., CTLA-4, PD-1/PD-L1) [,,] [45] [46] [47] - Can upregulate HLA class I on tumor cells, enhancing their recognition by T cells [,] [48] [49] |
4. Analysis of Gut Microbiome and Response to ICIs
4.1. Analysis Pipeline Overview
The investigation of the gut microbiome and ICI response follows a structured pipeline: (1) prospective sample collection at key time points; (2) stratification of patients into ICI responder and non-responder groups; (3) microbiome profiling and bioinformatic processing; and (4) statistical analysis to integrate microbiome data with clinical outcomes (Figure 2).
Reproducibility is a major challenge in microbiome research. Discrepancies between studies often arise from variations at each step of the pipeline. Adherence to reporting standards, such as the Minimum Information about a Marker Gene Sequence (MIMARKS), and detailed documentation of protocols are crucial for enabling cross-study comparisons and validating findings [50].
Analysis pipeline of gut microbiome and ICI response. Schematic of the study design and analytical workflow for investigating the gut microbiome in ICI-treated patients. Stool samples are typically collected at baseline, during, and after ICI therapy for responders and non-responders. Integrative analyses link microbiome profiles to clinical outcomes, including progression-free survival, overall survival, and immune-related adverse events. Lower panels illustrate commonly used analytical approaches: 16S rRNA and shotgun metagenomics for taxonomic and functional profiling; metatranscriptomics, metaproteomics, and metabolomics for gene expression, protein, and metabolite analysis; and culturomics for isolating viable strains and expanding microbial catalogs. Created with BioRender.com/9bguul0 (accessed on 9 November 2025).
4.2. Sample Types for Microbiome Profiling
4.2.1. Fecal Samples
Fecal specimens are currently the gold standard for gut microbiome analysis, serving as a proxy for the distal colon’s microbial community. Collection is non-invasive, repeatable, and provides sufficient biomass for analysis [51]. To preserve microbial integrity, samples should be immediately cryopreserved at −80 °C or stored in commercial preservation buffers. Standardized protocols for collection, storage, and transport are essential, as variability can significantly alter results [52,53].
4.2.2. Oral Samples
Oral samples (e.g., saliva and swabs) are readily accessible, but their role in systemic immune modulation is less well established [54]. These samples are also limited by low microbial biomass, high levels of human DNA contamination, and significant variability across oral sites [55,56].
4.2.3. Direct Gut Sampling (Swab, Biopsy, and Swallowable Capsules)
Mucosal biopsy and luminal swab enable direct study of host tissue and microbiome interactions. Catheter aspiration facilitates sampling from difficult-to-reach sites. However, these methods are invasive, requiring special preparation, and may not be suitable for routine use. Swallowable capsules can autonomously collect intestinal fluid at the targeted gut location with minimal invasiveness. Nevertheless, their adoption is limited by technical complexity and availability [51].
4.2.4. Tumor Samples
Historically considered sterile, tumor tissue is now recognized to harbor distinct microbial communities, referred to as the intratumoral microbiome. Early hints date back to the 1890s with William B. Coley’s work on bacterial toxin-mediated antitumor effects [57], and modern sequencing technologies have since confirmed the presence of these microbes. Intratumoral microorganisms are now considered integral components of the tumor microenvironment and have been linked to treatment outcomes, representing a promising new frontier of investigation [58,59,60,61,62,63].
4.3. Relative vs. Absolute Quantification of Microbiome
Microbiome data can be interpreted in two ways:
Relying on relative abundance alone can lead to false correlations [68,69]. For example, after probiotic administration, an increase in the relative abundance of Lactobacillus may reflect a decline in other commensals rather than true colonization. In contrast, detecting Lactobacillus at levels of 109 CFU/g via absolute quantification confirms successful engraftment and intervention efficacy. Absolute quantification is crucial for developing robust and reliable biomarkers.
4.4. Methods for Microbiome Analysis
4.4.1. Sequencing-Based Methods
4.4.2. Culture- and Metabolic-Based Methods
4.4.3. Multi-Omics Integration: A Holistic View
The most robust insights now emerge from multi-omics approaches that integrate metagenomics, metatranscriptomics, proteomics, and metabolomics. This holistic strategy can unravel complex host-microbe interactions and identify robust, multifaceted biomarkers. While challenges in standardization and data complexity remain, multi-omics integration is essential for translating microbiome discoveries into reliable clinical applications.
5. Microbial Features Associated with ICI Response
Although reproducibility can be a challenge in microbiome research, several key microbial features have been consistently identified as predictors of ICI efficacy. These signatures represent promising biomarkers and therapeutic targets.
5.1. Microbial Diversity
Microbial diversity is assessed in two main ways:
In multiple cancer types, higher baseline alpha diversity has been associated with improved responses to ICI therapy [88,89,90,91]. However, the magnitude of this difference is generally modest and often overlaps between groups. A meta-analysis reported that greater microbial diversity correlated with improved PFS (HR = 0.64, 95% CI 0.42–0.98), although heterogeneity across studies was high [92]. Conversely, reduced diversity, often observed in patients exposed to antibiotics, has been linked to poorer clinical outcomes [88,93].
5.2. Beneficial Bacterial Taxa
Most studies implemented 16S rRNA sequencing or shotgun metagenomics to measure relative abundance. As noted in, this compositional approach limits interpretation, and absolute quantification will be essential in future studies to validate these associations. Given these methodological limitations, several bacterial taxa have been linked to enhanced ICI response: Section 4.3
5.2.1. Akkermansia muciniphila
A. muciniphila is a common human gut microbe, specializing in degrading mucin and maintaining intestinal integrity [94]. In preclinical models, oral administration of A. muciniphila can reinvigorate exhausted T cells and restore anti-PD1 efficacy [95]. Higher relative abundance of A. muciniphila in stool at baseline is associated with improved progression-free survival in non-small cell lung cancer (NSCLC) and renal cell carcinoma (RCC) treated with PD-1 blockade [96,97,98]. In a prospective study of 338 advanced NSCLC patients, baseline stool A. muciniphila was associated with increased objective response rates and overall survival, independent of PD-L1 status [99].
5.2.2. Faecalibacterium prausnitzii
F. prausnitzii, a major butyrate producer, is one of the most abundant bacteria in gut microbiota, representing more than 5% of gut microbiota in healthy adults [100,101]. In patients diagnosed with cancer, the relative abundance of F. prausnitzii was significantly lower than in non-cancer subjects [102,103]. In vitro, the F. prausnitzii strain EXL01 enhances dendritic cell and T cell activity, and oral administration of this strain restores anti-PD-L1 efficacy in mouse models with antibiotic-induced microbiota disruption [104]. Enrichment of F. prausnitzii at baseline has been observed in ICI responders across multiple cancer types [89,105,106].
5.2.3.Species Bifidobacterium
Bifidobacteria are predominant in infants but generally constitute a smaller proportion (<10% of the relative abundance) of the adult gut microbiota [107]. In mouse models, oral administration of Bifidobacterium enhances ICI effects by augmenting dendritic cell function and producing the metabolite inosine [40,108,109,110]. Enrichment of B. longum and B. breve has been associated with improved outcomes in melanoma and NSCLC patients receiving ICIs, respectively [111,112].
5.2.4.Family Ruminococcaceae
Members of the Ruminococcaceae family are highly prevalent in the human gut microbiome, with particular species having been linked to ICI response [113]. For example, R. gnavus enhanced anti–PD-1 efficacy in mouse models by promoting CD4+ T cell migration into tumors and activating pro-inflammatory macrophages [114]. In clinical cohorts of advanced NSCLC and melanoma patients, the Ruminococcaceae family was enriched in ICI responding patients [88,115]
5.3. Key Microbial Metabolites
5.3.1. Short-Chain Fatty Acids (SCFAs)
SCFAs—notably butyrate, acetate, and propionate—are produced by the gut microbiota through fermentation of dietary fiber. They play critical roles in linking the microbiome to both local and systemic immune regulation. These functions are mediated by several key mechanisms, including histone deacetylase (HDAC) inhibition, G-protein-coupled receptor (GPCR) signaling, and modulation of cellular energy and signaling pathways [116]. However, clinical data are mixed: some studies link high fecal and plasma SCFA levels to better ICI outcomes [117,118,119], while others find no significant correlation [120,121,122]. Such discrepancies may reflect context-dependent effects of SCFAs on regulatory and effector T cells within the tumor microenvironment [38,123].
5.3.2. Inosine
Inosine, a purine nucleoside, is involved in purine metabolism, RNA function, and immune modulation [124]. Produced by bacteria such as Bifidobacterium pseudolongum, inosine activates antitumor T cells through adenosine A2A receptor signaling in preclinical models [40]. In RCC patients, higher plasma inosine levels were associated with response to nivolumab [125].
5.3.3. Tryptophan Metabolites
The essential amino acid tryptophan can be metabolized through multiple pathways that influence both cancer progression and antitumor immunity, including the kynurenine, indole-3-pyruvate, and serotonin pathways. Tumor cells frequently channel tryptophan into the immunosuppressive kynurenine pathway, whereas commensal gut microbes can redirect it toward alternative routes. For example, gut bacteria can convert tryptophan into a ligand for the aryl hydrocarbon receptor (AHR), a key regulator of intestinal homeostasis [126]. Certain metabolites, such as indole-3-aldehyde (I3A) produced by Lactobacillus reuteri, enhance CD8+ T cell activity in mouse models [127]. In cancer patients, plasma biomarkers, including the kynurenine-to-tryptophan (Kyn/Trp) ratio and metabolites such as I3A and 3-hydroxyanthranilic acid (3-HAA), have been correlated with ICI efficacy [127,128,129].
5.3.4. Secondary Bile Acids
In addition to their role in lipid absorption, bile acids function as systemic signaling molecules regulating host metabolism and immune function [130]. Primary bile acids are synthesized in the liver and subsequently converted by microbial enzymes, mainly from Clostridium species such as Clostridium butyricum, into secondary bile acids. These secondary bile acids display stronger activation of host nuclear receptors than their primary counterparts [131]. In hepatocellular carcinoma (HCC) models, accumulation of conjugated bile acids in tumors impairs anti-PD-1 efficacy, whereas dietary supplementation of ursodeoxycholic acid (UDCA) suppresses tumor growth and promotes T cell responses [132]. Clinically, HCC patients receiving ICIs who had fecal enrichment of UDCA and ursocholic acid demonstrated improved treatment outcomes [133].
5.4. The Importance of Temporal Dynamics
The gut microbiome is not static; its composition shifts dynamically following ICI treatment, with distinct patterns emerging between responders and non-responders. Notably, certain microbial alterations emerge only after treatment initiation, rather than at baseline.
In melanoma and NSCLC patients receiving ICI therapy, responders exhibit stable microbial taxa and functional profiles over time compared to non-responders [134,135]. Other studies have shown that both responders and non-responders develop unique microbial abundance patterns after ICI initiation, even when baseline differences are minimal or absent [90,136,137].
5.5. Tools Incorporating Microbial Signature to Predict Prognosis and ICI Response
Emerging tools are being developed to integrate microbial signatures into prognostic models and ICI response prediction. Although still in early stages and requiring further validation, these approaches demonstrate the translational potential of microbiome-informed biomarkers.
As a biomarker, the gut microbiome offers both predictive and prognostic potential in immuno-oncology. Specific microbial signatures and functional profiles have been linked to ICI response, resistance, and toxicity, suggesting that microbiome-based metrics could complement existing biomarkers. However, it is important to note that although several studies report similar microbiome signals, the findings remain inconclusive, as not all studies consistently replicate the same results. Ongoing efforts to standardize studies and improve analytical pipelines in microbiome research are expected to enhance reproducibility and reliability.
6. Therapeutic Applications of the Gut Microbiome
The early evidence supporting the therapeutic potential of the gut microbiome in oncology came from preclinical studies in which fecal microbiota transplantation (FMT) from ICI-responsive patients into germ-free mice enhanced antitumor immune responses, whereas FMT from non-responders did not [96,112,115]. These findings were later translated into early-phase clinical trials. Subsequent proof-of-concept clinical studies in ICI-refractory melanoma patients confirmed that FMT, when combined with re-induction anti-PD1, could overcome ICI resistance in a subgroup of patients by altering the gut microbiome and tumor microenvironment [140,141]. Building on these findings, several strategies are now under investigation to modulate the microbiota to enhance immunotherapy efficacy and mitigate treatment-related toxicity. These include FMT, supplementation of pre-, pro-, and postbiotics (collectively referred to as biotics), engineered microbial strains, and antibiotic modulation (Figure 3).
Therapeutic applications of the gut microbiome to enhance ICI therapy. The gut microbiome can influence both efficacy and toxicity of immune checkpoint inhibitors (ICIs). Therapeutic strategies to optimize microbiome composition include: (1) Fecal microbiota transplantation (FMT): transfer of a healthy or responder-derived microbial community; (2) Antibiotic stewardship: minimizing microbiome-disruptive antibiotic use; (3) Biotic supplementation: administration of prebiotics, probiotics, or postbiotics to restore beneficial microbial function; and (4) Engineered microorganisms: synthetic or genetically modified bacteria designed to deliver immunomodulatory molecules. These interventions aim to enhance ICI response and reduce immune-related adverse events. Created with BioRender.com/goujhtp (accessed on 9 November 2025).
6.1. Fecal Microbiota Transplant (FMT) to Enhance ICI Efficacy
Early-phase studies of FMT combined with anti-PD1 re-challenge in ICI-refractory melanoma showed encouraging signals, with overall response rates (ORR) of 20–30% and durable disease control exceeding 6–12 months in responders. Responders of FMT typically demonstrated greater donor microbiome engraftment and enrichment of specific bacterial taxa. More recent studies have expanded FMT evaluation to earlier-line settings and across multiple tumor types (Table 3a,b).
FMT was generally safe and feasible across studies, with most adverse events related to mild gastrointestinal symptoms (grade 1–2). Although donor-derived infection is a recognized potential risk of FMT [123], it has not yet been reported in studies combining FMT with ICI therapy. However, the FMT-LUMINate melanoma cohort reported a notably high incidence (65%) of ≥grade 3 irAEs, likely reflecting the additive toxicity of dual ICI therapy and potential donor-related immune effects, as 43% of participants received FMT from the same donor. This finding underscores that FMT is not without risk and highlights the critical importance of donor selection and stringent safety monitoring in future trial designs.
Despite promising efficacy signals, FMT protocols have shown considerable heterogeneity, including donor selection (responder-derived versus healthy individuals), use of different preconditioning regimens (antibiotics and bowel preparation), route of administration (oral or colonoscopy), and maintenance dosing. Further research is needed to clarify cancer-specific and regimen-dependent differences in microbiome–immune interactions.
Higher microbial engraftment has consistently been associated with improved clinical outcomes. Identification of species-specific engraftment patterns and integrating metagenomic analyses may enable personalized FMT strategies [149,150,151]. Ongoing efforts aim to define the optimal donor characteristics, preparation, and delivery methods to maximize therapeutic benefit.
| Study | N | Phase | Population | Intervention | Key Outcomes | ≥Grade 3 irAEs |
|---|---|---|---|---|---|---|
| ()a | ||||||
| Baruch et al. (2021) [] [140] | 10 | I | ICI-refractory melanoma | Responder-derived FMT + Nivolumab | ORR 30%; all responders with >6 mo PFS | 0% |
| Davar et al.(2021) [] [141] | 15 | I | ICI-refractory melanoma | Responder-derived FMT + Pembrolizumab | ORR 20%; 3 patients with >12 mo stable disease | 0% |
| MiMic(2023)[,] [142] [143] | 20 | II | Untreated meta-static melanoma | Healthy donor FMT + pembrolizumab or nivolumab | ORR 65%; median PFS 29.6 mo; median OS 52.8 mo | 25% |
| FMT-LUMINate(2024) [] [144] | 20 | II | Untreated meta-static melanoma | Healthy donor FMT + anti-PD1 + anti-CTLA4 | ORR 75% | 65%(myocarditis 15%) |
| ()b | ||||||
| Kim et al.(2024) [] [145] | 13 | I | ICI-refractory cancer(gastric n = 4, esophageal n = 5, HCC n = 4) | Responder-derived FMT + nivolumab | ORR 7.7% | 7.7% |
| RENMIN-215(2023)[,] [146] [147] | 20 | II | Refractory MSS colorectal cancer (≥2 prior lines) | Responder-derived FMT + Tislelizumab + Fruquintinib | ORR 20%; median PFS 9.6 mo; median OS 13.7 mo | 10% |
| FMT-LUMINate(2024) [] [144] | 20 | II | Untreated meta-static NSCLC | Healthy donor FMT + anti-PD1 | ORR 80% | 0% |
| TACITO(2024) [] [148] | 50 | II | Untreated meta-static RCC | Intervention:Responder-derived FMT + pembrolizumab + axitinibControl:Placebo + pembrolizumab + axitinib | ORR 54% vs. 28%Median PFS 14.2 vs. 9.2 mo;1-year PFS rate 66.7% vs. 35%; median OS NR vs. 25.3 mo | 10% |
6.2. Fecal Microbiota Transplant (FMT) to Mitigate ICI-Induced Colitis
Colitis is the most extensively studied irAE in relation to gut microbiome composition. Reduced microbiome diversity and prior antibiotic use have been linked to the development of ICI-related colitis [152,153,154,155]. Shifts in microbial composition, particularly with strain-specific enrichment, have also been observed; however, the results are inconsistent [156,157,158,159]. Administration of F. prausnitzii and Bifidobacterium helps mitigate ICI-related colitis in animal models [160,161]. Several case reports have shown improvement of steroid-refractory immune-related colitis following FMT administration [162,163]. Ongoing clinical trials are exploring the benefits of FMT in preventing (Clinical Trials.gov identifiers: NCT04163289↗ and NCT06508034↗) and treating immune-related colitis in patients receiving ICIs (Clinical Trials.gov identifiers: NCT04038619↗, NCT06206707↗, and NCT06499896↗). Preliminary data from a prospective study suggest that frontline FMT is safe and can be an effective treatment, reducing the need for corticosteroids [164].
6.3. Supplementation with Biotics: A Targeted Approach
Unlike FMT, which introduces the entire microbial community and environment, biotic interventions such as prebiotics, probiotics, and postbiotics provide a more targeted approach to transform the gut microbiome and host immune system. According to the International Scientific Association for Probiotics and Prebiotics (ISAPP), the definitions of prebiotics, probiotics, and postbiotics are summarized in Table 4.
Traditional probiotics mainly include a limited number of species, such as Lactobacillus and Bifidobacterium, which have a long history of safe use as food ingredients or dietary supplements. Advances in microbiology techniques and bioinformatics have enabled the precise identification and culture of novel gut microbes with therapeutic potential. These next-generation probiotics (NGPs) include Prevotella copri, Christensenella minuta, Parabacteroides goldsteinii, Akkermansia muciniphila, Bacteroides thetaiotaomicron, Faecalibacterium prausnitzii, Bacteroides fragilis, and Eubacterium hallii [168,169]. Notably, A. muciniphila and F. prausnitzii have shown potential to enhance ICI efficacy in preclinical and translational studies, as mentioned above.
Several phase 1 studies have explored the benefits of adding probiotics in combination with ICIs in advanced RCC patients (Table 5).
Although studies employing Clostridium butyricum CBM588—a butyrate-producing bacterial strain—did not increase the abundance of beneficial Bifidobacterium spp., the observed improvement in clinical outcomes suggests that CBM588 may exert its effects through alternative mechanisms, such as modulation of microbial metabolites or enrichment of other taxa like Ruminococcaceae, which have been associated with favorable ICI responses [171].
Despite promising mechanistic insights, clinical data on the use of biotics to enhance immunotherapy in cancer patients remain in the early stages. Current challenges include heterogeneity and a lack of standardized quality control for biotic products, interference from patients’ background diets, and limited trial designs that account for microbiome variability. Therefore, no firm recommendations on routine use of prebiotics, probiotics, or postbiotics in ICI-treated patients can be made at this time. Several ongoing trials are now investigating dietary interventions and biotic supplementation as adjuncts to ICIs across multiple cancer types, aiming to establish whether microbiome-targeted strategies can improve response rates and reduce immune-related toxicities [173].
| Biotic | Definition | Function | Examples |
|---|---|---|---|
| Prebiotics | substrates that are selectively utilized by host microorganisms, conferring a health benefit | nourish beneficial microbes, promoting their growth and metabolite production | Galactooligosaccharides (GOS), Fructooligosaccharides (FOS), Inulin, lactulose; naturally present in whole grains, onions, garlic, asparagus, bananas |
| Probiotics | live microorganisms that, when administered in adequate amounts, confer a health benefit. | directly introduce beneficial microbes to shape the gutenvironment | fermented foods such as yogurt, kefir, miso, natto, kimchi, and some cheeses containing specific live microbes (e.g.,,)Lactobacillus acidophilusBifidobacterium longum |
| Postbiotics * | preparation of inanimate microorganisms and/or their components that confer a health benefit. | deliver beneficial effectswithout living organisms,using inactivated microbial cells, components, ormetabolites | heat-inactivatedor, bacterial lysatesBifidobacteriumLactobacillus |
| Study | N | Phase | Intervention | Primary Endpoint | Results and Safety |
|---|---|---|---|---|---|
| Dizman et al.(2022) [] [170] | 30 | I | Nivolumab + ipili-mumab ± CBM588 ()Clostridium butyricum | Change inspp. abundance at 12 weeksBifidobacterium | No difference inspp. abundance. The CBM588 arm had a significantly improved PFS (12.7 vs. 2.5 mo) and ORR (58% vs. 20%). No significant difference in toxicity between the two arms.Bifidobacterium |
| Ebrahimi et al.(2024) [] [171] | 30 | I | Cabozantinib + nivolumab ± CBM588 | Change inspp. abundance at 13 weeksBifidobacterium | No difference inspp. abundance. The CBM588 arm had a significantly higher ORR (74% vs. 20%,= 0.01). 6-mo PFS: 84% vs. 60%. No significant difference in toxicity between the two arms.Bifidobacteriump |
| Derosa et al.(2025) [] [172] | 9 | I | Nivolumab + ipili-mumab + Onco-bax-AK (strain p2261, SGB9228) in patients lacking stool®A. massiliensisAkkermansia | ORR,pharmacodynamics, safety | ORR 50% with evidence ofimmune and metabolicmodulation. No toxicity related to Onco-bax-AK observed.® |
6.4. Engineered Microorganisms
Advances in genetic and synthetic biology have enabled the development of engineered microorganisms that can augment immunotherapy against cancer in multiple aspects. By modifying microbial chassis, researchers can add features that promote immune activation while minimizing systemic side effects associated with naturally derived microbes (Table 6).
Beyond antigen delivery and cytokine release, engineered strains can also remodel the tumor microenvironment and deliver immunomodulatory payloads directly into the microenvironment. However, challenges include limited tumor colonization in humans, competition with endogenous microbiota, potential systemic inflammation, and reproducibility [177,178].
| Mechanisms | Examples |
|---|---|
| Presentation of tumor antigens and cancer vaccine carriers | Phase 2: ADXS-503, an engineeredexpressing 22 common NSCLC antigens, combined with pembrolizumab after progression. Induced antigen-specific T-cell responses with 15% ORR (2/13) []. Listeria monocytogenes [174] Phase 2a: VXM01, an oral VEGFR2 DNA vaccine delivered via engineeredTy21a, combined with avelumab in recurrent glioblastoma. Showed 12% ORR (3/25) []. Salmonella Typhi [175] |
| Cytokine and chemokine release to enhance immune function | Phase 1: SYNB1891, engineeredNissle expressing a STING agonist, given intratumorally ± atezolizumab. Activated IFN pathways and immune gene signatures in refractory cancers []. E. coli [176] |
6.5. Antibiotic Stewardship
Inappropriate antibiotic use can disrupt intestinal homeostasis and cause dysbiosis characterized by reduced microbial diversity, expansion of potentially harmful strains, and depletion of beneficial taxa. Intestinal dysbiosis has been associated with impaired efficacy of ICIs. While randomized controlled trials studying this association are not feasible, extensive preclinical data and multiple large observational studies and meta-analyses [179,180] consistently demonstrate that antibiotic exposure around the time of ICI initiation (up to 90 days before and after) is linked to inferior clinical outcomes.
Current recommendations emphasize strict adherence to international antibiotic stewardship principles [181,182]. Clinicians should confirm the presence of infection before initiating antibiotics, prioritize narrow-spectrum agents when possible, prescribe the shortest effective duration, and regularly assess the indication. These measures help minimize the negative impact of antibiotics on ICI efficacy.
7. Conclusions and Outlook
The clinical translation of gut microbiome research in immuno-oncology depends on overcoming key challenges of standardization and validation. Future progress will require:
The relationship between the gut microbiome and cancer immunotherapy has evolved from a compelling association to an emerging field with growing clinical relevance and tangible translational potential. Looking forward, integrating microbiome-derived biomarkers with established predictors such as PD-L1 and TMB may enable the development of composite stratification tools, improving patient selection and optimizing immunotherapy outcomes. For practicing medical oncologists, the most immediate and impactful strategies remain prudent antibiotic stewardship and encouraging patient enrollment in microbiome-focused clinical trials.
In summary, the gut microbiome is both a powerful biomarker and a therapeutic target that can shape immunotherapy outcomes. Continued methodological refinement, innovative clinical approaches, and translational research will be critical to realizing its full potential and bringing microbiome-informed strategies into routine oncology practice.
Abbreviations
The following abbreviations are used in this manuscript:
| 16S rRNA | 16S ribosomal RNA |
| 3-HAA | 3-hydroxyanthranilic acid |
| A2A | Adenosine A2A receptor |
| AHR | Aryl hydrocarbon receptor |
| CFU | Colony-forming units (e.g., CFU/g) |
| CMS | Consensus Molecular Subtypes (colon cancer) |
| CTLA-4 | Cytotoxic T-lymphocyte–associated protein 4 |
| CXCL9/CXCL10 | C-X-C motif chemokine ligand 9/10 |
| DC/DCs | Dendritic cell(s) |
| dMMR | Deficient mismatch repair |
| DNA | Deoxyribonucleic acid |
| E. coli | Escherichia coli |
| FDA | U.S. Food and Drug Administration |
| FMT | Fecal microbiota transplantation |
| GPCR | G-protein–coupled receptor |
| H&E | Hematoxylin and eosin (stain) |
| HCC | Hepatocellular carcinoma |
| HDAC | Histone deacetylase |
| HLA | Human leukocyte antigen |
| ICI/ICIs | Immune checkpoint inhibitor(s) |
| IFN-γ | Interferon-gamma |
| IL-1/IL-12 | Interleukin-1/Interleukin-12 |
| IHC | Immunohistochemistry |
| I3A | Indole-3-aldehyde |
| irAE(s) | Immune-related adverse event(s) |
| Kyn/Trp | Kynurenine-to-tryptophan ratio |
| LPS | Lipopolysaccharide |
| MDSC(s) | Myeloid-derived suppressor cell(s) |
| MLH1, PMS2, MSH2, MSH6 | Mismatch repair proteins/genes |
| MMR | Mismatch repair |
| MS | Mass spectrometry |
| MSI | Microsatellite instability |
| MSI-H | Microsatellite instability–high |
| NGP(s) | Next-generation probiotic(s) |
| NGS | Next-generation sequencing |
| NK (cells) | Natural killer (cells) |
| NMR | Nuclear magnetic resonance |
| NR | Not reached (survival endpoint) |
| NSCLC | Non-small-cell lung cancer |
| ORR | Objective response rate |
| OS | Overall survival |
| PCR | Polymerase chain reaction |
| PD-1 | Programmed cell death protein 1 |
| PD-L1 | Programmed death-ligand 1 |
| PFS | Progression-free survival |
| POLE/POLD1 | DNA polymerase epsilon/delta 1 (genes) |
| qPCR | Quantitative PCR |
| RCC | Renal cell carcinoma |
| RNA-Seq | RNA sequencing (metatranscriptomics) |
| SCFA(s) | Short-chain fatty acid(s) |
| STING | Stimulator of interferon genes |
| TIL(s) | Tumor-infiltrating lymphocyte(s) |
| TLR(s) | Toll-like receptor(s) |
| TMB | Tumor mutational burden |
| TNF-α | Tumor necrosis factor-alpha |
| UDCA | Ursodeoxycholic acid |
| VEGFR2 | Vascular endothelial growth factor receptor 2 |
Author Contributions
Conceptualization: T.S., A.P. and S.C.; Data curation: T.S. and P.E.; Visualization: T.S. and P.E.; Interpretation of data and literature: T.S., P.E., A.P., S.C., M.V.R. and F.A.F.; Writing—original draft preparation: T.S.; Writing—review and critical revision for important intellectual content: P.E., A.P., S.C., M.V.R. and F.A.F.; Supervision: A.P. and S.C. All authors have read and agreed to the published version of the manuscript.
Data Availability Statement
No new data were created or analyzed in this study.
Conflicts of Interest
A.P. is employed by Pendulum Therapeutics, Inc., a biotechnology company developing microbiome-targeted products, including formulations using Akkermansia muciniphila. This review was conducted independently of the company, which had no role in the design, interpretation, or preparation of the manuscript. The remaining authors declare no conflicts of interest.
Funding Statement
This research received no external funding.
Footnotes
References
Associated Data
Data Availability Statement
No new data were created or analyzed in this study.