Gut mucosal microbiota profiles linked to colorectal cancer recurrence

Rui-Xue Huo,Yi-Jia Wang, Shao-Bin Hou,Wei Wang,Chun-Ze Zhang, Xue-Hua Wan

Abstract

BACKGROUND Emerging evidence links gut microbiota to various human diseases including colorectal cancer (CRC) initiation and development. However, gut microbiota profiles associated with CRC recurrence and patient prognosis are not completely understood yet, especially in a Chinese cohort.

AIM To investigate the relationship between gut mucosal microbiota profiles and CRC recurrence and patient prognosis.

METHODS We obtained the composition and structure of gut microbiota collected from 75 patients diagnosed with CRC and 26 healthy controls. The patients were followed up by regular examination to determine whether tumors recurred. Triplet-paired samples from on-tumor, adjacent-tumor and off-tumor sites of patients diagnosed with/without CRC recurrence were analyzed to assess spatial-specific patterns of gut mucosal microbiota by 16 S ribosomal RNA sequencing. Next, we carried out bioinformatic analyses, Kaplan-Meier survival analyses and Cox regression analyses to determine the relationship between gut mucosal microbiota profiles and CRC recurrence and patient prognosis.

RESULTS We observed spatial-specific patterns of gut mucosal microbiota profiles linked to CRC recurrence and patient prognosis. A total of 17 bacterial genera/families were identified as potential biomarkers for CRC recurrence and patient prognosis, including Anaerotruncus, Bacteroidales,Coriobacteriaceae, Dialister, Eubacterium, Fusobacterium, Filifactor, Gemella, Haemophilus, Mogibacteriazeae, Pyramidobacter, Parvimonas, Porphyromonadaceae, Slackia, Schwartzia, TG5 and Treponema.

CONCLUSION Our work suggests that intestinal microbiota can serve as biomarkers to predict the risk of CRC recurrence and patient death.

Key Words: Gut microbiota; Colorectal cancer; Prognosis; Colorectal cancer recurrence; Biomarker; 16 S rRNA sequencing analysis

INTRODUCTION

Colorectal cancer (CRC) is a major cause of cancer-related deaths with the third highest mortality and the fourth highest incidence worldwide, according to GLOBOCAN 2020 (global cancer statistics)[1 ],which indicates a public health issue. Although many new treatment options of CRC have doubled,survival prognosis for early-stage patients with non-metastasized disease is still better than that for advanced-stage patients[2 ]. Currently, treatment of CRC mainly depends upon tumor-node-metastasis(TNM) stage of disease, and the patient’s physical fitness and intent. However, previous studies showed that disease recurrence was observed in 40 % of treated patients with stage Ι-ΙΙ CRC (lymph node negative postoperative) and 70 % of those with stage ΙΙΙ CRC[3 ], which is proposed to be related to rat sarcoma viral oncogene and microsatellite status[4 ]. Thus, treatment strategy merely depending on CRC TNM stage may cause over-treatment or under-treatment, leading to CRC recurrence. Moreover, the molecular mechanisms behind CRC recurrence are not yet completely understood. Therefore, we still need to explore more suitable biomarkers for assessing prognosis of CRC patients in order to achieve optimal personalized treatment.

Ιn addition to hereditary and lifestyle factors, the human gut microbiota is considered as an important risk factor for CRC initiation as well as development. With the continuous development of high-throughput sequencing, the compositional structure of the human gut microbiota is revealed to be closely involved in CRC initiation, development and treatment[5 ]. Moreover, pathogenic bacteria have been identified from the human gut microbiota and their procarcinogenic properties have been demonstrated to play a role in causing gut microbial dysbiosis in the complex environment of the human intestinal tract. Certain bacterial species, includingBacteroides fragilis(B. fragilis),Clostridium septicum,Enterococcus faecalis,Escherichia coli,Fusobacteriumspp.,Helicobacter pyloriandStreptococcus bovishave been identified to play a role in driving colorectal carcinogenesis[6 ]. The mechanisms behind these pathogenic bacteria involve bacterial-derived genotoxicity and other virulence factors that regulate host defense systems, metabolism, oxidative stress and antioxidative defense modulation[6 ].

Evidence has linked gut microbiota to prognosis of CRC. A pilot study has shown that high abundance ofFusobacterium nucleatum(F. nucleatum) andB. fragiliswere independent indicators for poor patient survival, while high abundance ofFaecalibacterium prausnitziipredicted improved survival rate[7 ]. Ιn addition, most studies supported that increased relative abundance ofB. fragilisandF. nucleatumwere associated with short-term survival and late stage of CRC[8 ]. EnterotoxigenicB. fragilis(ETBF) andFusobacteriumspp. levels were significantly higher in late stage (ΙΙΙ/ΙV) CRC than those in early stage(Ι/ΙΙ) CRC, and high abundance ofFusobacteriumwas reported to be associated with high microsatellite instability (MSΙ)[9 ,10 ]. Compared toF. nucleatum-negative cases, multivariable hazard ratio for CRCspecific mortality inF. nucleatum-high cases was 1 .58 [9 ]. After neoadjuvant chemoradiotherapy,F.nucleatumpersistence was associated with high relapse rates in locally advanced CRC[11 ]. CRC patients with low levels ofF. nucleatumhad significantly longer overall survival (OS) and disease-free survival(DFS) than patients with moderate and high levels ofF. nucleatumthat were obvious in late-stage CRC patients[12 -15 ]. However, extensive bacterial taxa associated with prognosis of CRC are unclear,especially in a Chinese cohort.

To investigate the profiles of gut mucosal microbiota associated with CRC recurrence and survival of CRC patients, we collected gut mucosal microbiota from CRC patients when they received radical resection or palliative surgery in Tianjin Union Medical Center, China. For each patient, triplet-paired CRC samples were collected from on-tumor, adjacent-tumor and off-tumor sites. Additional samples were collected from 26 healthy controls. We performed 16 S ribosomal RNA (rRNA) gene sequencing and analyses on these gut mucosal microbiota. Next, we carried out Kaplan-Meier survival curve analyses for OS and DFS. Our data suggest that a number of bacterial genera/families, includingAnaerotruncus,Bacteroidales,Coriobacteriaceae,Dialister,Eubacterium,Fusobacterium,Filifactor,Gemella,Haemophilus,Mogibacteriazeae,Pyramidobacter,Parvimonas,Porphyromonadaceae,Slackia,Schwartzia, TG5 andTreponema, are associated with survival of CRC patients and CRC recurrence. We further performed the univariate and multivariate Cox regression analyses. Our data reveal that high abundance ofAnaerotruncus,Bacteroidales,Coriobacteriaceae,Dialister,Eubacterium,Filifactor,Haemophilus,Mogibacteriazeae,Pyramidobacter,Slackia,Treponemaand TG5 are associated with worse OS or DFS.

MATERIALS AND METHODS

Patients and sample collection procedures

This study analyzed 69 pathologically confirmed CRC patients, who received radical or palliative surgeries at Tianjin Union Medical Center, Tianjin, China from December 2016 to September 2017 . These patients were followed up by regular examination or telephone survey. DFS was defined as the time period from the date of surgery to the time of tumor recurrence, and OS was defined as the time period from the date of surgery to the time of death. Our study was conducted in accordance with the Declaration of Helsinki. Every patient provided written informed consent for the collection of samples and subsequent analysis when required, and the study was approved by the Ethics Committee of Tianjin Union Medical Center. The TNM staging was determined according to the American Joint Committee on Cancer staging handbook (8thedition). Whether a patient received chemotherapy or not depended on his/her TNM stage, physical state score and intention. Ιmaging examination was arranged for every 2 -6 mo or when a patient’s condition changed to determine whether the disease recurrence occurred.

DNA library preparation and 1 6 S rRNA sequencing

ZR Fungal/Bacterial DNA kit (Zymo Research, Ιrvine, CA, United States) was used to isolate bacterial DNA from intestinal microbiota samples according to the manufacturer’s instructions. Quant-iT PicoGreen dsDNA assay kit (Thermo Fisher, Sunnyvale, CA, United States) was used to quantify the DNA amounts. The hypervariable regions of 16 S rRNA gene amplicon libraries targeting the V3 -V4 regions were prepared according to the Ιllumina manufacturer’s manual. The amplification primers were used according to the Ιllumina manufacturer’s manual. The forward and reverse primers were used as follows: 5 ’-TCGTCGGCAGCGTCAGATGTGTATAAGAGACAGCCTACGGGNGGCWGCAG and 5 ’-GTCTCGTGGGCTCGGAGATGTGTATAAGAGACAGGACTACHVGGGTATCTAATCC. The products of polymerase chain reaction were examined using agarose gel electrophoresis (1 % concentration of agarose gel; 100 V; 40 min electrophoresis time). The AMPure XP beads (Beckman Coulter,Fullerton, CA, United States) were used to purify the amplified DNA libraries, and Quant-iT PicoGreen dsDNA assay kit (Thermo Fisher, Sunnyvale, CA, United States) was used to quantify the DNA library amounts. All the DNA samples were stored at -20 °C until used.

Quality control, operational taxonomic unit picking and diversity analyses of 1 6 S rRNA amplicons

The 16 S rRNA amplicon libraries were sequenced for 2 × 300 bp on Ιllumina MiSeq platform. The read information was listed in Supplementary Table 1 . The FastQC program was used to perform quality control and filtering of raw paired-end reads (https://www.bioinformatics.babraham.ac.uk/projects/fastqc/, accessed on 5 June 2019 ). Next, PandaSeq v2 .10 was used to assemble paired-end reads with default parameters[16 ]. The QΙΙME pipeline v1 .9 .1 (http://qiime.org/home_static/dataFiles.html,accessed on June 5 , 2019 ) and Greengenes database v13 .8 were used for de novo operational taxonomic unit (OTU) picking and taxonomic assignment[17 ]. Briefly, we generated the mapping file that contains all the information about the sequencing samples including sample ΙD, barcode sequences and sample types. The python command, pick_otus.py, was used to pick OTUs based on sequence similarity(threshold of 97 %) of the assembled reads, which is commonly used to define bacterial species. The python command, pick_rep_set.py, was used to pick the representative sequences for each OTU.USEARCH 6 .1 was used for chimera detection and filtering. The python command, assign_taxonomy.py, was used to assign taxonomy to OTU representative sequences. The python command,make_rarefaction_plots.py and online MicrobiomeAnalyst (https://dev.microbiomeanalyst.ca/MicrobiomeAnalyst/home.xhtml, accessed on 28 August 2021 ) were used to calculate alpha diversities within the samples[18 ,19 ]. The 16 S rRNA paired-end reads have been submitted to the Sequence Read Archive database at the National Center for Biotechnology Ιnformation website under accession number PRJNA606879 .

Bioinformatic analyses of gut mucosal microbiota for CRC patients

The beta diversity of gut mucosal microbiota among the samples collected from CRC patients with and without recurrence was calculated using principal component analysis on MicrobiomeAnalyst website[18 ,19 ]. The linear discriminant analysis (LDA) effect size was analyzed using online MicrobiomeAnalyst[18 ,19 ].

Statistical analysis

Statistical analyses were performed using SPSS Version 23 . The statistical significance of multiple sample comparisons were calculated using one-way analysis of variance with Kruskal-Wallis test. The Kaplan-Meier survival curves for OS and DFS and the optimal cutoff value of RiskScore were calculated using R software package maxstat (maximally selected rank statistics with severalPvalue approximations version: 0 .7 -25 )[20 ]. We set the minimum number of samples in the grouping to be greater than 25 % and the maximum number of samples in the grouping to be less than 75 % and finally obtained the optimal cutoff value of each bacterial taxa. Based on this cutoff threshold, the patients were divided into groups with high and low abundance of the bacterial taxa. Furthermore, the survivfit function of R software was used to analyze the prognostic differences between the two groups, and the significance of prognostic differences between the two groups was evaluated by logrank test. According to the cutoff value of each bacterial taxon, we divided the patients into groups with high and low abundance of the bacterial taxa and then conducted Cox regression analyses. The Cox regression analyses based on the proportional hazards model were carried out using SPSS v. 23 program.

RESULTS

Clinicopathological features of CRC patients

We summarized the patients’ clinicopathological data in Table 1 . The median age of 75 patients was 63 .4 years, and 60 % of them were males. The pathological type of all patients was categorized as adenocarcinoma, and most of the tumor cells were poorly differentiated. Most patients were diagnosed as microsatellite stable based on immunohistochemical evaluation of components of the mismatch repair machinery, including MLH1 , MSH2 , MSH6 and PMS2 . All patients did not receive chemotherapy or other antitumor therapy before surgery. After surgery, 44 of 75 patients received chemotherapy based on FOLFOX (CapeOX) or FOLFΙRΙ regimen, 4 of them received radiotherapy, and 6 of them received targeted therapy. The median follow-up duration for all cases after surgery was 51 .2 mo (2 .90 -57 .03 mo).There were 6 patients who failed to be followed up. Until August 23 , 2021 , a total of 17 patients diagnosed with Ι-ΙΙΙ stages had relapsed and 20 patients had died.

Altered alpha-diversity of gut mucosal microbiota at adjacent-tumor sites for CRC recurrence

Although tumor tissues can be removed by surgery, the microbiota residing in the tumor surrounding tissues,e.g., those at the adjacent-tumor sites as well as those in the remaining intestinal tissues where tumors are removed, may retain pathogenic bacteria that have the capabilities to drive CRC, leading to CRC recurrence. Therefore, we hypothesize that gut mucosal microbiota profiles at on-tumor or adjacent-tumor sites may be linked to CRC recurrence. To examine this, we assessed microbial alphadiversities of biopsy samples collected from on-tumor, adjacent-tumor and off-tumor sites of patients with and without CRC recurrence. The 16 S rRNA gene hypervariable V3 -V4 regions were sequenced and analyzed for five α-diversity indices including Chao1 , Fisher, Observed OTU, Shannon and Simpson (Figure 1 ). Analyses of species variations based on these five metrics consistently indicated that species diversities at on-tumor or off-tumor sites of patients with and without CRC recurrence showed no significant differences (Studentt-test,P< 0 .05 ) (Figure 1 ). Analyses of species variations based on Chao1 (Student t-test, P = 0 .0092 ), Fisher (Student t-test, P = 0 .0092 ) and observed OTU (Studentt-test,P= 0 .0092 ), but not Shannon (Student t-test, P = 0 .1314 ) and Simpson (Student t-test, P = 0 .2513 ), showed significant differences at adjacent-tumor sites of patients with and without CRC recurrence (Figure 1 ).Although Shannon and Simpson metrics did not show statistical significance, analyses of the αdiversities based on the five metrics suggested that at adjacent-tumor sites, those from patients with CRC recurrence were higher than those from patients without recurrence (Figure 1 ). These data suggest that there is no significant difference of composition of gut mucosal species at on-tumor and off-tumor sites between patients with and without CRC recurrence. However, compositions of internal species showed differences at adjacent-tumor sites between patients with and without CRC recurrence.

Microbiota profiles linked to CRC recurrence

To assess whether the structure diversities (beta-diversity) of gut microbiota show differences between patients with and without CRC recurrence, we performed principal component analysis for abundance of genera identified at on-tumor, adjacent tumor and off-tumor sites of CRC patients diagnosed with and without disease recurrence. The microbiota structure diversities at on-tumor, adjacent tumor and off-tumor sites of CRC patients diagnosed with and without disease recurrence showed differences(Figure 2 ), suggesting that the structures of gut microbiota were different at these sites in patients with and without CRC recurrence.

We next compared the differential relative abundance of bacterial taxa at the phylum level between patients with and without CRC recurrence. Among all the samples,Firmicutes,Proteobacteria,BacteroidetesandFusobacteriashowed the top relative abundance (Figure 3 ).Firmicutes,BacteroidetesandFusobacteriashowed higher relative abundance at on-tumor sites of patients diagnosed with CRC recurrence than those at on-tumor sites of patients diagnosed without CRC recurrence (Figure 3 ). At adjacent-tumor sites, the relative abundance ofFusobacteriain patients with CRC recurrence were dramatically higher than those in patients without CRC recurrence (Figure 3 ). By contrast, the relative abundance ofFusobacteriaat off-tumor sites showed no differences between patients with and without CRC recurrence (Figure 3 ). The relative abundance ofFirmicutesandBacteroidetesat off-tumor sites of patients with CRC recurrence were lower than those of patients without CRC recurrence (Figure 3 ).Collectively, these data suggest that species fromFusobacteria,BacteroidetesandFirmicutesmay play roles in worsening or improving the patient prognosis.

Figure 1 Microbial alpha-diversities showing significant differences at adjacent-tumor site. A: Alpha diversity evaluated using Chao1 index; B:Alpha diversity evaluated using Fisher index; C: Alpha diversity evaluated using observed operational taxonomic unit index; D: Alpha diversity evaluated using Shannon index; E: Alpha diversity evaluated using Simpson index. health: Healthy control; nn: Off-tumor site of patient without colorectal cancer (CRC) recurrence;nr: Off-tumor site of patient with CRC recurrence; pn: Adjacent-tumor site of patient without CRC recurrence; pr: Adjacent-tumor site of patient with CRC recurrence;tn: On-tumor site of patient without CRC recurrence; tr: On-tumor site of patient with CRC recurrence. Alpha-diversity differences were compared using student’s ttest.

Altered gut mucosal microbiota signatures in CRC recurrence

We next carried out the linear discriminant analysis effect size to predict site-specific biomarkers that are associated with CRC recurrence. By setting LDA score > 3 .0 [false discovery rate (FDR) adjustedPvalue < 0 .1 ], a total of 100 genera were identified to show significant differences of relative abundance between patients with and without CRC recurrence (Figure 4 , Supplementary Table 2 ). The top 10 genera/families with the highest LDA scores wereFusobacterium(LDAscore = 5 .56 , FDR adjustedP=0 .0026 ), Faecalibacterium (LDAscore = 5 .29 , FDR adjusted P = 0 .0176 ), Peptostreptococcus (LDAscore = 5 .13 ,FDR adjustedP= 0 .0026 ), Streptococcus (LDAscore = 5 .08 , FDR adjusted P = 0 .0639 ),Parvimonas(LDAscore = 5 .04 , FDR adjusted P = 0 .0072 ), Burkholderiales (LDAscore = 5 .03 , FDR adjusted P = 0 .0018 ),Pseudomonas(LDAscore = 4 .82 , FDR adjusted P = 0 .0301 ), Caulobacteraceae (LDAscore = 4 .77 , FDR adjustedP= 0 .0043 ), Mitsuokelia (LDAscore = 4 .77 , FDR adjusted P = 0 .0011 ) andPseudomonadales(LDAscore = 4 .76 , FDR adjusted P = 0 .0106 ) (Supplementary Table 2 ). Seven genera/families, includingFusobacterium,Pyramidobacter,Mogibacteriaceae,Coriobacteriaceae,Anaerotruncus,SlackiaandBacteroidales,showed higher abundance at on-tumor and adjacent-tumor sites (but not off-tumor sites of patients with CRC recurrence than those without CRC recurrence and healthy controls (Supplementary Table 2 ). Four genera, includingDialister,Selenomonas, TG5 andSchwartzia, showed higher abundance at on-tumor,adjacent-tumor and off-tumor sites of patients with CRC recurrence than those without CRC recurrence and healthy controls (Supplementary Table 2 ). By contrast, some well-recognized CRC drivers,e.g.,PeptostreptococcusandStreptococcus, showed lower abundance at on-tumor sites of patients with CRC recurrence than those without CRC recurrence. These CRC-recurrence-associated genera may play roles in interacting with host cells and worsening patient prognosis.

Figure 2 Principal component analysis showed spatial- and recurrence-specific patterns of microbiota profiles. health: Healthy control; nn: Offtumor site of patient without colorectal cancer (CRC) recurrence; nr: Off-tumor site of patient with CRC recurrence; pn: Adjacent-tumor site of patient without CRC recurrence; pr: Adjacent-tumor site of patient with CRC recurrence; tn: On-tumor site of patient without CRC recurrence; tr: On-tumor site of patient with CRC recurrence.

Figure 3 Patterns of bacterial taxonomy at the phylum level collected from spatial-specific sites of patients with or without colorectal cancer recurrence. health: Healthy control; nn: Off-tumor site of patient without colorectal cancer (CRC) recurrence; nr: Off-tumor site of patient with CRC recurrence; pn: Adjacent-tumor site of patient without CRC recurrence; pr: Adjacent-tumor site of patient with CRC recurrence; tn: On-tumor site of patient without CRC recurrence; tr: On-tumor site of patient with CRC recurrence.

Figure 4 Linear discriminant analysis effect size analysis showed the genera or families with unknown genus with significant differential abundances at off-tumor, adjacent-tumor or on-tumor sites of patients with and without colorectal cancer recurrence. The colors in the heatmap represent the abundance of genera/families with unknown genus. Red: High abundance; Blue: low abundance. health: Healthy control; nn: Off-tumor site of patient without colorectal cancer (CRC) recurrence; nr: Off-tumor site of patient with CRC recurrence; pn: Adjacent-tumor site of patient without CRC recurrence; pr:Adjacent-tumor site of patient with CRC recurrence; tn: On-tumor site of patient without CRC recurrence; tr: On-tumor site of patient with CRC recurrence; LDA: The linear discriminant analysis.

Gut mucosal microbiota profiles associated with prognosis and survival of CRC patients

Next, we selected those genera/families that were significantly associated with CRC recurrence based on LDA effect size analysis and used their abundance to evaluate their effects on prognosis and patient survival. The Kaplan-Meier survival analysis curves showed that seven bacterial genera at on-tumor sites and nine bacterial genera at adjacent-tumor sites were capable of significantly predicting the OS of patients (P< 0 .05 ) (Figure 5 ). High abundance ofAnaerotruncus,Bacteroidales,Fusobacterium,Pyramidobacter,Pseudoramibacter_Eubacteriumand TG5 at on-tumor sites predicted shorter OS, whereas high abundance ofParvimonaswas associated with longer OS (Figure 5 A). At adjacent-tumor sites, high abundance ofAnaerotruncus,Coriobacteriaceae,Dialister,Filifactor,Mogibacteriazeae,PyramidobacterandTreponemapredicted shorter OS, whereas high abundance ofHaemophilusandBacteroidalesindicated longer OS (Figure 5 B). The cutoff values were shown in Supplementary Table 3 .

We next performed Kaplan-Meier survival analyses to analyze DFS between patients with high and low abundance of specific bacterial taxa. A total of eleven genera at on-tumor sites and eight genera at adjacent-tumor sites were capable of predicting DFS obviously (P< 0 .05 ) (Figure 6 ). High abundance ofAnaerotruncus,Bacteroidales,Erysipelotrichaceae_Eubacterium,Filifactor,Mogibacteriazeae,Pyramidobacter,Pseudoramibacter_Eubacterium,Porphyromonadaceae,Slackiaand TG5 at on-tumor sites were associated with shorter DFS, whereas high abundance ofGemellawas associated with longer DFS (Figure 6 A). At the adjacent-tumor sites, high abundance ofAnaerotruncus,Coriobacteriaceae,Dialister,Filifactor,PyramidobacterandSchwartziashowed shorter DFS, while high abundance ofHaemophilusandBacteroidaleswere associated with longer DFS (Figure 6 B).

According to the abundance cutoff value of each genus calculated by Kaplan-Meier survival analyses(Supplementary Table 3 ), we divided the patients into two groups with high or low abundance of each genus. Then, we investigated the survival risk associated with the abundance of each genus/family and other clinicopathological featuresviaunivariate and multivariate COX regression analyses. According to the univariate Cox regression analysis results, we chose bacterium or clinicopathological feature with significance (P< 0 .1 ) and additional bacterium with significance in Kaplan-Meier analysis (P < 0 .05 ) to further perform multivariate Cox regression analysis.

Ιnterestingly, although gender, age, differentiation, smoking and drinking histories showed no significance (P> 0 .05 ) in univariate DFS or OS Cox regression analyses (Supplementary Tables 4 and 5 ),the TNM stage and location of tumor in intestine showed significant influences on patient survival based on multivariate OS Cox regression analysis (P< 0 .05 ) (Supplementary Figures 1 and 2 ). CRC ΙΙΙ/ΙV stage and CRC located in the right colon revealed shorter OS than CRC Ι/ΙΙ stage and CRC located in the left colon or rectum, respectively. Moreover, only CRC ΙΙΙ/ΙV stage showed shorter DFS than CRC Ι/ΙΙ stage (Supplementary Figure 2 ). Ιn addition, MSΙ was associated with improved DFS rates in all patients based on multivariate Cox regression analysis (Supplementary Figure 3 ). Univariate Cox regression OS analysis indicated patients with high abundance ofAnaerotruncus,Bacteroidales,Pyramidobacter,Pseudoramibacter_Eubacteriumand TG5 at on-tumor sites were associated with shorter OS rates (Supplementary Figure 1 ). However, no significant differences were found between these bacteria and OS in multivariate analysis (Supplementary Figure 1 ). At adjacent-tumor sites, univariate analysis showed high abundance ofAnaerotruncus,Coriobacteriaceae,Dialister,Filifactor,Mogibacteriazeae,PyramidobacterandTreponemaand low abundance ofBacteroidaleswere associated with shorter OS rates.Ιn multivariate analysis, high abundance ofAnaerotruncusand low abundance ofHaemophiluswere associated with shorter OS rates (Supplementary Figure 2 ).

High abundance ofAnaerotruncus,Bacteroidales,Erysipelotrichaceae_Eubacterium,Mogibacteriazeae,PyramidobacterandPseudoramibacter_Eubacteriumat on-tumor sites predicted shorter DFS rates in univariate analysis, whereas high abundance ofMogibacteriazeaeandSlackiawere associated with shorter DFS rates in multivariate analysis (Supplementary Figure 3 ). Ιn univariate analysis of bacterial taxa at adjacent-tumor sites, high abundance ofAnaerotruncus, Coriobacteriaceae,Dialister,Filifactor,PyramidobacterandSchwartziaindicated shorter DFS rates (Supplementary Figure 4 ). Meanwhile, low abundance ofBacteroidaleswas associated with shorter DFS rates (Supplementary Figure 4 ). Ιn multivariate analysis, there was no correlation between these bacteria and DFS rates (Supplementary Figure 4 ).

DISCUSSION

Emerging evidence indicates that the gut microbiota plays pivotal roles in CRC incidence and progression[21 ]. Most previous studies have focused on identifying gut microbiota profiles linked to CRC carcinogenesis and revealing the physiological roles of specific species,e.g.,F. nucleatum,Peptostreptococcus anaerobius,B. fragilisandEubacterium rectale, in CRC tumorigenesis and development[22 -25 ]. However, few reports have fully screened the gut microbiota profiles linked to prognosis and survival of CRC patients[7 ]. Up to date, onlyF. nucleatumandB. fragiliswere evaluated for their impacts on patient prognosis[7 ,8 ,13 ,14 ]. Therefore, our understanding of bacterial taxa associated with clinical outcomes of CRC is incomplete. Profiling these bacterial taxa will pave a way for further understanding their functional roles in impairing clinical outcome of CRC and development of novel strategies for prevention of CRC recurrence. Ιn this study, we explored large-scale screening of gut mucosal microbiota of triplet-paired biopsy samples collected from on-tumor, adjacent-tumor and off-tumor sites of CRC patients and identified critical bacterial taxa that were linked to prognosis and survival of CRC patients.

Our data revealed that a number of bacterial genera/families at on-tumor and adjacent-tumor sites are capable of influencing DFS and OS rates. High abundance ofAnaerotruncusandPyramidobacterindicated shorter DFS and OS rates in Kaplan-Meier survival analyses and increased the risk of CRC recurrence and patient death according to our Cox regression analyses (P< 0 .05 ). High abundance ofCoriobacteriaceae,DialisterandFilifactorat adjacent-tumor sites and high abundance ofBacteroidales,Pseudoramibacter_Eubacteriumand TG5 at on-tumor sites indicated shorter DFS and OS rates and increased the risk of CRC recurrence and patient death (P< 0 .05 ). Conversely, high abundance ofParvimonasat on-tumor sites showed longer OS rates. Meanwhile, high abundances ofBacteroidalesandHaemophilusat adjacent-tumor sites indicated longer DFS and OS rates, but onlyHaemophilusdecreased the risk of death in multivariate Cox regression analysis (P< 0 .05 ). High abundances ofFusobacteriumat on-tumor sites andTreponemaat adjacent-tumor sites indicated shorter OS rates, but onlyTreponemaincreased the risk of death (P< 0 .05 ). High abundance ofErysipelotrichaceae_Eubacterium,Gemella,PorphyromonadaceaeandSlackiaat on-tumor sites andCoriobacteriaceaeat adjacent-tumor sites indicated shorter DFS rates, andErysipelotrichaceae_Eubacterium,Gemella,SlackiaandSchwartziaincreased the risk of recurrence (P< 0 .05 ). Ιn multivariate regression analysis,Haemophilusshowed a protective effect andAnaerotruncusshowed a detrimental effect when referred to death (P< 0 .05 ), andMogibacteriazeaeandSlackiashowed obvious detrimental effects when referred to recurrence (P< 0 .05 ).

As well-recognized oral pathogens,F. nucleatum,Parvimonas micraandGemella morbillorumwere significantly enriched in both right- and left-sided CRC tumors[26 ].F. nucleatumin tumor samples was reported to be associated with worse outcomes in terms of OS, DFS or cancer-specific survival, with hazard ratios ranging from 1 .58 to 19 .96 [27 ]. However, our data showed that the abundance ofF.nucleatumonly affected OS but not DFS rates. This observation is consistent with two previous studies.Weiet al[7 ] reported that high abundance ofF. nucleatumorB. fragiliswas associated with poor OS rates after surgery. A meta-analysis found that enrichment ofF. nucleatumin tumor tissue was associated with worse OS among CRC patients (n= 5 studies, HR = 1 .87 ; 95 %CΙ: 1 .12 –3 .11 ; I2 = 60 .6 %) but was not associated with DFS (n= 3 studies, HR = 1 .48 ; 95 %CΙ: 0 .84 –2 .59 ; I2 = 88 .5 %)[28 ].

F. nucleatummay contribute to CRC progression in an established tumor microenvironment due to its highly adherent, invasive and proinflammatory nature that can take advantage of a compromised colonic epithelial cell layer. Moreover,F. nucleatumis an asaccharolytic bacterium that will not compete for glucose, a preferred substrate in tumor metabolism, andF. nucleatumcan tolerate the hypoxic tumor environment[26 ,29 ]. Ιn addition,F. nucleatumis capable of functioning as a bridge-forming bacterium to interact with other bacterial colonizers, leading to a complex biofilm formation in the human body[30 ,31 ]. The increases inF. nucleatumabundance were observed in both biopsy site and saliva samples of CRC[32 ].

Figure 6 The relationship between bacterial abundance and disease-free survival. A: Kaplan-Meier curves of bacteria at on-tumor site and diseasefree survival (DFS); B: Kaplan-Meier curves of bacteria at adjacent-tumor site and DFS. aP < 0 .05 ; bP < 0 .01 ; cP < 0 .001 ; dP < 0 .0001 .

Flynnet al[33 ] proposed a polymicrobial synergy model that certain oral pathogens may cooperate to fight off the host immune system for survival and be able to establish a niche containing mixed species in the gut. The intestinal mucosa and epithelium are falling off and replaced constantly, which provide available nutrients and binding sites for adhesive bacteria. Ιntestinal and oral environments share similar pH, which is conducive for bacteria to form biofilm and persist in the host. Ιnitiation or progression of tumorigenesis benefit these bacteria for proliferation because local inflammatory responses during tumorigenesis increase available nutrients in the niche[33 ]. Polymicrobial colonization at the tumor site by bacterial species that are phylogenetically related to those classified as oral pathogens (e.g.,Fusobacterium,AnaerococcusandParvimonas) could promote tumorigenesis by modifying the tumor microenvironment and eliciting an elevated response of T helper 17 cells, which is linked to a poor prognosis of CRC patients[34 ].

The orderBacteroidalescontains more than 35 species, including the best studied genusBacteroides,which is highly abundant in gut microbiota of a healthy human[35 -39 ]. Due to its high density, it is proposed that the species in this order may form mutualistic relationships with the host gut and play a role in stabilizing the compositional structure of the gut microbiota. However, certain species from this order are pathogenic and considered as potential driver bacteria for CRC. For example, ETBF secretes a zinc metalloprotease toxin, known asB. fragilistoxin, that is associated with inflammatory bowel disease and CRC[40 ]. ETBF can induce production of reactive oxygen species in host cells that cause oxidative DNA damage, induce inflammation and disrupt the integrity of the epithelial barrier. Ιn addition, ETBF is able to activate the β-catenin nuclear signaling cascade and induce proliferation of host cells[41 ].AlthoughB. fragilismay enhance the efficiency of immune checkpoint inhibitor therapy[42 ], ETBF has been reported to decrease OS and DFS of CRC patients[27 ,42 ].

Unexpectedly, our data showed thatBacteroidesat on-tumor and adjacent-tumor sites displayed distinguishable effects on OS and DFS (Figures 5 and 6 ). High abundance ofBacteroidesat on-tumor sites manifested worse OS and DFS, whereas those at adjacent-tumor sites showed better OS and DFS. Ιt was reported that high levels of defined chemokines (e.g., CCL5 and CCL17 ) in CRC tissues may attract beneficial T cells [cytotoxic T lymphocytes, T-helper (Th) 1 cells, interleukin-17 -producing Th cells and regulatory T cells] and lead to improved patient survival. Titers ofBacteroidaleswere positively correlated with expression levels of individual chemokines and the extent of T cell infiltration[43 ].LoadingBacteroidalesto tumor xenografts recruited T cells, indicating thatBacteroidalesis capable of controlling the extent of tumor infiltration by beneficial immune cells[43 ]. However, CRC tissue was infiltrated by more “not effector” T cells (Th2 /Th0 /regulatory T cells/Tnull) with regulatory or anergic properties, which are unable to kill CRC cells and may contribute to CRC promotion[44 ]. Therefore,Bacteroidalesat off-tumor sites here may play a protective role in recruiting beneficial T cells (e.g., Th1 ,Th17 ,etc), leading to improved prognosis of CRC patients. On the other hand,Bacteroidalesat on-tumor sites may contribute to CRC recurrence as pathogens or thrive as passenger bacteria.

Ιn our Kaplan-Meier survival analyses, high abundance ofAnaerotruncusat either on-tumor sites or adjacent-tumor sites was associated with shorter OS and DFS, suggesting that the genus increases the risk of CRC recurrence and patient death. The genusAnaerotruncuscontains only one validly published species, namelyAnaerotruncus colihominis.Anaerotruncus colihominiswas first identified as a Grampositive, anaerobic bacillus that was isolated from the stool specimens of two children[45 ]. Moreover,this species was isolated from the blood culture of humans with nosocomial bacteremia[45 ]. Significant enrichment ofAnaerotruncuswas found in the endometrium of patients with endometrial cancer,suggesting that this bacterium promotes inflammation and tumorigenesis[46 ]. High fat diets are generally considered as a high risk factor for CRC. Abundance ofAnaerotruncusis considered to be linked to consumption of saturated fatty acids in both men and women[47 ]. Ιn mouse model experiments, high fat diets and high sucrose diets led to conditional pathogenic bacterial growth, such asAnaerotruncusandBacteroides. These bacteria played a proinflammatory role in disrupting the integrity of epithelial barrier function[48 -50 ].

Several genera, includingPyramidobacterandMogibacteriaceae, are sulfidogenic and associated with CRC[51 -55 ].Pyramidobacteris mainly isolated from the human oral cavity, upper gastrointestinal tract and bile[56 ,57 ]. The genusPyramidobactercontains anaerobic, Gram-negative bacilli that produce acetic,isovaleric acids and many other trace chemicals as metabolism products[51 ]. Abundance ofPyramidobacterwas found to be higher in older adults and was positively correlated with proinflammatory cytokine interleukin-6 that promotes CRC development[58 ]. Ιn addition, the familyMogibacteriaceaewas reported to be associated with CRC and observed to co-occur withF. nucleatum[53 ,59 ]. Our previous study also reported thatMogibacteriumfrom the familyMogibacteriaceaewas associated withPeptostreptococcusin gut microbiota isolated from CRC patients[60 ].

Several genera identified in this study were reported to be associated with CRC previously. The role ofEubacteriumin CRC initiation was underestimated for a long time. Recently, we identifiedEubacteriumas a potential driver bacteria contributing to CRC and experimentally showed that the lipopolysaccharide ofEubacterium rectaleactivates the transcription factor NF-кB, which regulates innate and adaptive immune responses in normal colon epithelial cells[22 ]. The genusDialisterwas detected in the blood of patients with oral infections that cause bacteremia[61 ]. A meta-analysis based on 26 studies that used next-generation sequencing to analyze microbiota showed that the relative abundance ofDialisterwas significantly higher in cancer patients than those in control samples[62 ]. The metabolism end products ofDialisterinclude acetate, lactate and propionate that may cause carcinogenesis[62 ].Treponema denticolais an oral pathogen and associated with an increased risk of CRC[63 ]. The genusSchwartziais linked to CRC carcinogenesis-related gene methylation[64 ]. The familyCoriobacteriaceae is considered a commensal or probiotic bacteria residing in the human gut[65 ]. Their roles in driving CRC recurrence are unknown.

Unlike other critical genera analyzed in this study, low abundance ofHaemophilusat adjacent-tumor sites indicated longer OS and DFS than those with high abundance in our Kaplan-Meier analyses.Haemophilusis a commensal microorganism, which belongs to the phylumProteobacteria. Ιt is an opportunistic pathogen that may lead to infections such as endocarditis and pneumonia.Haemophilusin stool samples showed significantly higher proportions in the CRC group than in the control group[66 ].The proportions ofHaemophilusdecreased after tumor removalviasurgery, indicating it is a carcinogenesis pathogen indirectly[67 ]. However, decreased abundance ofHaemophiluswas observed in stage Ι/ΙΙ CRC compared to stage 0 (earliest) CRC, which may be due to overgrowth of other harmful bacteria that acted as competitors during the transition from precancerous lesions to late-stage CRC[68 ].

According to our COX regression analysis, location (right/left colon or rectum) is another risk factor for patient death. Compared to left colon or rectum, right colon obviously increased risk of death.Consistent with our results, a study showed that the 10 -year OS of patients with CRC at the right-sided colon was shorter than that of patients with CRC at the left-sided colon[68 ]. There is a more abundant blood supply in the right-sided colon than other parts of colon, which benefits tumor growth and results in common clinical symptoms including anemia, emaciation, fever and dyscrasia. Tight-sided CRC exhibits more mucinous and advanced TNM stage[69 ]. Obviously different patterns of microbiota structures and abundances were found between left-sided and right-sided colons of CRC patients[69 ].Moreover, invasive bacterial biofilms were found in 89 % of right-sided CRC cases but in only 12 % of left-sided CRC cases[69 ]. Therefore, right-sided CRC specific bacterial species with concomitant procarcinogenic epithelial responses may contribute to the development of right-sided CRC[70 ].

We further identified that TNM stage showed an obvious impact on survival of CRC patients.Patients with stage ΙΙΙ/ΙV CRC had a higher risk of death and disease recurrence, which is consistent with previously reported results[71 ]. At the same time, microsatellite status was another factor that influenced patient survival in our study. MSΙ may decrease the risk of CRC recurrence compared to microsatellite stable patients. Moreover, it was reported that MSΙ shows stage-specific impacts on the prognosis of CRC patients[70 ]. Ιn stages ΙΙ and ΙΙΙ CRC, high MSΙ tumors had superior prognosis compared with high microsatellite stable tumors. Ιn stage ΙV CRC, although 4 % of tumors were identified as high MSΙ tumors, these tumors were recognized to be associated with inferior survival[70 ].Sequencing paired colon tumor and normal-adjacent tissue and mucosa samples revealed significant enrichment ofB. fragilisandF. nucleatumin deficient mismatch repair CRC but not in proficient mismatch repair CRC[72 ].

CONCLUSION

Ιn this work, we identified critical bacterial taxa that are associated with prognosis and survival of CRC patients. Our work suggests that intestinal microbiota can serve as biomarkers to predict the risk of CRC recurrence and patient death. Unexpectedly, most of these identified genera have not been investigated for their physiological roles in interacting with host intestinal cells. On the other hand, some wellrecognized CRC drivers,e.g.,PeptostreptococcusandStreptococcus, are not associated with CRC recurrence according to our observations. Thus, the mechanism behind bacteria-driving CRC recurrence may be different from those proposed for bacteria-driving CRC development. The activities of complex immune cells,e.g., various types of T cells (e.g., Th1 , Th2 and Th17 ) and macrophages, in response to these bacterial activities may need to be considered. Further functional analyses of physiological roles of these bacteria in patient prognosis and CRC recurrence will shed light on developing novel strategies for CRC treatment and prevention.

ARTICLE HIGHLIGHTS

FOOTNOTES

Author contributions:Wan XH contributed to the conception of the study; Huo RX and Wang YJ contributed significantly to follow-up, analysis and manuscript preparation; Huo RX, Hou SB and Wan XH performed the data analyses and wrote the manuscript; Wang W and Zhang CZ helped perform the analysis with constructive discussions; Zhang CZ collected the samples; All authors have read and approve the final manuscript.

Supported byTianjin Science and Technology Plan Project, No. 19 YFZCSY00170 ; Tianjin Union Medical Center, No.2019 YJ007 ; Beijing Medical and Health Foundation, No. F1814 B; Key R&D Projects in the Tianjin Science and Technology Pillar Program, No. 19 YFZCSY00420 ; National Key R&D Program of China, No. 2017 YFC1700606 and 2017 YFC1700604 .

Institutional review board statement:The study was reviewed and approved by the Tianjin Union Medical Center Ιnstitutional Review Board (Approval No. B31 ).

Conflict-of-interest statement:The authors declare that there is no conflict of interest.

Data sharing statement:Technical appendix, statistical code, and dataset available from the corresponding author at xuehua.wan@nankai.edu.cn.

Open-Access:This article is an open-access article that was selected by an in-house editor and fully peer-reviewed by external reviewers. Ιt is distributed in accordance with the Creative Commons Attribution NonCommercial (CC BYNC 4 .0 ) license, which permits others to distribute, remix, adapt, build upon this work non-commercially, and license their derivative works on different terms, provided the original work is properly cited and the use is noncommercial. See: https://creativecommons.org/Licenses/by-nc/4 .0 /

Country/Territory of origin:China

ORCID number:Rui-Xue Huo 0000 -0001 -5755 -4934 ; Yi-Jia Wang 0000 -0002 -4026 -9245 ; Shao-Bin Hou 0000 -0003 -3467 -8242 ; Wei Wang 0000 -0002 -6660 -8540 ; Chun-Ze Zhang 0000 -0002 -2063 -5631 ; Xue-Hua Wan 0000 -0002 -6367 -848 X.

S-Editor:Zhang H

L-Editor:Filipodia

P-Editor:Wu RR