Articulo 4
Articulo 4
Articulo 4
Abstract
Introduction. The oral cavity is one of the largest reservoirs of microorganisms and many pathogenic bacteria have been shown
to be associated with the aetiology of oral cancers.
Gap Statement. Owing to the complexity of oral microbial communities and their unclear relationship with oral cancer, identi-
fication of specific bacteria which contribute to oral cancer is a key imperative.
Aim. To compare and investigate the variations in the composition of the bacterial microbiome and its functions between
patients with oral tumorous lesions and healthy subjects.
Methodology. Twenty-seven samples from individuals with oral tumours (five oral benign tumours and 22 oral squamous cell
carcinomas) and 15 samples from healthy subjects were collected. Genomic DNA was extracted and the V3–V5 region of the
16S rRNA gene was sequenced. Subsequently, bioinformatic assessment was conducted using QIIME2, PICRUSt and linear
discriminant analysis effect size analyses (LEfSe).
Results. The oral microbiota was composed mainly of the phyla Proteobacteria (31.76 %, 35.00 %), Bacteroidetes (30.13 %,
25.13 %) and Firmicutes (23.92 %, 17.07 %) in tumorous and healthy individuals, respectively. Neisseria, Prevotella, Fusobacterium,
Streptococcus, Capnocytophaga, Veillonella, Haemophilus, Prevotella, Porphyromonas and Leptotrichia were the most abundant
genera. Alpha diversity in the tumour group was significantly greater than that in the healthy group (P<0.05). Differential analy-
sis of microbes between groups demonstrated a significantly higher number of Neisseria, Veillonella, Streptococcus, Leptotri-
chia, Lautropia, Sphingopyxis, Sphingobium, Tannerella, Actinomyces and Rothia in healthy controls compared with the tumour
group. However, the genera Treponema, Micrococcus, Pseudomonas, Janthinobacterium, Parvimos, Loktanella, Staphylococcus,
Acinetobacter, Catonella, Aggregatibacter and Propionibacterium were significantly higher in the tumour group. Pathways related
to cancers, cell motility, environmental adaptation, metabolism and signal transduction were enhanced in the tumour group,
while functions associated with immune system diseases, replication, repair and translation were significantly enhanced in the
healthy group.
Conclusion. Variations in the oral microbiota and its functions showed a correlation with oral tumours. The tumour group
showed an increased abundance of some multi-drug-resistant and periodontitis-related pathogens. The significantly altered
microbiotas may serve as potential biomarkers or inform combination therapy for oral tumours.
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Introduction
Head and neck cancers are among the most common cancers worldwide [1], accounting for approximately 5 % of all tumours
[2]. Approximately half of all head and neck cancers occur in the oral cavity [2]. An estimated 354864 newly diagnosed cases of
lip and oral cavity cancers were reported in 2018, and these sites ranked 18th among the most commonly encountered cancer
sites [1]. In the USA, oral cancer was regarded as the sixth most common cause of cancer-related mortality [2] and 52260 new
cases of oropharyngeal cancers were diagnosed in 2020 [3]. Oral squamous cell carcinomas (OSCCs) are considered to be the
most common malignant oral tumours [1]. The financial cost for managing oral cancer is considered to be the highest among
all cancers [4]. In addition, oral carcinoma has a high prevalence in Southern Asia, because of widespread use of tobacco-related
products in this region [5]. In 2015, an estimated 51765 newly diagnosed cases of oral or oropharyngeal cancers were reported
in China, and 23830 deaths were attributable to oral cancer [6].
In-depth characterization of the causes of oral cancer can help inform preventive interventions. Chronic use of alcohol, tobacco
and betel quid chewing are the most important risk factors for oral cancer [7–9]. However, in a recent study by Bai et al., smoking
and alcohol consumption were not found to be prognostic factors for oral cancer [10], which suggested the possibility of addi-
tional aetiological factors for oral tumours. In the 1990s, Helicobacter pylori was identified as the main causative agent for the
development of gastric cancer [11]. Subsequent research revealed an association of human cancers with certain viruses, bacteria
and parasites, and several microbes were identified as strong risk factors for specific types of cancers [12–14]. The oral cavity
is considered as one of the largest reservoirs of different types of microorganisms, including different species of bacteria, fungi
and viruses [15]. Studies have suggested an aetiological role of many pathogenic bacteria in the causation of oral cancers [16].
Porphyromonas gingivalis and Fusobacteria species were more prevalent on the surface of OSCCs [17]. Al-hebshi et al. suggested
a close association of Fusobacterium nucleatum and Pseudomonas aeruginosa with OSSC [18]. In addition, Chen et al. unravelled
the variations in the composition of the salivary microbiome between patients with OSCC and oral submucosa fibrosis (OSMF)
and further found considerable reduction in species and phylogenetic diversity in OSMF patients compared with those with OSCC
[19]. Recently, Yang et al. found a close association of the oral microbiota community dynamics with OSCC stage; in addition,
microbiota communities in OSCC patients from stage 4 showed significantly greater complexity compared to that from healthy
controls [16]. Moreover, they found a significant increase in the abundance of Fusobacteria with the progression of oral cancer;
however, the abundance of Streptococcus, Haemophilus, Porphyromonas and Actinomyces decreased with the progression of oral
cancer [16]. In another study, the abundances of Bacillus, Enterococcus, Parvimonas, Peptostreptococcus and Slackia were different
between patients with premalignant lesions and OSCC [20]. Schmidt et al. found significant overrepresentation of Streptococcus
and Rothia at cancer lesion sites compared with the contralateral part of the anatomical site containing normal tissues in patients
with oral cancer [21]; however, other studies found no association between the presence of individual subgingival pathogens and
risk of cancer [22]. Owing to the complexity of oral microbial communities and the conflicting results of their relationship with
oral cancer, identification of specific bacteria that contribute to oral cancer is a key imperative.
A wide range of technologies have been adopted by researchers to assess the correlation of various microbiota with oral cancer,
such as pan-pathogen array [23], quantitative PCR [24], immunological staining [25], antibody detection [26] and fluorescence
in situ hybridization [27]. However, these methods either depend on bacterial culture or have low throughput. Of note, the vast
majority of the microbiota cannot be cultured [28]; therefore, these methods cannot elaborate on the profiles of the oral microbiota.
High-throughput sequencing technology, which is independent of culture, can identify thousands of microorganisms by partial
sequencing of the 16S rRNA gene.
To date, there is limited literature on the microbial variations between oral cancerous and healthy subjects. Therefore, in this
study, we aimed to compare the characteristics of oral microbiotas between patients with oral tumours and healthy subjects.
In addition, we compared the variations in the microbiome and its functions in patients with oral tumours (including benign
tumours and OSCCs) and in healthy subjects by high-throughput sequencing technology.
Methods
Tumour diagnosis was confirmed by histopathology. Patients who were diagnosed with oral cancer for the first time and had no
previous history of any type of tumour were included in the study. Patients who received antibiotics for ≥2 weeks before this study
were excluded from the study group. Healthy control samples were carefully examined clinically and specialized examination
was carried out to exclude the presence of any lesion; healthy controls had no history of other oral mucosal diseases or severe
systemic disorders. Based on a well-defined clinical protocol, patients with a history of betel chewing, diabetes mellitus or other
systemic complications, such as heart or liver failure, were excluded from this study.
Written informed consent was obtained from all participants. All experiments were performed according to the approved guide-
lines and regulations of this institution.
The surface of benign tumour tissues, OSCC tissues and identical tissues from healthy subjects were sampled using two identical
sterile swabs. Disposable sterile nylon flocking swabs were used (cy-98000; Hua Chen Yang) and then stored in oral swab
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Fig. 1. Rarefaction curves and boxplots of α-diversity in the healthy and tumorous groups. The healthy controls had no history of other oral mucosal
diseases or severe systemic disorders; the tumours from the patients were confirmed by histopathology. Observed species, Shannon indices and
Faith’s PD diversity were calculated using QIIME2, and then plotted using ggplot2. The plateau rarefaction curves indicated that the quenching depth
covered the maximum of the diversity per sample. The index of phylogenetic diversity (P<0.001, Mann–Whitney U test) and observed species (P=0.001,
Mann–Whitney U test) indicated that the diversity of the bacterial communities in the tumorous group was significantly greater than that in the
healthy control group. The Shannon index showed higher bacterial communities in tumorous subjects compared with healthy individuals; however, the
difference was not statistically significant (P>0.1, Mann–Whitney U test).
preservation solution (Tris, EDTA and antiseptic) to prevent DNA degradation. Sterile swabs without sampling were used as
controls. All samples were stored at 4 °C and transferred to an ultra-low-temperature freezer (–80 °C) until processing.
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Fig. 2. The most abundant phyla between tumorous and healthy control samples. The healthy controls had no history of other oral mucosal diseases
or severe systemic disorders; the tumours from the patients were confirmed by histopathology. A total of 32 phyla were identified in the two groups.
Among these, 10 were discovered in healthy subjects and 32 were discovered in patients with tumours. In this plot, only the five most abundant phyla
are shown, and the rest are classified as others.
Results
Sampling and sequencing
The details of the 42 swabs collected, which included 27 swabs from tumorous patients and 15 from healthy controls, are presented
in Table S1 (available in the online version of this article). There were no significant between-group differences with respect
to age (51.41±15.37 versus 46.07±11.09 years, t=1.2975, P=0.2025, t-test) or sex [Chi-squared test (χ2)=0.0021605, P=0.9629].
After genomic DNA extraction and sequencing, 1853614 paired reads were obtained. Following quality control and filtration
with the DADA2 pipeline, 519 545 reads were produced with an average of 12370 reads per sample. A total of 1901 features were
identified in the samples (Table S2). No nucleotides were detected in controls. All sequencing results were submitted to NCBI
with numbers SRR14583850–SRR14583891.
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Fig. 3. Heatmap and hierarchical clustering of the top 30 genera in all samples. The dendrogram was created based on the Euclidean distance
and Ward distance. D2 clustering methods were performed in heatmap packages in R software. The genera Neisseria, Prevotella, Fusobacterium,
Streptococcus, Capnocytophaga, Veillonella, Haemophilus, Porphyromonas, Leptotrichia and Aggregatibacter were the most abundant in all the groups.
Hierarchical clustering suggested that the samples from the tumorous group were clustered differently from those collected from the healthy controls.
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Fig. 4. Principal component analysis (PCoA) at the ASV level. PCoA was conducted using QIIME2, then plotted in R software using ggplot2. The ellipse
was plotted with a confidence level of 0.95. The spots that represent the tumorous samples show a more dispersed distribution pattern than those
from the healthy controls. Samples from the tumorous group were significantly different from those in the control group (PERMANOVA, pseudo-
F=5.756921, P=0.001).
Neisseria was the most dominant genus in the healthy control group, and accounted for 21.23 %, followed by Prevotella (17.57 %),
Streptococcus (9.74 %), Veillonella (9.09 %) and Fusobacterium (6.70 %). However, in the tumorous group, the most abundant genera
were Prevotella (11.02 %), Fusobacterium (9.02 %), Capnocytophaga (6.62 %), Neisseria (5.42 %) and Haemophilus (4.93 %) (Fig. 3).
Of interest, the top 10 genera in the control group accounted for 84.77 %, while the corresponding percentage in the tumorous
group was significantly lower (55.08 %). The top 30 genera decreased dramatically from 98.43 to 78.56 %. This indicated that the
microbiota in the tumorous group was more evenly distributed compared with that in the healthy control group.
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Fig. 5. Distinct taxa identified between two groups using linear discriminant analysis effect size analyses (LEfSe). The results of linear discriminate
analysis (LDA) showed that the bacteria were significantly different between the tumorous and healthy control samples: (a) Cladogram indicating the
phylogenetic distribution of bacteria that were significantly increased; and (b) LDA scores showing significant bacterial differences between groups
at the genus level. The genera Neisseria, Veillonella, Streptococcus, Leptotrichia, Lautropia, Sphingopyxis, Sphingobium, Tranerella, Actinomyces and
Rothia were significantly higher in the healthy control group, whereas Treponema, Micrococcus, Pseudomonas, Janthinobacterium, Parvimos, Loktanella,
Staphylococcus, Acinetobacter, Catonella, Aggregatibacter and Propionibacterium were significantly higher in the tumorous group.
(corrected P=0.010), cell motility (corrected P=0.009), environmental adaptation (corrected P<0.001), metabolism (corrected
P<0.001) and signal transduction (corrected P<0.011) were significantly enhanced in the tumorous group compared with the
control healthy group. However, the pathways related to immune system diseases (corrected P=0.013), replication and repair
(corrected P=0.021), and translation (corrected P=0.028) were significantly enhanced in the control healthy group (Fig. 6).
On level 3, 27 different pathways were significantly different (Fig. 7). Among these, 17 were more abundant in the tumorous group
and 10 were were more abundant in the control healthy group (t-test, Storey FDR correction, corrected P<0.05). The pathways
that were related to MAPK signalling, two-component system, bacterial chemotaxis, flagellar assembly, sulphur relay systems
and cell motility were significantly increased in the tumorous group compared with the healthy control group. However, the
samples from the control group had more genes related to lysine biosynthesis and aromatic amino acids (phenylalanine, tyrosine
and tryptophan) biosynthesis.
Discussion
There are approximately 1000 species that are capable of achieving stable colonization in the oral cavity [35]. The oral microflora
is regarded as the second most complex microbiota in humans [36]. The development of high-throughput DNA sequencing
technology at the molecular genetics level has facilitated in-depth characterization of the most important aspects of the oral
microbiota. In addition, it has helped identify the oral microbiota associated with oral health and oral cancer [37]. However,
the results pertaining to the relationship between oral health and specific microbiota have been inconsistent, because of diverse
human lineages, such as related to different living conditions, diverse cultural backgrounds and different dietary habits [38]. Use
of different technology [39], diverse types of sample [40, 41] and various methods of sequencing [42] may have contributed to
the inconsistent results. In this study, the surfaces of tumorous lesions and healthy controls were sampled and assessed further.
Oral samples from tumorous and healthy individuals were collected. The V3–V5 region of the 16S rRNA gene was chosen for
sequencing and analysis [43].
Our results indicated greater α-diversity in species in the tumorous group compared with the healthy control group (Fig. 1),
which was consistent with previous studies [40, 44]. In a detailed large-scale assessment of the salivary microbiota conducted by
Yoshihisa et al., the bacterial richness in the salivary microbiota was found to be significantly associated with poor oral health [38].
In general, good oral health was associated with lower diversity in the salivary microbiome [45]. A recent survey of in situ bacterial
effects indicated that patients with a high microbiome diversity had increased tumour infiltration of CD4+ lymphocytes, which
consequently prolongs the management of cancer [46]. Heshiki et al. examined the influence of the microbiome on the treatment
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Fig. 6. The gene functions on level-2 that were significantly increased in different groups. The functions were predicted by PICRUSt with default
settings, then the t-test and Storey FDR correction were conducted using STAMP. The functions connected with cancers (corrected P=0.010), cell
motility (corrected P=0.009), environmental adaptation (corrected P<0.001), metabolism (corrected P<0.001) and signal transduction (corrected
P<0.011) were significantly enhanced in the tumorous group compared with the healthy control group. However, the pathways related to immune
system diseases (corrected P=0.013), replication and repair (corrected P=0.021), and translation (corrected P=0.028) were significantly enhanced in
the healthy control group.
outcomes of eight diverse malignancy types and found that a more diverse intestinal microbiome was associated with improved
systemic and antitumour immunity [47]. Preserving diversity is an important element of the survival of various microbiota [48].
Changes in the oral microenvironment in tumorous patients may contribute to the changes in diversity, which is more likely to
induce a favourable antitumour response. However, some authors reported a significant reduction in microbial diversity in cancer
patients compared with controls [39]. This discrepancy may be attributable to the different ethnic background or lifestyle-related
factors in the study population. The relationship between microbial diversity and oral disease status needs to be identified.
In this study, Proteobacteria, Bacteroidetes, Firmicutes, Fusobacteria and Actinobacteria were the most abundant phyla (Fig. 2).
These results are similar to those of other studies [40]. However, the most abundant bacteria in these phyla by percentage were
not consistent with this study. Proteobacteria was the most abundant phylum detected in our study, while Bacteroidetes was the
most abundant phylum reported by Zhao et al. [40]. Firmicutes was the most abundant phylum reported in another study [21].
Neisseria was the most abundant genus in our study, while Prevotella was the most abundant genus reported in the previous study
[40] (Fig. 3). These differences may be attributable to the different genetic characteristics of the population or the different timing
of sampling; therefore, more accurate standardized inclusion criteria and protocols are required to achieve consistent results.
In our study, Neisseria, Prevotella, Streptococcus, Veillonella, Fusobacterium, Capnocytophaga and Haemophilus were the most
abundant genera; all these have been regarded as the common core oral microbiota in other studies [49]. Neisseria was the most
abundant genus in our healthy control group, while Prevotella was the most abundant in the tumorous group. Yoshihisa et al.
suggested that the predominance of the genus Prevotella in the salivary microbiota could be attributed to severe periodontal
disease, while the predominance of the genus Neisseria indicated healthy periodontal conditions [38]. Similar results were reported
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Fig. 7. The functions on level-3 that were significantly increased in different groups. The functions were predicted by PICRUSt with default settings,
then the t-test and Storey FDR correction were conducted using STAMP. Twenty-seven different pathways were significantly different. Among these,
17 were more abundant in the tumorous group and 10 were were more abundant in the control healthy group (t-test, Storey FDR correction, corrected
P<0.05). The pathways that were related to mitogen-activated protein kinase (MAPK) signalling, two-component system, bacterial chemotaxis, flagellar
assembly, sulphur relay systems and cell motility were significantly increased in the tumorous group compared with the healthy control group.
However, the samples from the control group had more genes related to lysine biosynthesis and aromatic amino acids (phenylalanine, tyrosine and
tryptophan) biosynthesis.
by Rafael et al., who compared the salivary microbiome from oropharyngeal cancer (OPSCC), OCSCC and normal healthy
controls, and found a significant decrease in Neisseria in OPSCC and OCSCC [39]. Zhao et al. suggested that Neisseria may play
an important role in maintaining the stability of the oral bacterial community [40]. In addition, our study found significantly
greater abundance of Streptococcus in the healthy group. Previous studies have suggested that Streptococcus may be beneficial to
the host, because these bacteria may produce molecules that are inhibitory to pathogenic species [50]. Tagaino et al. suggested
that Streptococcus mitis, Streptococcus salivarius and Streptococcus mutans may have the ability to produce acetaldehyde from
ethanol or glucose [51]. Acetaldehyde is a carcinogen and was shown to contribute to sister chromatid exchanges, gene mutations
and DNA-strand breaks [51, 52]. The production of acetaldehyde is affected by the oral microenvironment, such as pH, oxygen
concentration, metabolic substrates and even salivary secretions [51]. Therefore, the production of acetaldehyde in healthy
individuals should be studied in future research.
Of the top 30 genera, Sphingobium was almost only exclusively discovered in healthy individuals. Recent studies have suggested
its potential protective role in breast cancer, because of its ability to metabolize oestrogen [53, 54]. Aggregatibacter was more
abundant in tumorous patients in our study. Aggregatibacter actinomycetemcomitans is one of the key causative pathogens in
chronic periodontitis. In addition, it has been associated with aggressive periodontitis [55]. Long-term chronic periodontal
disease increases the risk of oral cavity cancers, especially OSCC [56]. However, consistent chronic inflammation may not be
the only reason for carcinogenesis, because accumulation of genome instabilities, such as point mutations, deletions, inversions,
duplications, translocations and chromosome loss, is a key factor for carcinogenesis [57]. Teshima et al. discovered that Aggre-
gatibacter actinomycetemcomitans infection can cause breakage in the DNA double-strand in host cells [57], which suggested that
Aggregatibacter actinomycetemcomitans may increase the risk of genome instabilities in host cells and subsequently increase the
risk of carcinogenesis. Leukotoxin (LtxA), which is produced by Aggregatibacter actinomycetemcomitans, can kill neutrophils,
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lymphocytes and monocytes, allowing it to evade host immune surveillance [58]. Therefore, Aggregatibacter actinomycetemcomi-
tans may have a deleterious effect on the human immune system. In addition, it has been shown to be associated with systemic
complications, such as endocarditis, rheumatoid arthritis [59] and lung cancer [60, 61]. Some studies have found an association
between Aggregatibacter actinomycetemcomitans and development of pancreatic cancer and oesophageal cancer [62, 63]. There-
fore, further research is required to reveal its role in the development and progression of oral cancers. In addition, Acinetobacter
baumannii is one of the most common clinical multidrug-resistant bacteria that is frequently isolated in wound infection following
surgical intervention for OSCC [64]. However, our study was conducted before the surgical procedure; therefore, higher numbers
of Acinetobacter baumannii may have existed before surgery, which might have contributed to its commonly reported isolation
following oral cancer surgery. Inhibiting Acinetobacter growth before a surgical procedure could be an effective method to reduce
multidrug-resistant bacterial infection. The abundance of the genus Propionibacterium was significantly greater in the tumour
group compared with that in the healthy control group. Perera et al. discovered that rates were higher in fibroepithelial polyps
(FEPs) compared with OSCCs [65]. It would be of interest to explore the role of Propionibacterium in the aetiology of FEPs or
benign tumours.
PICRUSt and the STAMP method were used to assess the functions of various bacterial communities. Genes related to signal
transduction were upregulated in the tumorous group compared with the healthy controls (Fig. 6). Further analysis suggested
that the genes connected to two-component sensing systems (TCSs) were more abundant in the tumorous group (1.46–1.08 %,
P=0.04, t-test, FDR-corrected). These regulatory systems are ubiquitous signalling units found in prokaryotes, which tailor the
response based on the local conditions. TCSs were shown to mediate bacterial acclimatization to various environmental changes
by coupling environmental signals to gene expression [66]. Upregulation of these systems may promote bacterial survival. The
correlation of MAPK pathway changes with the oral microbiota may inform novel combination therapies for oral tumours.
Of interest, bacterial chemotaxis and flagellar assembly, which are involved in cell motility, were significantly higher in the
tumorous group (Fig. 7). Williams et al. showed that H. pylori mutants with defective chemotaxis induced less inflammation
than the wild-type H. pylori [67]. Wang et al. suggested an important role of bacterial chemotaxis in periodontitis-related
inflammation [68]. Similar results were indicated in other reports [18]. Flagellin was shown to stimulate significant migration
of innate immune cells, such as macrophages, dendritic cells and neutrophils to colonized tumours [69]. The functions of
both genes demonstrate their antitumour ability, and the upregulation of these suggested antitumour immunological effects
of some bacteria in the oral microbiota. In addition, genes correlated with replication and repair were significantly reduced
in tumorous patients. Oral bacterial virulence factors produced by bacteria such as Aggregatibacter actinomycetemcomitans
(which was more abundant in the tumorous group, Fig. 5b) may induce single-strand DNA breakages, produce replication
stress response, and ultimately lead to breakage to double-strands and arrest cell cycle replication [70]. Inefficient repair of
damaged DNA could allow survival of cells with defective DNA, resulting in accumulation of multiple genome instabilities
and promoting tumorigenesis and progression [71]. In addition, the pathways related to immune system disease, replication or
repair, and translation were significantly overrepresented in controls. Lysine biosynthesis was upregulated in healthy controls
(Fig. 7). Because the bacterial biosynthesis of lysine is important in the construction of bacterial peptidoglycan cell walls [72],
the underrepresented lysine biosynthesis genes in tumours indicated that their microenvironment had compromised the
microbiota. Biosynthesis of three aromatic amino acids (phenylalanine, tyrosine and tryptophan) was upregulated in healthy
controls (Fig. 7). These aromatic amino acids are essential for protein synthesis [73], and dysmetabolism of aromatic amino
acids leads to cancers [74].
Some limitations of our study should be considered. First, the small sample size may have reduced the number of significantly
different genera between the tumorous and healthy groups. However, 21 genera were identified, which included some genera
that have been reported by other researchers. Second, consumption of alcohol and tobacco smoking are important aetiological
factors for oral cancers, and therefore these factors are likely to affect the oral microbiota. Because of the small sample size, we
did not discuss their impact. Therefore, large samples and a detailed comprehensive questionnaire survey on living habits might
be required in future studies. Third, we did not assess the variations in the significantly different genera during cancer progres-
sion from early to advanced stages. Further validation of the statistically different genera in various histopathological stages of
dysplastic oral cancer could provide valuable insights.
In conclusion, we observed a correlation between different variations in the oral microbiota and its functions with oral
tumours. The tumorous group exhibited significantly greater diversity, which may indicate poor oral health. The tumorous
group also showed significant overrepresentation of the abundance of some multi-drug-resistant and periodontitis-related
pathogens. The significantly altered microbiota could be explored further as novel biomarkers and may help inform combina-
tion therapies for oral tumours. The results of this study expended our knowledge of oral bacterial communities in patients
with oral tumours.
Funding information
This work was supported by Rapid Pathogen Detections and Infectious Disease Alerts, the Key Medical Discipline in Guangzhou (2021-2023-11); Basic
Research Project of Key Laboratory of Guangzhou (2021BRP004)
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Author contributions
J.Y. and X.W. conceived and designed research; M.Z., J.Z., X.T. and A.W. collected data and conducted research; P.H. and S.L. analysed and interpreted
data; P.H. and J.Y. wrote the initial paper; X.W. and P.H. revised the paper; X.W. had primary responsibility for final content. All authors read and approved
the final manuscript.
Conflicts of interest
The authors declare that they have no conflicts of interest.
Ethical statement
This work was approved by the Research Ethics Committee of the Hospital of Stomatology, Sun Yat-sen University at District of Yuexiu, Guangzhou
City, China.
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