The Emerging Clinical Application of m6A RNA Modification in Inflammatory Bowel Disease and Its Associated Colorectal Cancer.

Methylation, first proposed in DNAs, but later found in RNAs, serves as one of the most widespread epigenetic modifications in eukaryotes, where N6-methyladenosine (m6A) modification has been found to play an important role in a variety of cancers including colorectal cancer (CRC). Under the action of various enzymes and proteins, the regulatory role of m6A in RNAs and immune cells has also been gradually realized. This paper reviews the general biogenesis and effects of m6A, and its emerging crucial role in intestinal mucosal immunity via the regulation of RNAs and immune cells, and thus closely related to the occurrence and development of inflammatory bowel disease (IBD) and CRC. m6A-related genes and regulatory factors are expected to be potential predictive markers and therapeutic targets.

Introduction

IBD is a group of idiopathic chronic inflammatory diseases with abnormal immunity of intestinal mucosa caused by a combination of factors, and mainly include ulcerative colitis (UC) and Crohn’s disease (CD). Due to the abnormal autoimmune function in patients, other organs and tissues may be damaged. In addition, patients with IBD have a higher risk of colon cancer.1 Recent studies have shown that individual genetic susceptibility, environmental influence, intestinal microorganisms, and immune response are all involved and functionally integrated into the pathogenesis of IBD.2,3 Notwithstanding, the specific pathogenesis of IBD is still unclear and its clinical treatment mainly relies on surgery and traditional therapies that are unable to completely relieve the symptoms, and prone to adverse events that affect the quality of life of patients.4 Therefore, the urge to further explore the pathogenesis of IBD and find new alternative therapies is significantly necessitous.

Among the many (over 100) different chemical modifications, m6A has attracted wide attention due to its dynamic regulation and reversible post-transcriptional regulation. Its interaction with a variety of RNAs and signaling pathways makes it play an important role in the development of diseases. Common mRNA methylation modifications include m6A, N1-methyladenosine (m1A), and 5-methylcytosine (m5C). Methylation of adenosine N1 atoms to form 1-methyladenosine (m1A) has been identified at the nucleotide sites 9, 14, 22, 57, and 58 of different tRNAs. In some cases, these modifications have been shown to increase the stability of tRNA structures and induce correct tRNA folding.5 mRNA is locally modified by m5C at the DNA damage sites. The RNA methyltransferase, tRNA aspartic acid methyltransferase 1(tRDMT1), is recruited to the sites of DNA damage to promote m5C induction, suggesting that RNA post-transcriptional modification can also act as DNA damage code to regulate DNA repair.6 m6A was first found in mRNA in 19747 and is the most abundant internal RNA modification in eukaryotic cells, affecting many aspects of RNA metabolism, from RNA processing, nuclear output, RNA translation to degradation. Emerging evidence suggests that m6A methylation plays a key role in embryonic development, circadian rhythm, cell cycle, and tumorigenesis through a variety of mechanisms.8 Besides, m6A methylation provides more possibilities for the early diagnosis and treatment of a variety of cancers, such as gastric, liver, lung, bladder, and colon cancers.9–13

There is increasing evidence that m6A methylation, as an important post-transcriptional gene regulation mechanism, participates in IBD pathogenesis. For example, the deletion of RNA methylation writer methyltransferase like 14(METTL14), an RNA m6A methyltransferase component, in T cells triggers spontaneous colitis in mice, characterized by a Th1/Th17 phenotype. The development of colitis is due to dysfunctional regulatory T cells and is dependent on the gut microbiota.14 A similar study reports that mice with Foxp3-mediated deletion of methyltransferases like 3 (METTL3), an mRNA m6A methylation, in regulatory T cells develop a severe systemic autoimmune response,15 a characteristic of intestinal inflammatory conditions. This paper examines available literature on the major forms of m6A modification, explores their involvement in intestinal mucosal immunity, dendritic cell (DC) and T cell regulation, as well as the evolving clinical significance in IBD and CRC.

m6A RNA Modification

Biogenesis of m6A and Its Regulation of mRNA

m6A is the most abundant internal modification in mRNA and lncRNA in eukaryotes.16 It is a reversible and dynamic methylated modification of adenosine in the sixth N of mRNA.17 It was not until 2012 that the modification map of m6A in the transcriptome (epitope transcriptome) was first mapped with the development of next-generation sequencing technology.18 The modification sites of m6A have a typical recognition sequence – DRACH motif (D stands for G/A/U, R stands for G/A, and H stands for A/C/U), and are enriched in the coding sequence (CDS), 3ʹ untranslated region (3 ‘UTRs) and 5ʹ untranslated region (5ʹ UTRs) of mRNAs,19 especially high m6A modification is common near the stop codon regions. The 3 ‘UTRs bind to many mRNA-binding proteins. The dynamic modification of m6A is mainly performed by three components, “writers”, “erasers” and “readers”. The writers refer to adenosine methyltransferase as the representative, erasers as the demethylases, and readers as the m6A binding proteins. Its dynamic and reversible modification process is mainly dependent on demethylase, while the methylation localization of a specific region depends on its main consensus motif recognition. Researches have shown that m6A modification can affect the stability of A: U base pairing.20

The methylation of mRNA is mainly dependent on the polyprotein adenosine methyltransferase complex, of which METTL3, METTL14, and Wilms tumor 1-associated protein (WTAP) are common complexes. METTL3 acts as the catalytic core, which is the S-adenosyl-L-methionine (SAM) binding component of the complex and has a catalytic function itself. METTL3 transfers methyl from SAM to the receptor adenine portion, while METTL14 acts as an RNA binding platform, facilitating RNA substrate binding and enhancing complex integrity. By intracellular localization of METTL3, it was found that METTL3 is expressed in both the nucleus and cytoplasm of the cell, which confirms that it could play a methylation function in different sites.21 Also, this multi-protein complex is essential in cells, and its removal leads to cell death. The loss of METTL3 in mice can lead to the death of early embryos,22 where METTL3 knockout in mouse embryonic stem cells (ESCs) significantly reduces the m6A peak, resulting in the loss of the self-renewal ability of the damaged ESCs and the differentiation of multiple lineages in vivo and in vitro.23

METTL14 is a homologous gene of METTL3, which can independently and specifically recognize the common motif GAC. The formation of a stable heterodimer core complex between the two makes the methylation component more active.24 The main function of WTAP is to recruit METTL3 and METTL14. Although the WTAP protein does not play a direct role in transmethylation, its homologous analogs Mum2 and FIP37 are related to METTL3 and are necessary components for effective methylation of mRNA. The interaction of WTAP with the METTL3-METTL14 complex can promote the translocation of the complex to nuclear spots. One study showed that methylation profiles defined by monitoring m6A levels at the depletion of WTAP could be divided into two categories: WTAP-dependent sites and non-WTAP dependent sites.25 Among them, WTAP dependent sites are located in the transcript, with a static topological structure and inversely proportional to mRNA stability, which can promote its degradation. A non-WTAP dependent site is formed at the base of the first transcription as part of the cap structure. Such sites exist in tens of millions of sites, resulting in unprecedented transcriptome complexity. It is worth mentioning that WTAP is not only a regulator required by m6A but also up-regulated in many tumors. A study has shown that both METTL3 knockdown and overexpression lead to up-regulation of WTAP protein,26 suggesting that METTL3 levels are critical to WTAP homeostasis and further suggesting that the oncogenic ability of WTAP may be closely related to the functional m6A methylation complex.

In addition to the above enzymes which play an important role in the methylation process, in recent years, through proteomic screening and other high-throughput technologies, researchers have found that KIAA1429,25 RBM15,27 and METTL1628 may be other subunits of the methyltransferase complex, which can selectively identify binding sites to achieve accurate post-transcriptional regulation. In 2019, Methyltransferase like 5 (METTL5) was identified as the enzyme responsible for 18S rRNA m6A modification, and zinc finger CCHC-type containing 4 (ZCCHC4) was identified as a 28S rRNA modification enzyme, while METTL5 must form a heterodimer with the known methyltransferase activator tRNA methyltransferase subunit 11–2 (TRMT112) to achieve metabolic stability in cells.18,29

Although methyltransferases have been discovered since the 1970s, it was not until 2011 that the first demethylase – fat mass and obesity-associated protein (FTO) was discovered by Jia et al,30 which established the recognition of methylation reversibility. In vitro experiments have shown that FTO has effective oxidative demethylation activity targeting abundant m6A sites in RNA. Knocking down FTO with siRNA leads to an increase in m6A in mRNA, while overexpression of FTO leads to a decrease in m6A in human cells. Further results of nuclear spot co-localization confirmed that m6A is the main physiological substrate of FTO in nuclear RNA. Exogenous overexpression of FTO enables it to efficiently bind to RNA sites containing the m6A motif and specifically remove m6A modification in the GGACU and RRACU motifs in a concentration-dependent manner. This finding highlights the role of the dynamics of FTO in target selection, which is expected to promote the dynamic modification of m6A and the plasticity of FTO in biological function and disease.31 In 2013, Zheng et al found another enzyme ALKBH5 with a demethylation effect – mammalian RNA demethylation enzyme that affects RNA metabolism and mouse fertility,32 and its N terminal has an alanine-rich region and a unique coiled-coil structure. This demethylation activity of ALKBH5 significantly affected mRNA output, RNA metabolism, and the assembly of mRNA processing factors in nuclear spots. Recently, a new demethylase ALKB10B was discovered in Arabidopsis thaliana.33 The bidirectional modulation effect of Writers and Erasers deepened the clinical understanding of the disease, and it is believed that more m6A modification-related effects will be explored in future studies to guide clinical diagnosis and treatment.

m6A-modified mRNAs perform specific biological functions mainly through two pathways: while the first is to fine-tune the methylated transcript to block or induce protein–RNA interactions, the second is to require recognition by a specific RNA-binding protein (also known as methylated readers), to induce subsequent reactions. A variety of reading proteins have been identified by RNA pull-down assay, including proteins in the YTH domain, nuclear heterogeneous ribose protein (HNRNP), and eukaryotic initiation factor (eIF). The functions of these reading proteins include specific binding to the m6A methylation region, weakening the homologous binding of RNA-binding proteins, and altering the secondary structure of RNA to alter the protein-RNA interaction. Proteins with the YTH domain include YTHDC1,34,35 YTHDC2,36,37 YTHDF1,38 YTHDF2,39 and YTHDF3.40 While YTHDF1-3 specifically recognizes m6A-modified mRNA in the cytoplasm, YTHDC1-2 mainly acts in the nucleus. These proteins have the YTH domain at the C-terminal and can overlap with the m6A consensus motif to mediate RNA-specific binding, while the P/Q/N-rich domain is related to subcellular localization.

The eIF3 protein can bind to the m6A modified base on RNA 5 ‘UTRs to promote mRNA translation. The interaction between METTL3 and eukaryotic translation-initiator 3 subunit h (eIF3h) is necessary to promote translation and form densely packed multi-ribosomes and carcinogenic transformation. The findings of Choe et al reveal a mechanism for translation control based on the mRNA cycle and identify METTL3-eIF3h, as a potential therapeutic target for cancer patients.41 Moreover, HNRNPA2B1, a member of the hnRNP family of proteins, functions as a reading protein. Unlike YTHDC1, HNRNPA2B1 does not bind directly to the m6A modified base. In addition to activating the downstream pathway of miRNA primers (pri-miRNAs), HNRNPA2B1 is also involved in the processing of miRNA precursors (pre-miRNAs). Kwon et al showed that HNRNPA2B1 plays an important role in early embryogenesis by regulating transcription-related factors and determining cell fate transformation. HNRNPA2B1 is regulated by METTL3-dependent m6A RNA methylation.42 In summary, m6A can be deposited on the transcript during transcription and regulates biological processes such as cutting, output, translation, and degradation of mRNA by changing the structure of mRNA or depending on the specific recognition of readers, and thus may play an important role in the occurrence and development of a variety of diseases. Figure 1 summarizes the different roles played by methyltransferases, demethylases, and methylation binding proteins in the m6A modification of RNA.

Figure 1

Role of different regulatory factors in m6A modification of RNA. Writers, erasers, and readers play different roles in the dynamic m6A modification of RNA. Methyltransferase complex with METTL3 as the core positively regulates m6A modification, while demethylases represented by FTO and ALKBH5 negatively regulate m6A modification. Also, the recognition of m6A modification requires the recognition and combination of various readers.

Effects of m6A Modification on lncRNA

The role of lncRNAs in a variety of diseases has attracted increasing attention. ncRNAs modification may in its function adjustment, proteomic interactions, and downstream effector play an important role, and is very rich in m6A as eukaryotes lncRNA of interior decoration, by adjusting the cutting of ncRNAs itself, transshipment, stability, and degradation, affect the biological function of the cell to regulate cell proliferation and metastasis of cancer, stem cell differentiation, and homeostasis. Hence, they play an indispensable role in regulating the body’s physiological functions. A study described the effect of m6A modification of two chromatin-related lncRNAs MALAT1 and XIST on gene expression.43 MALAT1 is a highly abundant m6A modified transcript with metastasis-associated lung adenocarcinoma transcript 1, and its mutation is highly correlated with upregulation and cancer development and metastasis. However, XIST exists in the nucleus and acts as a major regulator of X chromosome inactivation.

Another study by Yang et al showed that the internal m6A modification of LINC1281 mediates a competitive endogenous RNA (ceRNA) model to regulate the differentiation of mouse ESC (mESCs).44 m6A is highly enriched in the LINC1281 transcript, which ensures the characterization of mESCs by isolating the pluripotency-related let-7 family of microRNAs (miRNAs), and this RNA–RNA interaction is dependent on m6A. After a comprehensive analysis of the m6A modification of lncRNA in CRC, Zuo et al found that the level of m6A of lncRNA in CRC tissues is higher than that in normal tissues of adjacent tumors. A total of 8332 m6A peaks were detected in 6690 lncRNAs in CRC tissues. Approximately 91% of the modified lncRNAs had a unique m6A modification peak. A total of 383 lncRNAs were differentially methylated in CRC, 48.24% of which were 1–1000 bp in length, and most of them were located on chromosomes 1, 2, 7, 11, 16, and 19. GO and KEGG analysis showed that genes close to differentially methylated or expressed lncRNAs were related to the occurrence and development of CRC. Methylation was positively correlated with lncRNA expression levels in CRC and normal tissues adjacent to tumors.45

Similarly, Liu et al showed that the internal m6A modification of lncRNA Thor modulates cancer cell proliferation in an m6A reader-dependent manner. Specific m6A readers YTHDF1 and YTHDF2 can read the highly enriched m6A motif on lncRNA Thor transcripts, regulate its stability, and thus maintain the carcinogenic effect.46 Interestingly, the two studies of He et al47 and Chen et al48 respectively confirmed that ALKBH5 played two opposite effects of promoting cancer and inhibiting cancer in different cancers by regulating different lncRNA levels through demethylation. ALKBH5 inhibits the progression of pancreatic cancer by demethylation of lncRNA KCNK15-AS1, while the up-regulation of lncRNA PVT1 mediated by ALKBH5 promotes the proliferation of osteosarcoma cells in vitro and tumor growth in vivo.

Effects of m6A Modification on miRNA

m6A peaks are enriched at miRNA target sites at the 3ʹ end and 5ʹ end of the 3ʹUTR, suggesting a potential association between m6A modification and miRNA target sites. The relationship between the two is mainly reflected in miRNA biosynthesis, mRNA–miRNA interaction, and m6A target selection. Moreover, the abundance of m6A positively correlates with the Dicer enzyme mediating miRNA maturation.49,50 Research in mammals has shown that the m6A marker promotes the initiation of miRNA biogenesis as a key post-transcriptional modification. METTL3 can methylate pri-miRNAs and label them for recognition and processing by DGCR8. Similarly, METTL3 deletion reduces the binding of DGCR8 to pri-miRNAs, leading to an overall reduction in mature miRNAs, accompanied by the accumulation of unprocessed pri-miRNAs.51 Hao et al found that using RNA guide base editing technique of miRNA 675 m6A area of the base, substitution, and target mutations can induce the occurrence of apoptosis, and miR675 m6A modification sites upstream regions of mutations, resulting in a loss of the H19 gene expression in HEK293T cells and apoptosis induction. This shows that the methylation modification of miRNA plays an important role in cell.52 Furthermore, manipulation of miRNA expression or sequence can alter the modification level of m6A by regulating the binding of METTL3 methyltransferase to mRNAs containing miRNA targets. The increase of m6A content promotes the reprogramming of mouse embryonic fibroblasts (MEFs) into pluripotent stem cells. Conversely, the reduced m6A level impedes reprogramming53 and studies have shown the excellent potential of miRNA–mRNA interactions and methylation modifications in the field of cell reprogramming.

As described above, HNRNPA2B1 is involved in the processing of pri-miRNA. HNRNPA2B1 direct binding to a set of nuclear transcripts and produces a selective splicing effect similar to that of the m6A transcript METTL3. In addition, HNRNPA2B1 binds to the m6A marker in the subsets of primary miRNA transcripts and interacts with the miRNA microprocessor protein complex DGCR8 to promote primary miRNA processing. HNRNPA2B1 and METTL3 deletions also lead to similar processing defects in these pri-miRNA precursors. HNRNPA2B1 moderates the effect of this marker on primary miRNA processing and selective splicing to a certain extent.54 Moreover, another study showed that insulin-like growth factor 2 mRNA-binding protein 1(IGF2BP1, an mRNA binding protein) could promote the expression of SRF by impairing the mRNA degradation of miRNA-mediated transcription regulator SRF in an m6A-dependent manner, and thus regulates the expression of genes in cancer.55 This study identified the stabilizing role of miRNome- and m6A-dependent regulation of gene expression in cancer. Jin et al showed that m6A demethylase ALKBH5 inhibits tumor growth and metastasis by reducing YTHDFs-mediated YAP expression and inhibiting miR-107/LATS2-mediated YAP activity.56 In addition to being regulated by methylation, miRNA can also reverse regulate the methylation level of mRNA. Yang et al showed that miR-145 regulates the level of m6A by targeting the 3ʹ-UTR of YTHDF2 mRNA in HCC cells,57 which confirms the interaction between miRNA and m6A RNA. Moreover, the newly discovered methyltransferase complex component KIAA1429 can promote the progression of osteosarcoma by promoting stem cell properties and is regulated by miR-143-3p. Knocking down KIAA1429 or ectopically overexpressing miR-143-3p can inhibit stem cell properties and alleviate the disease.58 These studies have further clarified the effect of m6A modification on miRNA biosynthesis and their interaction on cell function, as well as the potential role it may play in cancer and other diseases.

Effects of m6A Modification on circRNA

CircRNAs, a type of ncRNAs, are widely present in eukaryotes and their abnormal expression is closely related to a variety of diseases. More researches have shown that circRNA regulates cell function in a variety of ways and can be used as an effective diagnostic marker for diseases. Zhou et al showed that the genome-wide mapping of m6A circRNA can identify broad and specific cell type methylation patterns that are distinct from mRNA.59 Methylation usually occurs in the exon region (but not in mRNA), suggesting that some m6A modifications to circRNAs may occur during or after circRNA formation. m6A modification of circRNA can affect the reverse splicing and translation process. Taking circ-ZNF609 as an example, the reverse splicing reaction of circRNA requires the participation and guidance of METTL3 and YTHDC1. Due to the translation capability of circ-ZNF609, further studies show that m6A-modified circ-ZNF609 regulates its translation through YTHDF3 and eIF4G2 recognition.60 A recent study showed that the m6A modification of human circRNA inhibits innate immunity.61 Exogenous circRNAs are effective adjuvants for inducing antigen-specific T cell activation, antibody production, and in vivo antitumor immunity. Unmodified circRNAs directly activate RNA pattern recognition receptor RIG-I in the presence of lysine-63-linked polyubiquitin chains, leading to filamentation of junction protein MAVs and activation of downstream transcription factor IRF3, while modification of m6A would inhibit its original activity. Findings by He et al suggest that circNSUN2 is a key biomarker for oncogenic circRNAs and liver metastasis from CRC.62 At present, due to the lack of understanding of the regulatory role of ncRNAs, its abundant chemical modification types present different challenges to be studied, with the potential of presenting significant progress of the mechanism, clinical diagnosis, and treatment of diseases.

In conclusion, m6A modification plays an important role in regulating gene expression, splicing, RNA editing, RNA stability, controlling mRNA lifetime and degradation, and mediating circRNA translation. m6A RNA methylation greatly affects RNA metabolism which is involved in the pathogenesis of a variety of diseases including cancer and gastrointestinal inflammation; hence, it is imperative to further study its regulatory mechanism.

Regulation of Intestinal Mucosal Immunity by m6A RNA Modification

m6A RNA Modification and Dendritic Cells

Dendritic cells (DCs), as important antigen-presenting cells, link innate and adaptive immune responses and are the core of coordinating host tolerance and host immunity in peripheral lymphoid tissues, as well as the first point of contact between intestinal flora and the immune system. Typically, immature DCs (imDCs) induce immune tolerance, and mature DCs (maDCs) stimulate and activate the immune response. The abnormal maturation or activation disorder of DCs at different stages can lead to abnormal responses of the host immune system, and even induce inflammation and autoimmune diseases.

As early as 2005, researchers found that DCs exposed to nucleoside modified RNA expressed significantly fewer cytokines and activation markers than DCs treated with unmodified RNA. In other words, nucleoside modification inhibits the potential of RNA to activate DCs.63 The study of Wang et al confirmed that METTL3-mediated mRNA m6A methylation promotes the activation and function of DCs.64 m6A modification of the METTL3-mediated CD40, CD80, and TLR4 signal adapter TIRAP transcription factors enhance its translation in DCs to stimulate T cell activation and enhance Toll-like receptor 4 (TLR4)/nuclear factor-κB (NF-κB) signal-induced cytokine production. However, the specific loss of METTL3 in DCs leads to impaired phenotype and functional maturation of DCs, decreased expression of co-stimulatory molecules CD40, CD80, and cytokine interleukin (IL)-12, which reduces its ability to stimulate T cell response in vivo and in vitro. Similarly, Wu et al found that METTL3-silences of DCs showed immature characteristics and prolonged allograft survival after constructing a mouse heart transplant model with METTL3 knockout,65 highlighting the regulatory role of m6A in DCs maturation and host immune response. Also, one study showed that C-C chemokine receptor 7 (CCR7) stimulation up-regulates lnc-Dpf3 by removing the m6A modification to prevent RNA degradation. The deletion of specific lnc-Dpf3 in DCs increases CCR7-mediated DC migration, leading to excessive adaptive immune response and inflammatory damage.66 In mechanism, CCR7 stimulation can activate the hypoxia-inducible factor 1α (HIF-1α) transcription factor pathway in DCs. lnc-Dpf3 directly binds to HIF-1α and inhibits the transcription of HIF-1α-dependent glycolytic gene LDHA, thereby inhibiting the glycolytic metabolism and migration of DCs.

In addition to the effects of m6A modification on the maturation and activation of DCs, DCs can also exert antitumor immunity through methylation-related modifications. Han et al established a mouse model of the m6A binding protein YTHDF1 deficiency and found that the defective mice showed an elevated antitumor response of antigen-specific CD8+ T cells.67 At present, most studies point to DCs maturation at different stages with s different effects on the body’s immune response, and m6A modification occurs in DCs by regulating the degradation and translation of RNA, which can be explored to restore the function of DCs required for normal stimulation of molecules and immune response, as shown in Figure 2. Current data still lack a complete and clear understanding of its detailed mechanism; therefore, further research on methylation modification in DCs needs to be carried out.

Figure 2

Effects of m6A on the normal maturation and physiological function of DCs. (A) the role of m6A in the maturation of DCs and activation of T cells. The m6A modification of Trap transcription factor in DCs promotes the translation of CD40, CD80, and TLR4 signals on its membrane surface, which not only activates T cells but also enhances the production of cytokines induced by TLR4/NF-κB signals. (B) the role of m6A in the migration of mature DCs. Stimulation of CCR7 activates the HIF-1α transcription factor pathway in DC. m6A modified lnc-Dpf3 directly binds to HIF-1α and inhibits the transcription of HIF-1α-dependent glycolytic gene LDHA, thus inhibiting the glycolytic metabolism and migration ability of DCs. (C) m6A mediated the antitumor effect of DCs. Transcript Flt3L encoding lysosomal protease is labeled with m6A and recognized by YTHDF1, which enhances the translation of lysosomal cathepsin in DCs. However, the deletion of YTHDF1 in classical dendritic cells leads to its inhibition, which significantly enhances the cross-presentation ability of tumor antigen, and makes CD8+T cells highly express PD-L1 and IFN-γ.

m6A RNA Modification and Its Regulation of T Cells

In recent years, with the continuous exploration of epigenetic modifications such as methylation, many papers have reported the crucial role of m6A in the regulation of T cell homeostasis and related pathways. Li et al showed that the loss of METTL3 in mouse T cells disrupts T cell homeostasis and differentiation.68 The mRNAs of suppressor of cytokine signaling (SOCS) family genes encoding signal transducer and activator of transcription 1 (STAT1), suppressor of cytokine signaling 3 (SOCS3), and cytokine-inducible SH2 containing protein (CISH) are all labeled with m6A. In METTL3-deficient naive T cells, the mRNA attenuation is slow and the protein expression level is increased, while the increased SOCS family activity further plays a role in inhibiting IL-7-mediated STAT5 activation and T cell homeostasis proliferation and differentiation. Another study confirmed a similar effect of m6A on T cells, in which m6A had control over transcription stability in unstimulated T cells. m6A affects all RNA kinetic rates during T cell differentiation mainly by 1) delaying induction of synthesis rate and simultaneously impair T cell, 2) regulation of processing rate and 3) continuous upregulation of degradation rate.69

Similarly, Zhu et al found that m6A is involved in regulating the development of follicular helper T cells (Tfh cells) through glycolysis. E3 ubiquitin ligase von Hippel–Lindau (VHL) is required for Tfh cells development and function during acute viral infection or antigen immunity. VHL actively regulates early Tfh cell initiation through HIF-1α dependent glycolysis pathway. However, once VHL is defective, its glycolytic activity is increased. Through RNA interference screening, it was found that the glycolytic enzyme glyceraldehyde-3-phosphate dehydrogenase (GAPDH) decreased the expression of inducible T cell costimulator (ICOS) through the modification of m6A, which is a key molecule in the development of Tfh cells.70 Tong et al found that m6A mRNA methylation maintains the inhibition function of Tregs and that m6A RNA modification could specifically target the same gene class, which encodes components of essential signaling pathways in different T cell subtypes, thereby controlling the differentiation of juvenile T cells and maintaining the inhibition function of Tregs.15 Interestingly, Sprent et al also demonstrated that inhibition of mRNA methylation by blocking the m6A writers’ action promotes T cell infantilization.71 In conclusion, m6A plays an important role in the normal cell biological functions of various T cells, regulating the state and maturity of cells, affecting the secretion and release of cytokines, and participating in the immune regulation process.

Advances in the Role of m6A in Intestinal Mucosal Immunity

Under normal physiological conditions, intestinal mucosal tissue is an important barrier to isolate the body from foreign pathogens and maintain the immune homeostasis of the intestinal environment. Intestinal microecological imbalance harms the function of the intestinal mucosal barrier and permits pathogen invasion of the intestinal mucosa, leading to recruitment of intestinal inherent lymphocytes and mesenteric lymphatic tissue inflammation, where other immune cells are mobilized to the site to remove pathogen. Long-term chronic inflammatory pathological cases and excessive immune response are often accompanied by serious damage of intestinal mucosa, wherein pathogens damaged the mucous membrane layer to induce a continual immune response.

Wu et al showed that the dynamic epigenetic modification of intestinal tissue strongly mediates the crosstalk between intestinal microbes and the intestinal mucosal barrier. Lactobacillus and Bifidobacterium species in the intestinal symbiotic flora can synthesize folic acid to increase DNA methylation and mRNA m6A modification in the intestinal tract, thus ensuring the normal development of the intestinal tract.72 Similarly, Jabs et al found that the intestinal microbiota affects the epithelial transcriptome of m6A in the cecum of mice. Changes in intestinal microbiota are associated with m6A modification in the cecum and to a lesser extent, affect m6A modification in the liver, affecting pathways related to metabolism, inflammation, and antimicrobial responses.73 In addition to the involvement of intestinal microorganisms in m6A modification, Han et al confirmed the important role of m6A modification in intestinal stem cells (ISCs). The high expression of YTHDF1 in ISCS is detected to promote the translation of Wnt signal effectors including TCF7L2/TCF4, thus enhancing β-catenin activity. Gene ablation of YTHDF1 significantly blocks Wnt-driven regeneration and tumorigenesis and reduces the stem cell characteristics of ISCs. Targeting YTHDF1 in ISCs with established tumors shrinks the tumors and prolongs survival. These findings reveal that YTHDF1 is an amplifier of Wnt/β-catenin signaling at the translational level, which is necessary for maintaining ISCS regeneration and tumorigenesis and is essential for normal intestinal development in mice.74

DCs and T cells are also important participants in intestinal immunity, and the corresponding effects generated by their internal m6A modifications can control the excessive immune response, thus alleviating the persistent intestinal inflammation and excessive destruction of the mucosal barrier. In addition to these immune cells, intestinal mucosal epithelial cells (IECs), as the main component of the barrier, play an indispensable role, but when methylation occurs in IECs, it affects its normal barrier function. A recent study has shown that dietary gluten-induced RNA methylation changes regulate intestinal inflammation through allele-specific chromosome region maintenance protein 1 (XPO1, nuclear output receptor involved in key signaling pathways) translation in IECs.75 Individuals with celiac disease risk alleles have higher m6A methylation at 5ʹUTR of XPO1 RNA, which leads to higher XPO1 protein volume mediated by YTHDF1, resulting in downstream nuclear factor kappa B (NF-κB) activity, stimulating epithelial cells to produce large amounts of the pro-inflammatory cytokine IL-8, and mediating the subsequent inflammatory response. The results further support the possibility that the m6A-XPO1-NF-kB axis may respond to intestinal epithelial injury caused by other drugs, which may have direct significance for the treatment of a variety of gastrointestinal diseases.

In conclusion, all the m6A modifications involved in the composition of the intestinal mucosal barrier play an irreplaceable role in mucosal immunity. Surprisingly, a recent study by Gan et al showed that resveratrol and curcumin decrease m6A enrichment on intestinal tight junction protein transcripts and heme oxygenase-1, increase intestinal antioxidant capacity and tight junction protein mRNA expression, and ultimately improve intestinal mucosal integrity of weaned piglets.76 However, the current research on m6A and intestinal mucosal immunity are poorly understood. Therefore, future studies can carry out extensive exploration and discussions on the role of m6A in intestinal mucosal immunity, and further research the various effects of epigenetic modification. Figure 3 illustrates how m6A regulates intestinal immune components and participates in the process of intestinal mucosal immunity.

Figure 3

Mechanism of m6A regulation of intestinal mucosal immunity. The folic acid produced by intestinal symbiotic flora such as Lactobacillus and Bifidobacterium, as well as vitamin B2 and B6 in the intestinal tract, participate in SAM synthesis, which are the main raw materials for m6A modification. As an important part of the intestinal mucosal barrier, m6A modification of intracellular XPO1 in IECs further activates the NF-κB pathway and releases inflammatory factors such as IL-8. As an important component of the immune response, the intracellular SOCS m6A modification promotes the activation of the TCR and STAT5 pathway and promotes the proliferation and differentiation of intestinal T cells and the secretion of cytokines such as IL 2/7.

m6A RNA Methylation Modification and Inflammatory Bowel Disease

It is well known that IBD is accompanied by an inflammation of the intestinal mucosal barrier and an abnormally persistent immune response. A large number of previous studies have confirmed that m6A plays an important role in the regulation of immune cell state, normal physiological function, and intestinal mucosal immunity.77–79 Therefore, scholars speculate that m6A modification may play a role in the occurrence and development of IBD. An important question remains, whether clinical diagnosis and treatment be carried out by targeting m6A modification sites?

A recent study showed that the deletion of METTL14, a component of RNA m6A methyltransferase, in T cells causes spontaneous colitis in mice. METTL14 deficiency in T cells causes spontaneous colitis in mice, and its development can be attributed to the dysfunction of Tregs. The decreased expression of Rorγ T in METTL14 deficient Tregs results in impaired induction from naive T cells to induce Tregs, while the adoptive transfer of wild-type Tregs weakens the colitis phenotype.14 Howell et al collected samples from 236 pediatric patients newly diagnosed with IBD with DNA methylation patterns and transcriptome of primary IECs, the results showed that compared with the control group, patients with CD and UC have obvious colon epithelium DNA methylation and transcription pattern, and DNA methylation changes with time are stable. Further in vitro analysis suggested a possible clinical application of distinguishing between IBD subtypes and prognosis judgment accordingly.80 In an experiment that investigated the regulatory effect of m6A on T cells, naive METTL3-deficient T cells were unable to expand their homeostatic balance in a mouse model of lymphatic adoptive transplantation and remained in a naive state for up to 12 weeks, thereby preventing the development of colitis.68

In addition, the novel m6A-XPO1-NF-kB pathway that is activated in CD patients also clearly explains the regulatory role of m6A in IBD.75 As the first demethylase known to humans, FTO plays an important role in protecting against adverse reactions caused by the treatment of IBD. Several studies have shown that FTO protects IBD patients from adverse reactions after thioprine treatment.81–83 However, whether it plays a role in IBD through demethylation is unknown, which is a very interesting area to investigate. One recent study of m6A associated-inflammatory pain in a complete Freund’s adjuvant in induced mice model revealed a significant rise in spinal cord m6A modification level with an increased spinal cord METTL3 expression. When expressed in uninfected mice’s spinal cord, METTL3 can lead to pain as observed in their behavior and neuron sensitization. This development of m6A modifications in pathological pain provides a new angle of view.84 Unfortunately, the current research on m6A and IBD is very limited, so the cognition of m6A is relatively limited. There is a need for relevant exploration to provide more possibilities for the pathogenesis, clinical diagnosis, and treatment application in IBD. Except in IBD, m6A also has an important function in IBD-associated CRC.

m6A RNA Methylation Modification and Colorectal Cancer

At present, a large number of studies have confirmed that m6A modification plays an important role in the occurrence and development of various cancers, including gastric cancer,11,85 lung cancer,13 breast cancer,9 liver cancer,10,62 and colon cancer.86,87 CRC, as the top three cancers in the world, has been studied by many scholars with regards to the mechanism of m6A modification. Zhang et al carried out methylated RNA immunoprecipitation sequencing (MeRIP-seq) on six pairs of CRC samples and normal tissues adjacent to the tumor, and found that compared with normal tissues adjacent to the tumor, CRC samples had 1343 out-of-balance m6A peaks, of which 625 were significantly up-regulated and 718 were significantly down-regulated. Genes involved in m6A peak changes play a key role in regulating glucose metabolism, RNA metabolism, and cancer stem cells.87 Liu et al used cancer genome atlas (TCGA), the gene expression omnibus (GEO), the human protein atlas (HPA) databases, and a tissue microarray (TMA) to verify the expression of m6A-related genes at mRNA and protein levels. It was found that most m6A-related genes were significantly up-regulated in tumor tissues, while METTL14, YTHDF3, and ALKBH5 were downregulated in CRC, and there was no significant difference in FTO,88 which suggests that the abnormal expression of m6A-related genes in CRC may play an important role in its progression. The latest research results of Wang et al further indicate that the poor prognosis of CRC may be closely related to the high expression of m6A and the high expression of METTL3, METTL16, and WTAP.89 Table 1 summarizes the different roles and mechanisms of m6A-related enzymes and proteins in IBD and CRC.

Table 1

Functions of m6A Related Enzymes and Binding Proteins in IBD and CRC Progression

m6A-Related Molecules	Effect of Deficiency	Targets	Mechanisms and Functions	References
METTL3	Downregulated in IBD	T cell	T cells are unable to expand in homeostatic balance and remain in a juvenile state, thus preventing the occurrence of colitis.	[68]
METTL3	Upregulated in inflammatory pain disease	Neuron cell	Overexpression of METTL3 in the spinal cord leads to painful behavior and neuronal sensitization.	[84]
METTL14	Downregulated in IBD	Treg	The decreased expression of RORγt in Tregs results in impaired induction from naive T cells to induce Tregs, and dysfunctions leading to spontaneous colitis.	[14]
METTL3	Upregulated in CRC	CRC cell	The proliferation and metastasis of CRC cells can be promoted by regulating the expression of cell cycle-related proteins and glucose uptake and utilization.	[92,94,95]
METTL14	Downregulated in CRC	CRC cell	Greatly enhances the proliferation and invasion ability of CRC cells in vitro, and promotes tumorigenicity and metastasis in vivo.	[96,97]
YTHDF1	Downregulated in CRC	CRC cell	Significantly inhibits the tumorigenicity of CRC cells in vitro and the growth of xenograft tumors in mice.	[100]
hnRNPCL2	Upregulated in CRC	CRC cell	Reprograms mitochondrial metabolism in cancer cells and is associated with poor prognosis.	[105]

In CRC resistant to immunotherapy, the deletion of METTL3 and METTL14 can inhibit m6A modification, and promote IFN-γ-Stat1-Irf1 signal transduction through YTHDF2 to stabilize STAT1 and Irf1 mRNA, thus enhancing the response to anti-PD-1 therapy, which provides METTL3 and METTL14 as potential therapeutic targets for anti-cancer immunotherapy.90 Li et al detected the expression of METTL3 in CRC patients and found that higher METTL3 expression is found in CRC metastatic tissues, which was related to poor prognosis. Furthermore, the target gene and downstream binding site of METTL3 were screened by bioinformatics. MeRIP-seq and showed that SRY (sex-determining region Y)-box 2 (SOX2) was the downstream gene of METTL3. Mechanically, methylated SOX2 transcripts, especially the CDS region, are bound by specific m6A binding protein insulin-like growth factor 2 mRNA binding protein 2 (IGF2BP2) to prevent SOX2 mRNA degradation.91 This research reveals a new mechanism that METTL3, as an oncogene, maintains SOX2 expression in CRC cells in an m6A-IGF2BP2-dependent manner, and provides a potential biomarker for predicting CRC prognosis.

Another clinical study found that METTL3 stabilizes the expression of HK2 and SLC2A1 (GLUT1) in CRC through an m6A-IGF2BP2/3-dependent mechanism, suggesting that targeting METTL3 and its pathway provide other reasonable therapeutic targets for CRC patients with high glucose metabolism.92 Similarly, Peng et al research revealed that the upregulated METTL3 is related to the abnormal modification of m6A in CRC, and positively correlates with tumor metastasis. METTL3 can methylate pri-miR-1246 and further promote the maturation of pri-miR-1246. Bioinformatics tools predict that the anti-cancer gene SPRED2 is the downstream target of miR-1246, and the downregulation of SPRED2 further reverses the inhibition of the MAPK pathway.93 The results suggest that the METTL3/miR-1246/SPRED2 axis plays an important role in tumor metastasis. Chen et al found that METTL3 induces GLUT1 translation in an m6A-dependent manner and promotes glucose uptake and lactic acid production, which leads to the activation of the mTORC1 signal and the development of CRC.94 In addition, METTL3 promotes CRC proliferation by stabilizing cyclin E1 (CCNE1) mRNA in an m6A-dependent manner.95 The above studies revealed that METTL3 plays a role in promoting CRC by interacting with various RNA and proteins and can be used as a potential biomarker and therapeutic target.

Interestingly, METTL14, as another important component of the methyltransferase complex, exerts an opposite effect on CRC progression. A clinical study has revealed that METTL14 deficiency is associated with poor prognosis in patients with CRC. Functional experiments show that the knockdown of METTL14 can greatly enhance the proliferation and invasion ability of CRC cells in vitro and promote tumorigenicity and metastasis in vivo. In terms of its mechanism, lncRNA XIST is identified as a downstream target of METTL14, and m6A methylated XIST is recognized by an m6A reader protein YTHDF2 to mediate the degradation of XIST. Once the METTL14 is knocked down, the m6A level of XIST is eliminated and XIST expression is enhanced.96 Therefore, preliminary studies have shown that METTL14 can inhibit the proliferation and metastasis of CRC by down-regulating the oncogenic lncRNA XIST.

Similarly, Chen et al also found that the knockout of METTL14 promotes CRC, but further screening of other targets of METTL14 indicated that METTL14 inhibits the growth of CRC cells through the miR-375/Yes-associated protein 1 (YAP1) pathway, and prevents the migration and invasion of CRC cells through the miR-375/SP1 pathway,97 which provides new insights into the mechanism of METTL14 in CRC. Another study showed that METTL14 knockout significantly inhibits the m6A modification of SRY-related high-mobility group box 4 (SOX4) mRNA and increases SOX4 mRNA expression, while METTL14-mediated degradation of SOX4 mRNA depends on the YTHDF2 pathway. Mechanically, METTL14 may partially inhibit the malignant process of CRC through the SOX4-mediated epithelial-mesenchymal transformation (EMT) process and the PI3K/Akt signal.98 The above studies reveal the mechanism of different pathways mediated by METTL4 in CRC.

Moreover, the regulatory factor of m6A mRNA methylation also plays an important role in CRC, and Kuai et al identified four m6A genes (YTHDF1, IGF2BP1, IGF2BP3, and eIF3b) as potential biomarkers of CRC and adenoma.99 In addition to a methyltransferase, which plays an important role in CRC, m6A binding protein is also indispensable as the core factor of methylation modification. Knocking down YTHDF1 expression significantly inhibits tumorigenicity of CRC cells in vitro and xenograft tumor growth in mice. YTHDF1 silencing inhibits the ability to form colon cancer in vitro. The silencing of YTHDF1 significantly inhibits the activity of the Wnt/β-catenin pathway in CRC cells, revealing a positive regulatory role of YTHDF1 in CRC.100

LncRNAs play an important role in the epigenetic regulation of cancer cells. In recent years, researches on the regulatory role of m6A modification of lncRNA in a variety of cancers have gained attention. Currently, several studies have reported the key role of m6A modification of lncRNA in the progression of CRC. A study conducted by Zuo et al detected the correlation between the modification of lncRNA m6A in CRC and adjacent normal tissues and found that lncRNA m6A levels in CRC tissues are higher than those in adjacent normal tissues. A total of 8332 m6A peaks were detected in 6690 lncRNAs in CRC tissues. About 91% of the modified lncRNAs had a unique m6A modification peak, and a total of 383 lncRNAs were differentially methylated in CRC.101 Ni et al found that lncRNA GAS5 expression negatively correlates with YAP and YTHDF3 protein levels in tumors from patients with CRC, and YAP activation is an important participant in a variety of cancers including CRC. The researchers found that the lncRNA GAS5 modified by m6A is negatively regulated by m6A “readers” YTHDF3, and further inhibits the progress of CRC by interacting with YAP to trigger its phosphorylation and degradation process.12 This experiment reveals the negative regulatory loop of the lncRNA GAS5-YAP-YTHDF3 axis and expands a new idea for the treatment of CRC.

Wang et al screened the highly expressed lncRNAs in human CRC samples and found that lncRNA LINRIS is upregulated in CRC tissues with poor overall survival, and inhibition of LINRIS prevents tumor proliferation in both the in-situ tumor model and patient-derived xenotransplantation (PDX) model. LINRIS knockout weakens the downstream effects of m6A “readers” IGF2BP2, especially the Myc-mediated glycolysis of CRC cells.102 LINRIS can be used as an independent prognostic marker of CRC and the LINRIS-IGF2BP2-MYC axis promotes the progression of CRC, which is a potential clinical therapeutic target. The methylation modification of RP11/hnRNPA2B1 mRNA compound accelerates the two E3 ligase Siah1 and Fbxo45 mRNA degradation stops the Zeb1 ectomesenchymal transformation (a kind of epithelial related transcription factor) of the proteasome degradation, and increases RP11 nuclear accumulation, thus promote the CRC cell migration, invasion, and EMT. Therefore, RP11 has the potential as a predictive biomarker or therapeutic target for CRC.103 Similarly, LINC00460 enhances the stability of HMGA1 mRNA by interacting with IGF2BP2 and DHX9, and binding to m6A-modified HMGA1 mRNA, thereby inducing the EMT process, promoting the proliferation, migration, and invasion of tumor cells in vitro, and tumor growth and metastasis in vivo.104 Therefore, LINC00460 can be used as a promising predictive biomarker for the diagnosis and prognosis of patients with CRC.

In CRC liver metastasis, circNSUN2 plays a promoting role. In circNSUN2 exists an m6A base sequence (GGACU), one IGF2BP2 combined with base sequence (CAUCAU), and one HMGA2 mRNA binding sites (AAACA), so the tag has m6A motif circNSUN2 through combination with IGF2BP2 recognition and forming circNSUN2/IGF2BP2/HMGA2 complex, wherein HMGA2 mRNA is stable from degradation, thus promoting the settlement of colorectal liver metastasis.62 This suggests that circNSUN2 may represent a key prognostic marker or therapeutic target for this disease. Table 2 lists the recent research advances of the m6A-modified-RNA in the development of colitis and CRC.

Table 2

Advances in the Mechanism of m6A Modification-Related RNA in the Development of Colitis and CRC

RNA	Expression in Disease	Regulatory Proteins	Function and Mechanism	Clinical Significance	References
XPO1	Upregulated in CD	METTL3 and YTHDF1	The 5ʹUTR of XPO1 RNA has higher m6A methylation, resulting in higher XPO1 protein, activation of NF-κB, and subsequent inflammatory response.	A target under evaluation for the treatment of intestinal disorders	[75]
SOCS	Upregulated in colitis	METTL3	METTL3 controls T cell homeostasis by targeting the IL-7/STAT5/SOCS pathway.	A new mechanism of T cell homeostasis and signal-dependent induction of mRNA degradation in colitis	[68]
SOX2	Upregulated in CRC	METTL3 and IGF2BP2	Increasing SOX2 expression promotes the dryness of CRC cells and leads to the progression of CRC through downstream SOX2 target metastasis.	A potential biomarker panel for predicting prognosis in CRC.	[91]
HK2 and SLC2A1	Upregulated in CRC	METTL3 and IGF2BP2/3	METTL3 regulates the mRNA levels and stability of HK2 and SLC2A1, and promotes hyperglycemic metabolism in CRC cells, leading to the activation of mTORC1 signaling and the development of CRC.	Provides potential therapeutic targets for CRC patients with high glucose metabolism	[92,94]
pri-miR-1246	Upregulated in CRC	METTL3	Its maturation downregulates the expression of downstream target SPRED2, further activating the RAF/MEK/ERK pathway.	Suggests that METTL3 /miR-1246/SPRED2 axis plays an important role in CRC metastasis	[93]
XIST	Downregulated in CRC	METTL14 and YTHDF2	METTL14 can inhibit the proliferation and metastasis of CRC by downregulating the oncogenic lncRNA XIST.	METTL4 and XIST can be used as potential diagnostic markers	[96]
miR-375	Downregulated in CRC	METTL14	METTL14 inhibits the growth, migration, and invasion of CRC cells through the miR-375/YAP1 and miR-375/SP1 pathways.	Reveals the role of m6A in regulating miRNA in CRC	[97]
SOX4	Downregulated in CRC	METTL14 and YTHDF2	By increasing SOX4 content, the EMT process mediated by the SOX4 and PI3K/Akt signal inhibition of CRC is promoted.	A potential prognostic biomarker and effective therapeutic target for CRC	[98]
GAS5	Downregulated in CRC	YTHDF3	Under the negative regulation of YTHDF3, CRC progression is further inhibited by its interaction with YAP to trigger its phosphorylation and degradation process.	Provides a new idea for the treatment of CRC	[12]
LINRIS	Upregulated in CRC	IGF2BP2	Glycolysis mediated by the LINRIS-IGF2BP2-Myc axis promotes CRC progression.	As an independent prognostic marker for CRC	[102]
RP11	Upregulated in CRC	hnRNPA2B1	By accelerating the mRNA degradation of SIAH1 and FBXO45 and preventing the degradation of the ZEB1 proteasome, it promotes the migration, invasion, and EMT of CRC cells.	As a predictive biomarker or therapeutic target for CRC	[103]
LINC00460	Upregulated in CRC	IGF2BP2 and DHX9	By binding to m6A modified HMGA1 mRNA to enhance its mRNA stability, the EMT process of the tumor is induced.	For diagnosis and prognosis of patients with CRC	[104]
HSF1	Upregulated in CRC	METTL3 and YTHDF1	β-Catenin inhibits miR455-3p to increase HSF1 mRNA m6A modification, thereby promoting CRC progression.	Potential strategies for interventions in β-catenin-driven cancers	[78]
miR-96	Upregulated in CRC	FTO	By down-regulating AMPKα2, FTO expression is increased, and MYC m6A modification is blocked to upregulate its expression, promoting cell proliferation and anti-apoptosis.	Promising targets for clinical treatment	[79]
circNSUN2	Upregulated in CRC	IGF2BP2	The CircNSUN2/IGF2BP2/HMGA2 complex is formed to stabilize HMGA2 mRNA from degradation, thus promoting liver metastasis of CRC.	Key prognostic markers or therapeutic targets	[62]

Abbreviations: m6A, N6-methyladenosine; IBD, inflammatory bowel disease; CRC, colorectal cancer; UC, ulcerative colitis; CD, Crohn’s disease; m1A, N1-methyladenosine; m5C, 5-Methylcytosine; tRDMT1, tRNA aspartic acid methyltransferase 1; METTL3, methyltransferase like 3; METTL14, methyltransferase like 14; WTAP, Wilms tumor 1-associated protein; SAM, S-adenosyl-L-methionine; ESCs, embryonic stem cells; METTL5, methyltransferase Like 5; ZCCHC4, zinc finger CCHC-type containing 4; TRMT112, tRNA methyltransferase subunit 11–2; FTO, fat mass and obesity-associated protein; ALKBH5, AlkB Homolog 5; HNRNP, nuclear heterogeneous ribose protein; eIF, eukaryotic initiation factor; MEFs, mouse embryonic fibroblasts; IGF2BP1, insulin-like growth factor 2 mRNA-binding protein 1; imDCs, immature DCs; maDCs, mature DCs; TLR4, toll-like receptor 4; NF-κB, nuclear factor-κB; CCR7, C-C chemokine receptor 7; HIF-1α, hypoxia-inducible factor 1α; SOCS, suppressor of cytokine signaling; STAT1, signal transducer and activator of transcription 1; CISH, cytokine Inducible SH2 Containing Protein; VHL, von Hippel–Lindau; GAPDH, glyceraldehyde-3-phosphate dehydrogenase; ICOS, inducible T Cell Costimulator; ISCs, intestinal stem cells; IECs, intestinal mucosal epithelial cells; MeRIP-seq, methylated RNA immunoprecipitation sequencing; YAP-1, Yes-associated protein 1; SOX2, sex-determining region Y-box 2; SOX4, SRY-related high-mobility group box 4; EMT, epithelial-mesenchymal transformation.

Conclusion

Extensive modification is a general code of RNA and the basis of its structure and catalytic function but remains largely uncharted territory. Silencing of m6A methyltransferase can significantly affect gene expression and other splicing patterns, leading to regulation of the p53 signaling pathway and apoptosis.18 Large numbers of studies have confirmed that m6A-related genes and different regulatory factors are positively or negatively regulated in the progression of CRC through a variety of mechanisms, which can be used as promising biomarkers for early diagnosis and prognosis as well as therapeutic targets. On the other hand, there has been very little research on IBD, so the general understanding of its relationship with m6A methyltransferase remains limited. However, given that m6A has been found to play an important role in intestinal mucosal immunity and colitis, future studies should pay more attention to the role of m6A in IBD, to lay a solid theoretical foundation for clinical diagnosis and possible cure for IBD, and to reduce the risk of CRC. The study of epigenetic modification represented by m6A in influencing RNA function and metabolism, cell physiological function, and the important role of abnormal modification in a variety of diseases should also receive extensive attention and exploration.