The mechanisms of action of the MTA2 protein are as follows (Fig. 2).

BC remains a major global health challenge due to its complex pathogenesis and varied clinical presentations, which hinder effective treatment and prevention (50-53). In BC, MTA2 primarily exerts its functions by regulating cytoskeletal reorganization and the Rho/Rho associated coiled-coil containing protein kinase (ROCK) signaling pathway. MTA2 inhibits Rho GTPase dissociation inhibitor α (RhoGDIα), thereby activating Rho GTPases such as RhoA and enhancing downstream ROCK activity (16). This activation promotes actin restructuring and lamellipodia formation, conferring amoeboid-like motility to breast cancer cells and significantly increasing migration and invasion. Reintroducing RhoGDIα or administering ROCK-specific inhibitors suppresses the MTA2-induced migration phenotype (11). In ERα-negative breast cancers, MTA2 expression undergoes reciprocal regulation by the Rho pathway: RhoGDIα overexpression reduces MTA2 protein levels, while MTA2 upregulation inhibits RhoGDIα, forming a positive feedback loop (16). In ERα-positive breast cancers, MTA2 overexpression is frequently accompanied by RhoGDIα downregulation. This is linked to tamoxifen resistance and increased anchorage-independent growth (15).

The antitumor small molecule MEQ directly binds MTA2, disrupting its interaction with the Mi-2/NuRD complex. This lifts repression of the seryl-tRNA synthetase (SerRS) gene and inhibits vascular endothelial growth factor A (VEGFA)-driven angiogenesis (54).

In BC, MTA1 overexpression reduces MTA2 protein levels without affecting mRNA. MTA1 induces activation of neutrophil elastase, which cleaves the C-terminal region of MTA2 at residues 486, 497, 542, 583 and 621, leading to MTA2 degradation. This antagonism partially explains why MTA1 can inhibit metastasis, whereas MTA2 promotes it (55).

GC is a significant global health concern (56). It ranks as the fifth most prevalent cancer and the third leading cause of cancer-related mortality worldwide, with >1 million new cases annually (57,58). MTA2 contributes to GC progression via several mechanisms. As a transcriptional regulator, MTA2 binds the promoter of minichromosome maintenance complex component 5, enhancing GC cell proliferation and metastatic potential (59). Overexpression of MTA2 promotes clonogenic formation and tumorigenesis in vivo, partly through activation of the downstream interleukin-11 (IL-11) pathway (60).

MTA2 preferentially binds DNA replication origins. This exacerbates olaparib-induced replication stress and renders BRCA-wild-type GC cells more sensitive to poly(ADP ribose) polymerase (PARP) inhibition, supporting targeted clinical use of PARP inhibitors in selected GC groups (61).

Circular RNA (circ)MTA2 binds the deubiquitinating enzyme ubiquitin C-terminal hydrolase L3 (UCHL3), preventing ubiquitination and degradation of the MTA2 protein. This stabilizes MTA2 and promotes tumor progression; the axis can be transmitted via exosomes (62). Conversely, long non-coding (lnc)RNAs in the small nucleolar RNA host gene family (SNHGs) retain MTA2 in the cytoplasm, preventing NuRD complex formation. This elevates acetylation of histone H3 and p53 and suppresses GC-cell proliferation and metastasis (63).

Liver cancer poses a significant global health challenge, with projections indicating it will impact >1 million individuals each year by 2025. HCC accounts for 90% of primary liver cancers and ranks as the fourth leading cause of cancer-related mortality globally (64-66). MTA2, an integral part of the NuRD complex, suppresses the transcription of target genes by facilitating histone deacetylation and independently regulates gene expression without relying on transcription factors. Immunohistochemical analysis reveals significantly elevated MTA2 expression in HCC tissues, primarily localized to the nucleus. Analysis of The Cancer Genome Atlas database further confirms markedly elevated MTA2 mRNA levels in HCC. Furthermore, MTA2 expression correlates with increased α-fetoprotein (ATP) levels in patient cohorts, suggesting a potential association with HCC recurrence (67).

Research indicates that MTA2 accelerates the growth, proliferation and metastasis of HCC cells by inhibiting the Hippo signaling pathway through suppression of genes such as FERM Domain Containing 6 (FRMD6). The MTA2/FRMD6/Hippo signaling axis plays a crucial role in HCC development and progression (68).

RC ranks as the third most prevalent cancer type worldwide and is the second leading cause of cancer-related mortality, comprising one-third of these cases (69). Despite a general decline in colorectal cancer incidence and mortality, RC rates among individuals under 50 years of age are rapidly increasing, with projections indicating a 124.2% rise for those aged 20 to 34 by 2030 in the United States (70-72). In RC, the biological function of MTA2 is precisely regulated through post-translational modifications. Among these, acetylation at lysine 152 mediated by the histone acetyltransferase p300 significantly enhances the oncogenic activity of MTA2, promoting proliferation, migration and invasion in RC cells. Conversely, mutations at this site inhibit RC cell growth and attenuate the migration and invasion capabilities of Rat-1 fibroblasts (73).

At the level of the immune microenvironment, RC progression is also regulated by MTA2. Tumor-infiltrating monocytes secrete human beta-defensin 3 (hBD-3) and inhibit cancer cell migration through a paracrine mechanism. This inhibitory effect is closely associated with downregulation of MTA2 mRNA. Importantly, hBD-3 does not directly inhibit cancer cell proliferation (74).

CC, primarily caused by persistent high-risk human papillomavirus (HR-HPV) infection, is a major cause of mortality among women globally and in the United States (75). CC remains a significant public health issue, with ~600,000 new cases and 300,000 deaths annually, making it the fourth most prevalent cancer type among women (76). MTA2 promotes tumor metastasis by negatively regulating kallikrein-related peptidase 10 (KLK10) expression and activating the microRNA (miR)-7/specificity protein 1 (Sp1) signaling axis. MTA2 is highly expressed in CC tissues, while KLK10, a known inhibitor of tumor migration, shows a significant negative correlation with MTA2 levels. Knockout of MTA2 leads to marked upregulation of KLK10. Concurrently, downregulation of MTA2 activates miR-7, which suppresses the activity of transcription factor SP1, forming a multilevel cascade regulatory network. Within this network, SP1 undergoes both direct regulation by MTA2 and indirect suppression by miR-7. Together, these factors act on downstream targets to influence the migratory capacity of CC cells (77).

Additionally, MTA2 exhibits synergistic carcinogenic effects with the calcium-calcium-phospholipid-binding protein copine 1 (CPNE1) in CC. MTA2 and CPNE1 expression levels show a significant positive correlation (r=0.668, P<0.01), suggesting they may act through shared signaling pathways to promote tumorigenesis and progression (78).

Lung cancer is the most common cause of cancer-associated death worldwide, with an estimated 1.6 million deaths each year (79,80). NSCLC accounts for ~85% of lung cancer cases, with lung adenocarcinoma and lung squamous cell carcinoma being the predominant subtypes (81). NSCLC is characterized by significantly elevated MTA2 expression. Research confirms that a specific antibody targeting MTA2 effectively blocks proliferation, migration and invasion in NSCLC cells. Further findings reveal that MTA2 activation is closely associated with enhanced activity in the extracellular signal-regulated kinase (ERK)/AKT signaling pathway and the VEGF pathway, while inhibition of MTA2 expression markedly reduces the phosphorylation levels and signaling efficiency of key molecules within these pathways. Silencing MTA2 reduces phosphorylation of ERK and AKT, significantly inhibiting NSCLC cell growth and invasiveness (82).

MTA2, a crucial part of the NuRD complex, plays dual roles in tumor progression. During the primary lung tumor stage, MTA2 negatively regulates NF-κB signaling independently of inhibitor of NF-κB kinase subunit beta (IKK2), thereby inhibiting tumor growth (83). However, when tumors progress to the metastatic stage, MTA2 dissociates from NF-κB target gene promoters and shifts to positively regulating NF-κB in an IKK2-dependent manner, thereby promoting EMT and cancer metastasis (83).

MTA2 is essential for maintaining the malignant phenotype of lung cancer and is highly expressed in invasive lung cancer cells. At the molecular level, MTA2 directly binds to the promoter regions of epithelial markers such as epithelial cell adhesion molecule (EPCAM) and cadherin 1 (CDH1), thereby suppressing the transcription of these genes and inducing EMT and tumor metastasis. Functional experiments demonstrate that MTA2 overexpression suppresses the promoter activity of CDH1 or EPCAM, whereas its deletion enhances the activity of these promoters (84). This stage-dependent dual role (tumor-suppressive in primary lesions, oncogenic in metastatic stages) indicates MTA2 function is highly context-dependent, regulated by NF-κB signaling and IKK2 dependency. Such stage-dependent dual functions of MTA2 in NSCLC are further fine-tuned by competitive dynamics between MTA2 and other MTA paralogs, where altered MTA1 abundance can displace MTA2 from NuRD complexes and reshape NF-κB-dependent tumor phenotypes in a context-specific manner.

Head and neck cancer, which arises in the lining or mucosa of the upper aerodigestive tract, specifically the oral cavity, oropharynx, larynx, hypopharynx and paranasal sinuses, is the seventh most common cancer type worldwide (85).

Oral squamous cell carcinoma (OSCC) significantly contributes to the morbidity and mortality associated with head and neck squamous cell carcinoma (86,87). Although there have been recent advancements in surgical methods, adjuvant therapy, molecular targeted therapy and immunotherapy, the outcomes remain inadequate (88). Studies on OSCC reveal that MTA2 enhances oral cancer cell migration and invasion by reducing the expression of autophagy markers light chain 3-II and phosphorylated cofilin. Suppression of MTA2 expression via gene knockdown markedly reverses these malignant phenotypes (89). At the regulatory level, lncRNA HOTAIR functions as a competitive endogenous RNA. By binding to miR-326, it relieves miR-326-mediated translational repression of MTA2 mRNA, thereby indirectly upregulating MTA2 expression. This HOTAIR/miR-326/MTA2 axis shows a significant positive correlation with EMT in OSCC, suggesting a pivotal role in tumor progression (90). Nasopharyngeal carcinoma (NPC) is an epithelial cancer originating from the mucosal lining of the nasopharynx (91). Tumors in the nasopharynx are frequently located at the pharyngeal recess. NPC exhibits a unique geographic distribution, being notably common in East and Southeast Asia (92). In NPC pathogenesis, MTA2 is directly targeted and regulated by miR-148b. miR-148b is notably downregulated in NPC and suppresses MTA2 expression by targeting the 3'-UTR of MTA2 mRNA to inhibit its translation. Restoration of miR-148b expression significantly inhibits NPC cell proliferation, migration, and invasion. Reintroduction of MTA2 partially counteracts the tumor-suppressive effects mediated by miR-148b, indicating that miR-148b exerts its antitumor activity in part by inhibiting MTA2 (93). Furthermore, analysis across ethnic groups reveals that in Han Chinese patients with NPC, MTA2 expression negatively correlates with patient age, with no significant association with clinical stage or lymph node metastasis. In Zhuang patients, MTA2 expression shows no correlation with clinical indicators (94).

Globally, esophageal cancer ranks as the ninth most prevalent cancer and the sixth leading cause of cancer-related mortality (95). The two primary histological subtypes, ESCC and esophageal adenocarcinoma (EAC), exhibit notable geographical distribution differences (96,97). ESCC is the most prevalent type, commonly found in developing countries, with its incidence declining in developed nations (98). Research on ESCC has identified a regulatory positive feedback loop between eukaryotic initiation factor 4E (EIF4E) and Twist in controlling EMT. MTA2 binds to EIF4E, which subsequently increases the expression of Twist, a crucial EMT regulator. Twist recruits MTA2 to the E-cadherin gene promoter, suppressing its transcription by decreasing histone acetylation. This positive feedback loop significantly promotes the metastatic process in ESCC (99).

Conversely, the lncRNA SNHG5 binds directly to the MTA2 protein, preventing its nuclear translocation and facilitating its degradation through ubiquitination. Furthermore, overexpression of SNHG5 can downregulate MTA2 expression at the transcriptional level. In esophageal cancer, downregulation of SNHG5 leads to abnormal accumulation of MTA2 protein, thereby accelerating the EMT process (100).

PDAC ranks as the fourth most common cause of cancer-related mortality in developed nations (101). By 2030, PDAC is projected to become the second leading cause of cancer-related mortality in the United States (102,103). Research on PDAC indicates that MTA2 recruits Snail protein and interacts with HDAC1 at the PTEN promoter, forming a transcriptional repression complex. The complex suppresses PTEN expression via histone deacetylation, diminishing negative regulation of the PI3K/Akt pathway and thereby enhancing PDAC cell proliferation, migration and invasion (104). Experimental evidence shows that benzyl isothiocyanate (BITC) treatment of MIA Paca-2 and PANC-1 cell lines leads to a dose- and time-dependent reduction in MTA2 expression, along with increased PTEN expression and reduced phosphorylated PI3K and AKT levels (105).

Research shows that MTA2 and HIF-1α create a positive feedback loop under hypoxic conditions. HIF-1α binds to the hypoxia response element (HRE) in the MTA2 promoter, boosting MTA2 transcription. Concurrently, the MTA2-HDAC1 complex deacetylates HIF-1α, increasing its protein stability. Activated HIF-1α further recruits MTA2 to the E-cadherin promoter region, suppressing the expression of this epithelial marker and driving the EMT process (106).

RCC accounts for 2-3% of all malignant diseases in adults. It ranks as the seventh most prevalent cancer in men and the ninth in women. Globally, there are ~209,000 new cases and 102,000 deaths annually (107). The rising incidence of all stages of this cancer over the years has led to a continuous increase in population-based mortality rates (108-110). Previous studies have confirmed that MTA2 negatively regulates miR-133b expression, thereby weakening the latter's binding to and inhibition of the 3' untranslated region of MMP9 mRNA. This ultimately promotes MMP9 expression, further enhancing the migration and invasive capacity of RCC. Research indicates that reducing MTA2 expression significantly inhibits RCC migration, invasion and metastatic potential in vivo, without appreciably affecting cell proliferation. In RCC cells with low MTA2 expression, the enzymatic activity, protein levels and mRNA transcription levels of MMP9 are all reduced (111). Another study indicated that melatonin combined with sorafenib synergistically reduces MTA2 expression, effectively inhibiting cancer cell migration and invasion in RCC cells (112).

Gliomas, comprising 81% of central nervous system malignancies, are the most prevalent primary brain tumors. Gliomas arise from neuroglial progenitor cells (113), evolving into astrocytoma, oligodendroglioma, ependymoma or oligoastrocytoma (114,115). The World Health Organization (WHO) classifies gliomas into four grades: Grades 1 and 2 are low-grade, while grades 3 and 4 are high-grade gliomas (HGG) (116). During the development of malignant gliomas, MTA2 expression is directly negatively regulated by miR-548b. This miRNA targets the 3'-UTR of MTA2 mRNA, leading to its degradation or translational inhibition, thereby decreasing MTA2 expression. Experimental evidence shows that miR-548b overexpression decreases MTA2 protein levels, thereby inhibiting glioma cell proliferation and invasive capabilities. Further rescue experiments demonstrate that restoring MTA2 expression can counteract the tumor-suppressive effects mediated by miR-548b (117).

Additionally, MTA2 participates in the progression of glioma by regulating cell-cycle processes. Research shows that significantly lowering MTA2 expression hinders the proliferation, migration and invasion of human glioblastoma cell lines GBM8401 and Hs683 and induces cell-cycle arrest at the G0/G1 phase. MTA2 expression was notably elevated in GBM8401 and Hs683 cells compared to other glioma cell lines, including M059J, M059K and U-87MG, at both the mRNA and protein levels. MTA2 expression in glioma tissues significantly correlates with tumor grade (P<0.001), indicating its potential as a biomarker for disease progression (49).

Osteosarcoma, the most prevalent primary malignant bone tumor, is characterized by malignant mesenchymal cells that produce osteoid or immature bone. It has a global incidence of about one to three cases per million annually (118,119). It mainly occurs in children and teenagers, with another increase in cases seen in individuals aged >50 years (120). Research on osteosarcoma has identified that MTA2 regulates urokinase-type plasminogen activator (uPA) expression through the ERK1/2 signaling pathway, significantly enhancing the migration and invasion of osteosarcoma cells. Experimental results indicate that knocking down MTA2 downregulates uPA expression and inhibits the formation of pulmonary metastatic lesions. Notably, treatment of MTA2-knockdown osteosarcoma cells with recombinant human (rh)-uPA leads to a marked recovery in migration and invasion capabilities (121).

In non-neoplastic diseases, earlier findings indicate that MTA2 regulates the plasticity of intestinal cell lineages. It acts synergistically with SATB homeobox 2, a protein that binds specifically to AT-rich sequences, to maintain the stability of colonic cell identity. Further studies indicate that MTA2 and hepatocyte nuclear factor 4α (HNF4A) co-occupy DNA on colonic chromatin. In the absence of MTA2, HNF4A detaches from colonic chromatin and binds to small intestinal chromatin, leading to the activation of genes involved in lipid absorption. This promotes functional lipid uptake processes and ultimately drives the transformation of colonic cells toward a small intestinal phenotype. This mechanism highlights the central role of MTA2 in tissue-specific enhancer regulatory networks (122).

In the epididymal epithelial cells of the male reproductive system, MTA2 was found to colocalize with ERα in the nucleus. By inhibiting the transactivation function of ERα, it participates in regulating the luminal microenvironment homeostasis essential for sperm maturation (123). MTA2 expression is notably increased in testicular Sertoli cells during the phagocytosis of apoptotic spermatogenic cells, leading to the transcriptional suppression of the follicle-stimulating hormone (FSH) receptor (FSHR) gene (124). This FSH/MTA2/FSHR negative feedback loop is crucial for maintaining the integrity of spermatogenesis by sustaining normal phagocytic function in supporting cells through the reduction of circulating FSH levels (125).

The MTA2/NuRD complex modulates the expression of crucial genes, including immunoglobulin lambda-like polypeptide 1 and V-set pre-B cell surrogate light chain 1, in pre-B cells during B-lymphocyte development by interacting with transcription factors IKAROS family zinc finger 3 (AIOLOS, IKZF3) and IKAROS family zinc finger 1 (IKAROS, IKZF1). The absence of MTA2 increases histone H3 lysine 27 acetylation (H3K27ac) at gene promoter regions, disrupting B-cell differentiation. This results in developmental defects in pro-B cells, immature B cells and marginal zone B cells, as well as abnormal differentiation of germinal center B cells (126).

MTA2 and MTA3 collaboratively maintain pluripotency in human embryonic stem cells by repressing genes linked to mesodermal differentiation. Studies show that ID8, an inhibitor targeting dual-specificity tyrosine phosphorylation-regulated kinases (DYRKs), partially mitigates the differentiation phenotype resulting from MTA2 or MTA3 knockdown. This effect is primarily mediated by inhibiting DYRK4 activity, suggesting that DYRK4 may function downstream of MTA2 or MTA3 in this pathway (127).

Collectively, MTA2 functions as a conserved epigenetic and metastatic driver across nearly all human cancers examined. All tumor types share core MTA2-mediated mechanisms, including NuRD complex-dependent transcriptional repression, induction of EMT, enhancement of MMP activity and non-coding RNA-mediated regulation. However, tissue-specific pathogenic mechanisms are evident: BC relies on Rho/ROCK cytoskeletal signaling; digestive system malignancies converge on epigenetic silencing, hypoxia/HIF-1α loops and mTOR pathway dysregulation; NSCLC uniquely exhibits stage-specific biphasic NF-κB regulation; gynecologic and urologic tumors act through distinct miRNA-MMP axes; head and neck cancers feature ceRNA crosstalk and ethnicity-associated expression patterns; and glioma and osteosarcoma are characterized by aberrant cell-cycle control and ERK/uPA-driven invasion. By contrast, MTA2 contributes to non-neoplastic homeostasis by maintaining lineage stability, reproductive function, immune development and stem cell pluripotency, representing a fundamentally distinct role from its oncogenic activity. This combination of shared core machinery and tissue-specific effector pathways defines the multifaceted landscape of MTA2-mediated pathogenesis.

In BC targeted therapy, small-molecule inhibitors such as MEQ, which target the MTA2-NuRD complex, can restore the expression of tumor suppressor genes such as SerRS, thereby inhibiting tumor angiogenesis (54). Furthermore, disrupting the interaction between MTA2 and amplified in breast cancer 1 (AIB1) can upregulate E-cadherin, partially reversing EMT (128). Enhancing miR-589 expression or altering the TTC39A-AS1/miR-483-3p/MTA2 signaling pathway markedly decreases MTA2 levels, suggesting a promising therapeutic approach for triple-negative BC (129,130). In ER+ BC, the synergistic inhibitory effect mediated by MTA2 and AIB1 indicates that therapy should be combined with endocrine strategies (128). Additional evidence indicates that knocking out the MTA2 gene increases tumor-cell sensitivity to chemotherapeutic drugs and induces apoptosis (131). In ER+ BC, the presence of the MTA2-AIB1 complex may predict resistance to endocrine therapy (128).

In targeted strategies for GC, epigenetic modulators targeting the MTA2-HDAC1 complex (e.g., HDAC inhibitors) may reverse the malignant phenotype of GC. MTA2 expression may also serve as a biomarker for predicting the efficacy of PARP-inhibitor therapy, such as Olaparib; when used with ataxia-telangiectasia and Rad3-related (ATR) inhibitors, this approach increases tumor-cell sensitivity and treatment effectiveness (61). Furthermore, disrupting the circMTA2/UCHL3/MTA2 signaling axis may offer novel strategies for curbing GC progression, particularly by targeting exosome-mediated intercellular communication. This approach also lays the groundwork for developing targeted inhibitors and designing combination regimens (62). The natural inhibitory molecules SNHG5 (132) and miR-1236-3p exert antitumor effects by regulating MTA2; their analogues or overexpression techniques may represent novel avenues for GC gene therapy (63,133). Combined detection with HDAC1 may further enhance prognostic accuracy (134).

In HCC targeted-therapy research, intervention strategies targeting MTA2 show potential value. MK-886 interacts with MTA2 through α-alkyl and alkyl interactions, leading to significant inhibition of HepG2 cell growth and dose-dependent apoptosis (135). Additionally, small interfering (si)RNA targeted at focal adhesion kinase (FAK) or FAK inhibitors (PF-573228) exhibit synergistic effects in the context of low MTA2 expression, jointly inhibiting MMP7-mediated invasion and metastasis (136).

For prognosis in HCC, MTA2 shows significantly higher expression in tumor cells, and its upregulation is closely linked to poor clinical outcomes, with both MTA2 and the proliferation marker Ki-67 markedly higher than in adjacent normal tissue. Nuclear MTA2 expression is positively correlated with Ki-67 (P=0.019). Furthermore, patients with HCC with elevated MTA2 display immune-microenvironment features marked by higher levels of activated CD4+ T cells and M0-type macrophages, indicating that immune regulation may contribute to tumor development (135).

In targeted therapy for RC, acetylation-focused interventions have gained attention. Inhibiting acetylation at K152 of MTA2 (e.g., with p300-specific inhibitors) may block its tumor-promoting functions, effectively suppressing tumor growth and metastasis (73). Preclinical models indicate that targeting lncRNAs in exosomes with antisense oligonucleotides or siRNA directed at the prostate cancer-associated transcript 1 (PCAT1)/ZNF217 (zinc finger protein 217)/MTA2 pathway may inhibit EMT and metastasis (137). In immune regulation, analogues or inducers of hBD-3 may suppress tumor cell migration by downregulating MTA2, offering a potential approach for metastatic disease in advanced RC (74). Small-molecule inhibitors that disrupt the MTA2-EZH2 interaction may restore TSC2 expression and suppress mTOR pathway activation, showing therapeutic potential in RC (36).

Studies of therapeutic targets for CC show that small-molecule inhibitors, such as p38 kinase inhibitors, can hinder the MTA2/MMP12 pathway. This disruption affects activator protein-1 (c-Fos/c-Jun) binding to the MMP12 promoter by interfering with phosphorylation of Y-box binding protein 1 (YB1), ultimately suppressing MMP12 expression and reducing metastatic potential (138). Additionally, oligonucleotide agents targeting the miR-7/SP1 pathway have shown therapeutic potential; these may reverse MTA2-mediated metastasis by promoting KLK10 expression, informing combination strategies (77). In molecular subtyping and personalized therapy, a positive correlation between MTA2 and CPNE1 expression in patients with HR-HPV (types 16 and 18) may serve as an additional marker for individualized treatment (78,139).

For prognosis, high MTA2 expression is associated with malignant progression. Positive expression rates are 0% in normal cervical tissue, ~30% in cervical intraepithelial neoplasia (CIN) and up to 73.4% in cervical squamous cell carcinoma. Expression correlates with International Federation of Obstetrics and Gynecology stage and lymph node metastasis (140).

Targeting MTA2 shows promise for NSCLC. Small-molecule inhibitors aimed at the MTA2-ERK/AKT/VEGF axis (e.g., AbMTA2) in vivo effectively suppress tumor growth, and siRNA-mediated MTA2 knockdown significantly inhibits proliferation (82). HDAC inhibitors targeting the MTA2-NuRD complex may relieve repression of tumor suppressors such as E-cadherin, facilitating re-epithelialization (84). Strategies may be stage-specific: During the primary phase, enhance the inhibitory effect of MTA2-NuRD on NF-κB signaling; at the metastatic stage, block the IKK2-MTA2 interaction (83). Meanwhile, MTA1 antagonizes MTA2 by promoting its degradation, and competitive dynamics within the NuRD complex further determine MTA2's pro- or anti-tumor activity. This inter-MTA competitive balance is highly disease- and stage-specific, making NuRD functional outputs and therapeutic responses distinct in NSCLC compared with other cancer types.

Targeting ceRNA networks shows promise. Antisense oligonucleotides or synthetic miR-326 mimics that suppress HOTAIR and restore miR-326 can disrupt the HOTAIR/miR-326/MTA2 axis, markedly reducing MTA2 and inhibiting EMT (90). Clinically, MTA2 levels in OSCC tissues are higher than in adjacent normal mucosa (P<0.01). Overexpression is associated with higher histological grade (P<0.01), underscoring MTA2's value for assessing OSCC progression and prognosis (90).

In NPC, miRNA-targeted therapy restoring or mimicking miR-148b suppresses MTA2 pathway activity and exerts antitumor effects (93). Given ethnic differences in MTA2 expression, treatment can be optimized. For patients of Zhuang ethnicity with lower MTA2 expression, carboplatin plus fluorouracil often yields more favorable outcomes. MTA2 expression also has prognostic value. In Zhuang patients with NPC and low MTA2 expression, the specified chemotherapy regimen notably enhances overall survival (OS) (hazard ratio=0.42, P<0.05) (94).

Targeting the EIF4E/TWIST signaling pathway is a promising strategy for ESCC. Designing small-molecule inhibitors to disrupt the MTA2-EIF4E interaction could block TWIST-mediated upstream EMT events and reduce metastatic foci (99). Epigenetic regulation is another route: Applying SNHG5 analogs or overexpression vectors promotes MTA2 ubiquitination and degradation, significantly inhibiting proliferation, migration and invasion in ESCC cells. This approach reverses the EMT phenotype and restores epithelial characteristics (100).

In PDAC treatment strategies, intervening through epigenetic regulation by using small-molecule inhibitors (such as structural analogues of BITC) to target the interaction between MTA2 and HDAC1 can restore PTEN expression. In preclinical experiments, this intervention significantly reduces tumor volume (105). MTA2 is a central component and potential therapeutic target in the regulatory network of the hypoxic tumor microenvironment, crucial for inhibiting PDAC progression and metastasis. Blocking the MTA2-HIF-1α signaling axis using antisense oligonucleotides or specific inhibitors effectively suppresses metastasis formation, offering a therapeutic option for patients with advanced PDAC (106).

Prognostic evaluations indicate that MTA2 expression is significantly elevated in PDAC tissues compared to adjacent normal tissues (P<0.01), with a positive correlation between its expression intensity and tumor grading (105).

In RCC, combined targeted strategies show potential. Melatonin plus sorafenib synergistically downregulates MTA2 expression and attenuates migration and invasion of RCC cells (112). miRNA-based interventions are also feasible. Restoring miR-133b or developing its analogs can block the MTA2-MMP9 axis and inhibit RCC metastasis (111). From a prognostic perspective, MTA2 expression is significantly higher in RCC tissues than in adjacent normal tissues (P<0.01). MTA2 overexpression is associated with higher tumor grade (P=0.002) and advanced TNM stage (P<0.001), indicating its potential as a prognostic biomarker (112).

In miRNA-targeted therapy for glioma, restoring or mimicking miR-548b inhibits the MTA2 pathway and exerts antitumor effects. miR-548b overexpression markedly suppresses growth of U-87MG xenografts (117). In clinical samples, MTA2 expression is higher in HGG (e.g., GBM8401 and Hs683) than in low-grade lines (e.g., M059J, M059K and U-87MG). MTA2 levels positively correlate with WHO grade (P<0.001), supporting its potential as an auxiliary marker of malignancy (49).

In clinical treatment strategies for osteosarcoma, interventions targeting the uPA signaling pathway demonstrate potential value. It has been indicated that rh-uPA treatment of MTA2-low osteosarcoma cells significantly reverses the suppression of their migration and invasion. Correspondingly, the application of small-molecule inhibitors targeting the MTA2/uPA axis markedly reduces the number of lung metastases. Furthermore, combining these inhibitors with ERK pathway inhibitors holds promise for further enhancing the suppression of tumor metastasis (121). In the prognostic analysis of patients with osteosarcoma, elevated MTA2 expression correlated significantly with advanced tumor stages (P<0.01). In vivo experiments also confirmed that reducing MTA2 expression markedly suppressed tumor metastatic activity and the formation of pulmonary nodules (121).

Research indicates that the MTA2/HNF4A signaling axis may serve as a therapeutic target for inflammatory bowel disease and short bowel syndrome. Modulating this pathway may enable colonic epithelial cells to acquire small-intestine-like absorptive properties, thereby improving nutritional deficiencies caused by malabsorption (122). Research on male infertility has revealed that abnormalities in the FSH/MTA2/FSHR negative-feedback regulatory pathway are associated with impaired spermatogenesis. Developing drugs targeting this pathway may correct defects in the phagocytic clearance function of supporting cells, offering a therapeutic strategy for such infertility conditions (125). Additionally, the study revealed that MTA2 interacts with ERα in the epididymis through a transactivation mechanism, offering insights for developing selective ER modulators to help maintain male reproductive function (123).

It should be noted that the current understanding of MTA2 in non-neoplastic diseases remains relatively limited compared with its well-established roles in various malignant tumors. Most existing studies have concentrated on the oncogenic functions of MTA2 in cancer initiation, progression and metastasis, whereas investigations into its physiological and pathological roles in non-neoplastic conditions are still in the preliminary stage with relatively scarce clinical and translational evidence. Therefore, the coverage of non-neoplastic diseases in this review is appropriately concise, while future studies are warranted to further explore the clinical and translational potential of MTA2 in these non-oncological contexts.

In summary, MTA2 serves as a pan-cancer prognostic biomarker and a broadly actionable therapeutic target, with conserved clinical value in predicting poor differentiation, lymph node metastasis and shortened survival across most malignancies. Common therapeutic strategies include disrupting NuRD assembly, inhibiting post-translational modifications, restoring regulatory miRNAs and blocking upstream regulatory axes. At the same time, tissue-specific clinical implications are critical: Digestive system tumors show unique sensitivities to PARP or HDAC inhibition; BC exhibits endocrine therapy resistance linked to MTA2; NSCLC requires stage-specific intervention; and head and neck, bone and brain tumors benefit from miRNA-based or ceRNA-targeted strategies. These conserved and distinct features highlight that MTA2-targeted diagnosis and therapy should be tumor-type-specific and mechanism-guided to maximize clinical efficacy.