EXOs are derived from intracellular bodies termed multivesicular bodies (MVBs) and are nanoscale extracellular vesicles, with a diameter of ~30 to 150 nm (15,16) and a density between 1.1 and 1.2 g/ml. They are found in various cell types and extracellular fluids, such as plasma, synovial fluid, urine, amniotic fluid, saliva, cerebrospinal fluid and breast milk (17-21). The cell membrane invaginates to form early endosomes, which turn into late endosomes under the control of various cellular signaling pathways (22-24). Stage 2 refers to the budding of late endosomes to form MVBs. Stage 3 of the process entails the amalgamation of MVBs with the plasma membrane, followed by the selective recruitment of cytoplasmic elements, including proteins, RNA and lipids, to form intact EXOs. The process of EXO formation is relatively complex and is regulated by a number of factors, such as tetraspanins, cholesterol, endosomal sorting complexes responsible for transport, sphingomyelinases and adhesion molecules, after which they are released into the microenvironment (25,26). When EXOs were first discovered, scholars considered them a way to expel unwanted components from cells (27). As research progressed, receptor-ligand interactions with EXOs, and direct membrane fusions for the delivery of biomolecules to target cells and mediate intercellular communications have been verified (28).

Exosomal vesicles are rich in lipids, proteins and various types of nucleic acids, such as DNA, mRNAs, microRNAs (miRNAs/miRs) and long non-coding RNAs, transcription factors and cytokine receptors. Organelles, such as ribosomes and mitochondria are typically absent. EXOs mediate cell-cell and cell-extracellular matrix (ECM) communications through the biologically active molecules within them to induce the necessary growth signals and transcriptional changes to cause phenotypic changes in the local environment (29,30). Various physiological and pathological mechanisms have been observed to exert an effect on recipient cells, including the amelioration of ischemic brain injury and the stimulation of angiogenesis, which leads to the acceleration of skin wound healing, thus holding promise as a potential therapeutic approach for addressing osteoarthritis (31-33). Depending on the cell type that produces the EXOs and changes in the cellular microenvironment, such as physiological and pathological states, the number of EXOs secreted and the composition of the contents of EXOs varies (34). For example, BMSC-derived EXOs (BMSC-EXOs) contain a variety of anti-inflammatory factors and growth factors, such as transforming growth factor-β (TGF-β), interleukin (IL)-10 and tumor necrosis factor (TNF)-stimulated gene ((TSG)-6 (35). It has been demonstrated that BMSC-EXOs contain miR-301a, miR-22 and miR-let-7, which are involved in immune-related pathways (36). Given their significant osmotic impact, EXOs possess the ability to traverse the blood-brain and blood-spinal cord barriers effectively. Moreover, they exhibit a selective propensity to infiltrate sites of inflammation within bodily tissues, thereby exerting regulatory control over the inflammatory response (37,38). In addition, the membrane transport process is involved in the production of EXOs. Several proteins that are closely related to this process, such as tetraspanins (CD9, CD63 and CD81), the membrane proteins, annexin and flotillin, heat shock proteins (HSP70 and HSP90) and markers of the endosomal sorting complex required for transport pathway, have been identified. Several proteins, including lysosomal-associated membrane protein 1 and TSG101, are highly enriched in various cell-derived EXOs (39). Therefore, they are often used as the marker proteins of EXOs and are widely used to extract and purify EXOs. The morphological and structural pattern of EXOs is illustrated in Fig. 1.

There are two types of TBI: Indirect insertion and direct insertion. For example, indirect insertion involves the insertion of the medial collateral ligament into the tibia. The ACL and RC are anatomical structures that are intricately integrated into the bone through a gradient structure comprising four consecutive layers of distinct tissue. These layers can be categorized from soft to hard, starting with the tendon, followed by noncalcified fibrocartilage, calcified fibrocartilage and ultimately bone tissue (40-42). Once the tendon-bone connection is damaged, restoring the natural anatomical structure is difficult (Fig. 2).

Tendon cells are responsible for synthesizing and secreting collagen, and are the basic units of tendon function. Healthy tendons primarily contain type I collagen, which provides mechanical strength and durability. Type II collagen is found in lower amounts and is typically concentrated where tendons connect to bones. Following a tendon injury, type III collagen is abundant in scar tissue and is crucial for tendon healing. An imbalance in type III and type I collagen in the tendons can cause mechanical damage. Notably, in addition to altering the phenotype and function of various cells, MSC-EXOs can also increase the content of type III collagen by increasing the level of TGF-β1, thus promoting tendon healing (43).

Tendon cells are closely associated with RC disease; studies have shown that they are involved in tendon repair through proliferation and migration (44). For example, tendon stem cell-derived EXOs induce tendon differentiation in mesenchymal stem cells via TGF-β (45), promote healing in injured tendons by balancing the synthesis and degradation of tendon extracellular matrix (6), and can regulate inflammation and promote high-quality healing of injured tendons (46).

TBI injuries are typically classified as acute and chronic. If not repaired in time, acute injury can gradually transform into chronic injury. The overuse or overload of tendons often leads to injury (42), while other factors such as age, metabolism and blood pressure can also exacerbate tendon injury (43). This condition severely affects the quality of life of affected individuals, and is a major cause of pain and disability (6). The distinguishing characteristics of the healing process between tendons and bones encompass the fusion of bone, heightened mechanical thresholds and the constricting of the bone tunnel (47,48). Tendon healing is divided into four phases: Inflammatory, proliferative, remodeling and maturation (49). During tendon healing, the levels of several growth factors, including TGF-β, platelet-derived growth factor, vascular endothelial growth factor (VEGF) and insulin-like growth factor-1, are increased and play critical roles in all stages of the recovery process (50).

TBI healing is very complex for several reasons. First, the region of fibrocartilage at the site of injury exhibits a deficiency in cells and blood supply, leading to a delayed or impaired healing process in TBI (51). Second, the regeneration of new bone is typically very slow, and strength and stiffness are correspondingly reduced (2). Third, during the healing of TBI, an initial inflammatory response occurs at the junction between the tendon and bone, and a large number of macrophages infiltrate, fibroblasts release extracellular matrix to form granulomas, and a large amount of collagen is deposited; the occurrence of fibrovascular scar tissue formation in the local area is a consequence that can be observed (52). In contrast to the initial anatomical arrangement, scar tissue has a significant impact on the process of new bone generation and the development of the interface between the tendon and bone. In comparison to the original physiological system, the presence of scar tissue has notable implications for the regeneration of new bone. The development of the tendon-bone interface and its ability to mediate load transmission and stress dispersion experiences a notable decline, which leads to decreased biomechanical properties in poorly regenerated tendons, impaired motor function, a shortened service life and a significantly reduced quality of healing (8,53).

Macrophages are derived from the bone marrow mononuclear cell line, are essential to the innate immune system and play an indispensable role in the immune response. Macrophages are divided into classically activated (M1) macrophages and alternately activated (M2) macrophages in response to various environmental stimuli. These two types of macrophages exhibit significant heterogeneity in phenotype and function. M1 and M2 macrophages are considered to have pro-inflammatory and fibrotic phenotypes, respectively (88,89). Previous studies have demonstrated that macrophages play a non-negligible role in the occurrence and development of TBI injury (90-92). In the early stages following tissue injury or tendon/ligament reconstruction, macrophages are recruited in large numbers to the graft-tunnel interface and are polarized toward the M1 type, inducing inflammatory responses and engulfing apoptotic cells, and removing cell debris (90). During this period, the expression of various pro-inflammatory factors, including TNF-α, IL-12, and inducible nitric oxide synthase, is significantly increased, thereby amplifying the inflammatory response in the affected area (90). The presence of inflammation in the surrounding environment helps attract additional cells from various locations to travel to the injured area and assist in the preparation of future tissue healing. In the advanced phase of the injury, M2 macrophages replace M1 macrophages in large numbers and secrete anti-inflammatory factors, such as IL-10 and TGF-β; by doing so, this decreases the localized inflammation and enhances the local regeneration and repair of tissues (93). Thus, accelerating macrophage polarization from M1 to M2 can accelerate tissue repair (94). If this is not achieved, it can lead to a prolonged inflammatory phase, increased apoptosis and decreased cell proliferation, resulting in slow healing. In addition, this condition can induce the excessive secretion of ECM by fibroblasts, leading to soft tissue fibrosis and scar tissue formation at the injury site, which hinders cartilage regeneration and graft remodeling (95-97). Therefore, regulating the polarization of macrophages may be key to promoting early tendon-bone healing.

Previous studies have reported that EXOs regulate inflammation through macrophage polarization, reduce cell infiltration and matrix deposition, promote collagen formation, and improve fiber continuity and alignment during tendon healing remodeling (46,98,99). In addition, EXOs derived from mesenchymal stem cells have been shown to modulate macrophage polarization in several in vitro and in vivo studies. For example, Huang et al (100) discovered that BMSC-EXOs were able to suppress inflammation by preventing the activation of M1 macrophages and the release of pro-inflammatory substances. Their study confirmed that BMSC-EXOs have the potential to enhance the fracture load and stiffness in the reconstructed RC, thereby inducing angiogenesis and inhibiting inflammation around RC endpoints, and promoting the healing of tendons and bones following RC reconstruction in rats. Li et al (8), in their groundbreaking study, demonstrated that BMSC-EXOs have the ability to induce the transformation of M1 macrophages into M2 macrophages through the involvement of miR-23a-3p. This finding suggests that early treatment with BMSC-EXOs may effectively suppress the inflammatory response at the interface between the tendon and bone. Furthermore, it was observed that BMSC-EXOs facilitated the regeneration of fibrocartilage and expedited the healing process of the tendon-bone junction following ACL reconstruction. Moreover, miR-23a-3p overexpression enhanced the therapeutic effect (8). Shi et al (101) demonstrated that BMSC-EXOs improved the inflammatory microenvironment and promoted fibrocartilage regeneration at the tendon-bone interface by increasing M2 macrophage polarization, thereby reducing the expression of the pro-inflammatory cytokines. IL-1β and IL-6. and enhancing the expression of the anti-inflammatory cytokines, IL-10, TGF-β and insulin-like growth factor during tendon healing. Furthermore, it is possible to enhance the biomechanical characteristics of the healing process between tendons and bones.

The characteristics of EXOs exhibit potential for reducing initial inflammatory reactions, which is necessary for effective tissue healing (102). However, the specific mechanism through which BMSC-EXOs control the polarization and function of M2 macrophages in TBI injury is not yet completely understood and warrants further investigation. The mechanisms of BMSC-EXOs in promoting tendon-bone healing are illustrated in Fig. 3.

After experiencing a traumatic brain injury, there is a decrease in blood flow to the area where the tendon connects to the bone. This decrease in blood flow means that important nutrients that are necessary for the healing of the tendon and bone are not being delivered properly. As a result, the biomechanical properties of the tendon and bone are negatively affected, which in turn affects the overall recovery of the tendon and bone (103). Numerous research studies have provided evidence that neovascularization plays a crucial role in facilitating the healing process of tendon-bone. It has been consistently demonstrated that following RC reconstruction, tendon-bone healing quality can be effectively improved by improving the blood supply at the tenodesis point or trough, where the blood supply is relatively poor (104).

VEGF is a key factor that regulates the natural formation of new blood vessels in the body. It plays a crucial role in activating, increasing in number and facilitating the movement of endothelial cells which line the inside of blood vessels and improve the circulation of blood to the transplanted tendon, which in turn facilitates the healing of the tendon-bone connection (103). Takayama et al (105) provided evidence that suppressing the expression of VEGF hindered the process of blood vessel formation and also hindered the mechanical integrity of tendon grafts following ACL reconstruction surgery. Furthermore, the overexpression of VEGF affected the enhancement of the biomechanical strength of tendon grafts (105). Huang et al (100) discovered that BMSC-EXOs have the ability to enhance the formation of new blood vessels around the area where the tendon and bone meet. Additionally, they found that these exosomes can increase the strength and rigidity of the tendon in rats following reconstruction, as well as stimulate the growth of the tendon-bone junction (100). During further mechanistic analyses, the researchers verified that BMSC-EXOs have the ability to stimulate the VEGF and Hippo signaling pathways. Additionally, they can enhance the growth, movement and formation of blood vessels in human umbilical vein endothelial cells in vitro (100). Notably, the researchers discovered that the stimulation of the VEGF and Hippo signaling pathways by BMSC-EXOs could be separate. This indicates that the activation of the Hippo signaling pathway by BMSC-EXOs does not solely rely on the VEGF signaling pathway. This suggests that BMSC-EXOs have extensive and beneficial impacts on enhancing angiogenesis (Fig. 4).

Bone is a dynamic tissue that undergoes continuous remodeling by a delicate equilibrium between the creation of new bone by osteoblasts and the breakdown of old bone by osteoclasts. The process of bone formation is carefully regulated and involves the direct transformation of BMSCs into osteoblasts. Following surgical reconstruction, up to 25% of patients require revision surgery, partly due to traumatic, technical, bacterial and biological factors. A significant factor contributing to this issue is the deterioration of bone surrounding the graft, which directly affects the secure connection of the transplanted tendon to the bone tunnel. Therefore, reducing bone loss around the graft may be a therapeutic strategy with which to promote tendon-bone tunnel healing and reduce the rate of reconstruction failure.

The healing quality of the grafted tendon-to-bone tunnel is closely related to the formation of bone around the graft, which is inseparable from early post-operative angiogenesis. The blood vessels located at the boundary between the transplanted tendon and the bone tunnel supply an ample amount of oxygen and nutrients to the cells. As a result, this has a direct impact on the formation of new bone around the graft (100,106). Zhang et al (107) examined a rat ACL reconstruction model and demonstrated that BMSC-EXOs promoted the formation of blood vessels around the graft and improved bone microstructure, which accelerated the healing of the transplanted tendon-bone tunnel following ACL reconstruction.

BMSC-EXOs can participate in bone remodeling by directly regulating the proliferation and activity of osteoblasts. Fang et al (108) found that BMSC-EXOs containing tsRNA-10277 altered the adipogenic and osteogenic potential of BMSCs. Zhang et al (109) found that miR-935-enriched EXOs produced by BMSCs directly enhanced osteoblast proliferation and activity by targeting signal transducer and transcription 1 activation to promote osteoblast proliferation and differentiation. In addition, miR-218, miR-196a and miR-181a contained in BMSC-EXOs have been confirmed to exert positive regulatory effects on osteoblast differentiation (110).

In addition to targeting osteoblasts, BMSC-EXOs can regulate the activity of osteoclasts, thereby regulating bone metabolism at the tendon-bone interface. Feng et al (111) demonstrated that EXOs containing a high amount of miR-6924-5p, derived from platelet derived growth factor receptor α (+) BMSCs overexpressing Scleraxis, could be used as a novel type of nanotherapeutic agent. These EXOs were able to prevent the formation of osteoclasts by targeting two specific proteins: Osteoclast stimulatory transmembrane protein and chemokine (C-X-C motif) ligand 1. In addition, this treatment could effectively hinder the process of tunnel osteolysis and enhance the biomechanical stability of tendon-bone healing (111).

Fibrocartilage is an essential component of the tendon-bone interface. Recently, Han et al (112) reported that BMP-2 and polylactic acid delivered by BMSC-EXOs in polyaspartic acid-polylactic acid-glycolic acid copolymer microcapsules promoted chondrogenic differentiation through the Smad/RUNX2 pathway, enhanced tendon interface stiffness and ultimate load strength, and promoted tendon-bone healing in rabbits with acute RC tears. BMSC-EXOs that have undergone low-intensity pulsed ultrasound stimulation (LIPUS) have the potential to enhance the regeneration of fibrocartilage at the interface between the tendon and bone. Additionally, they can help reduce the infiltration of fat in the supraspinatus muscle in a mouse model of RC repair. This is achieved by delivering miR-140 (113). Cai et al (114) reported that the local injection of EXOs derived from kartogenin-preconditioned BMSCs had the potential to efficiently stimulate the development of cartilage, enhance the maturation of collagen, and facilitate the regeneration of tissues in the rotator cuffs of rats with chronic RC tears, and enhance biomechanical properties following RC repair (Fig. 5).

The proliferation and migration of tendon cells are involved in tendon tissue repair and tendon-bone healing (115). Ample research has validated the positive impact of BMSC-EXOs in facilitating the restoration of tendons. For example, Yu et al (116) demonstrated that BMSC-EXOs promoted the proliferation, migration and tendon differentiation of tendon stem/progenitor cells (TSPCs) in vitro, and subsequent in vivo analyses further confirmed that BMSC-EXOs could be taken up and internalized by rat TSPCs, thereby promoting the proliferation and migration of TSPCs. This effect was characterized by improved histological scores of patellar tendons, the enhanced expression of Mohawk, tending-regulatory protein and type I collagen, and improved mechanical properties of the new tendons (116). Subsequent studies confirmed that exosomes derived from BMSCs promoted the proliferation, migration and fibrotic activity of rotator cuff tendon cells, and TGF-β1 was a key molecule that mediated the effect of exosomes (117). Pre-treatment of BMSCs with TGF-β1 can also significantly promote the secretion and release of EXOs from BMSCs. Li et al (118) first described that TGF-β1 treatment promoted BMSC-EXO secretion, and miR-29a promoted tendon cell proliferation, migration and fibrosis by targeting fatty acid binding protein 3, thereby improving tendon injury and RC tear. Several previous studies have shown that BMSCs-EXOs can promote skin wound healing by regulating the activation and proliferation of fibroblasts (119-121). Recently, Li et al (122) confirmed that BMSC-EXOs also play a critical role in promoting tendon-bone healing by promoting the proliferation and differentiation of fibroblasts. In addition, the downstream targets of miRNA, which is an active molecule in BMSCs-EXOs, have also been more fully verified in their study. According to the study conducted by Li et al (122), it was confirmed that miR-144-3p and miR-23b-3p enhanced the proliferation, migration and collagen synthesis of NIH3T3 fibroblasts through both bioinformatics analysis and in vitro experiments. Further analyses demonstrated that miR-144-3p and miR-23b-3p promoted fibroblast activation through the upregulation of the PTEN and PI3K/Akt signaling pathways (122). This discovery lays a theoretical foundation for RC tear therapy and provides a new avenue for further research (Fig. 6).