The Interplay between Autophagy and Mitochondria in Cancer

Besides producing cellular energy, mitochondria are crucial in controlling oxidative stress and modulating cellular metabolism, particularly under stressful conditions. A key aspect of this regulatory role involves the recycling process of autophagy, which helps to sustain energy homeostasis. Autophagy, a lysosome-dependent degradation pathway, plays a fundamental role in maintaining cellular homeostasis by degrading damaged organelles and misfolded proteins. In the context of tumor formation, autophagy significantly influences cancer metabolism and chemotherapy resistance, contributing to both tumor suppression and surveillance. This review focuses on the relationship between mitochondria and autophagy, specifically in the context of cancer progression. Investigating the interaction between autophagy and mitochondria reveals new possibilities for cancer treatments and may result in the development of more effective therapies targeting mitochondria, which could have significant implications for cancer treatment. Additionally, this review highlights the increasing understanding of autophagy’s role in tumor development, with a focus on modulating mitochondrial function and autophagy in both pre-clinical and clinical cancer research. It also explores the potential for developing more-targeted and personalized therapies by investigating autophagy-related biomarkers.


Introduction: The Function of Mitochondria
Mitochondria are often termed the "powerhouse" of the cell because of their ability to transform the energy contained in glucose or other organic molecules into adenosine triphosphate (ATP).
During cellular respiration, apart from ATP production (Figure 1), mitochondria primarily generate reactive oxygen species (ROS), mainly superoxide (O 2− ), due to electron leakage at complexes I and III [1].Under typical physiological conditions, mitochondria produce a modest level of mtROS (mitochondrial ROS), but in the presence of a mitochondrial dysfunction, the production of mtROS escalates uncontrollably.This excessive, unmanageable level of mtROS leads to modified mitochondrial redox signaling.Oxidative stress conditions within mitochondria are heralded by the impairment of the Krebs cycle, the degradation of mitochondrial proteins through their unfolding, also impacting cell death, mitochondrial DNA (mtDNA) mutations, and lipid damage [2].Moreover, mitochondrial oxidative stress induces the expression of genes that activate stress response pathways, including the activation of Nrf2 (nuclear factor erythroid 2-related factor 2).The Nrf2 transcription factor controls the expression of antioxidant response genes related to glutathione, thioredoxin, iron metabolism, and NADPH production.Disruption of mtDNA by mtROS can impair ETC function because mtDNA encodes 13 mRNAs for mitochondrial respiratory complexes, 22 tRNAs, and 2 rRNAs [3].The control of the accumulation and elimination of mtROS can be executed by either superoxide dismutase (SOD), NADPH oxidase (NOX), catalase (CAT), glutathione peroxidase (GSH-Px), or thioredoxin peroxidase (TRX-Px) [4].The effectiveness of GSH-Px and TRX-Px is contingent upon the presence of reduced glutathione (GSH) and reduced thioredoxin (TRX).The replenishment of GSH and TRX relies on the functionality of reductases and the quantity of their cofactor, NADPH.Additionally, mtROS can be eliminated through the controlled removal of mitochondria, known as mitophagy [2].

Autophagy
Originally, autophagy was defined as a cell survival mechanism that occurs under starvation or oxidative stress (hypoxia, ROS) conditions, wherein the cell degrades damaged or unnecessary organelles to generate nutrients.Recently, it was discovered that autophagy is involved in the quality control of organelles/proteins by degrading dysfunctional proteins/organelles.Autophagy is divided into selective and nonselective types.Nonselective autophagy is a process that transforms cellular energy by randomly removing organelles.In contrast, selective autophagy specifically targets damaged organelles, such as the ER, mitochondria, and peroxisomes, as well as cellular proteins.Nonselective autophagy is triggered under starvation or nutrient deprivation conditions, while selective autophagy is more prevalent in nutrient-rich environments [11].
It was recently reported that autophagic cell death (ACD) is likely an outcome of either extensive autophagy, prolonged stress, or inhibited apoptosis [12].During ACD, nuclear condensation increases, caspase activity decreases, and cellular vacuoles are generated [13].
Selective autophagy is a multistage process that includes the following steps: initiation, elongation, maturation, fusion, and degradation.Initiation (Figure 2A) commences with the activation of the ULK (Unc-51-like kinase) complex.This complex controls the commencement of selective autophagy by forming a stable protein assembly that includes ULK1/2 (serine/threonine Unc-51 like kinase 1/2), FIP200 (also known as RB1CC1), ATG13, and ATG101.Once this complex is formed, it initializes and regulates the formation of the pre-autophagosomal structure (PAS) and recruits ATG9 vesicles [14], which facilitate PAS expansion and are often referred to as the "seeds" of autophagosome formation [15].The activity of the ULK complex is regulated by leading regulators of nutrient stress sensors, namely, mechanistic target of rapamycin complex 1 (mTORC1) and AMP-activated pro- Mitochondria play crucial roles in maintaining calcium homeostasis, the reprogramming of metabolism to suit physiological needs, and the regulation of the cell and organelles' death.To maintain cellular homeostasis, mitochondria engage in communication with each other and with other organelles through various mechanisms, such as retrograde signaling, vesicular transport, signaling molecules, or direct interaction with the mitochondriaassociated membrane (MAM) of the endoplasmic reticulum (ER).Collaboration with ER supports mitochondria in regulating Ca 2+ transport, apoptosis, and phospholipids delivery.Additionally, cooperation with peroxisomes assists in fatty acid oxidation and the elimination of mtROS [5].The formation of a mitochondrial network occurs through the processes of the fission and fusion of both the outer (OMM) and the inner (IMM) mitochondrial membranes.A proper balance between mitochondrial fusion and fission is vital for ensuring effective cell metabolism and adaptation to stress.The fusion of mitochondria facilitates the mixing of mtDNA and enhances MMP, mitochondrial respiration, and ATP production.Conversely, mitochondrial fission regulates apoptosis and mitophagy [6].Furthermore, intact mitochondria possessing mtDNA are capable of transferring between cells via a mechanism termed horizontal mitochondrial transfer (HMT).The primary purpose of HMT is to share functional mitochondria with cells exhibiting aberrant mitochondrial functions.Consequently, cells receiving mitochondria restore mitochondrial respiration [3].
The ability of mitochondria to dynamically modulate and adapt cellular functions in response to stressful conditions is considered a pivotal factor in cancer development.
The key difference in cancer cells' mitochondria compared to those in healthy cells lies in the switching between the Warburg effect and OXPHOS, along with altered ROS production, disrupted calcium regulation, and aberrant interactions within the mitochondrial network [7].This switch allows cancer cells to generate energy and biosynthetic precursors, enabling their rapid proliferation even in oxygen-deprived conditions.Alongside the Warburg effect, cancer cell mitochondria may undergo modifications in fatty acid oxidation and glutamine metabolism [8].In cancer, mitochondria exhibit notable heterogeneity and dysregulation across various cellular processes, such as apoptosis, regulated necrosis, ferroptosis, and autophagic cell death (ACD).These characteristics significantly contribute to increasing the therapeutic resistance of patients [9].
The inhibition of mitochondrial function in malignant cells represents a promising strategy for selectively targeting malignant cells and reducing their adaptation to the tumor microenvironment, thereby impeding tumor progression.Mitochondria-targeted cancer therapy relies on distinctions between mitochondrial function in cancerous and healthy cells.One widely employed therapeutic approach involves inhibiting ATP production by suppressing either complex I or II in ETC.This generates significant energy stress in cancer cells, resulting in the initiation of autophagic cell death.Additionally, mitochondrial respiration can be inhibited by targeting specific enzymes in the TCA cycle, such as α-ketoglutarate dehydrogenase (KGDH) or pyruvate dehydrogenase (PDH) [10].Another approach to targeting mitochondria in cancer involves promoting oxidative stress or inducing autophagy.

Autophagy
Originally, autophagy was defined as a cell survival mechanism that occurs under starvation or oxidative stress (hypoxia, ROS) conditions, wherein the cell degrades damaged or unnecessary organelles to generate nutrients.Recently, it was discovered that autophagy is involved in the quality control of organelles/proteins by degrading dysfunctional proteins/organelles.Autophagy is divided into selective and nonselective types.Nonselective autophagy is a process that transforms cellular energy by randomly removing organelles.In contrast, selective autophagy specifically targets damaged organelles, such as the ER, mitochondria, and peroxisomes, as well as cellular proteins.Nonselective autophagy is triggered under starvation or nutrient deprivation conditions, while selective autophagy is more prevalent in nutrient-rich environments [11].
It was recently reported that autophagic cell death (ACD) is likely an outcome of either extensive autophagy, prolonged stress, or inhibited apoptosis [12].During ACD, nuclear condensation increases, caspase activity decreases, and cellular vacuoles are generated [13].
Selective autophagy is a multistage process that includes the following steps: initiation, elongation, maturation, fusion, and degradation.Initiation (Figure 2A) commences with the activation of the ULK (Unc-51-like kinase) complex.This complex controls the commencement of selective autophagy by forming a stable protein assembly that includes ULK1/2 (serine/threonine Unc-51 like kinase 1/2), FIP200 (also known as RB1CC1), ATG13, and ATG101.Once this complex is formed, it initializes and regulates the formation of the pre-autophagosomal structure (PAS) and recruits ATG9 vesicles [14], which facilitate PAS expansion and are often referred to as the "seeds" of autophagosome formation [15].The activity of the ULK complex is regulated by leading regulators of nutrient stress sensors, namely, mechanistic target of rapamycin complex 1 (mTORC1) and AMP-activated protein kinase (AMPK) [16].Specifically, mTORC1 suppresses the function of the ULK complex through the phosphorylation of ATG13 and ULK1 proteins [17].Furthermore, mTORC1 modulates the location of transcription factor EB (TFEB) by directing it to lysosomes.The key regulator of the autophagy pathway, TFEB, orchestrates the transcriptional regulation of autophagy genes via binding to the CLEAR (coordinated lysosomal expression and regulation) element in the nucleus.The interaction between TFEB and CLEAR promotes autophagy and facilitates lysosomal biogenesis [17].The initiation of autophagy requires either the inactivation of mTORC1 or the activation of AMPK.The activity of AMPK de-
The primary purpose of mitophagy is to regulate the quality and quantity of mitochondria via the selective elimination of dysfunctional or damaged organelles [24], and it is important for embryonic development, apoptosis, and cell differentiation.The main role of mitophagy is to maintain mitochondrial quality control and homeostasis.When mitophagy is ineffective at removing damaged mitochondria, the accumulation of dysfunctional or deficient mitochondria increases, resulting in decreased OXPHOS performance and increased levels of ROS.This imbalance can disrupt metabolism, cause cellular damage, and eventually result in cell death.Improper mitophagy contributes to the development of various pathological states, such as cancer and metabolic, neurodegenerative, cardiovascular, and skeletal muscle diseases [25].Mitophagy can be activated by nutrient limitation or mitochondrial dysfunction, among which the latter is caused by different types of stress factors, such as mtDNA damage, elevated levels of mtROS, misfolded mitochondrial proteins, hypoxia, and declined mitochondrial membrane potential (MMP) [26].Mitophagy is divided into ubiquitin-dependent (PARKIN-dependent and -independent) and ubiquitin-independent (receptor-based) types.The complex ULK initializes the formation of the second autophagic complex, also known as the PI3K (phosphatidylinositol 3-kinase) complex.It is composed of VPS34 (Vacuolar protein sorting 34, a class III Pi3K), VPS15, Beclin1 (Bcl-2-interacting myosinlike coiled-coil), ATG14, p150, and NRBF2 (nuclear-receptor-binding factor 2).This complex is engaged in the extension of the phagophore (an isolated lipid double-membrane structure) and the production of phosphoinositide 3-phosphate (PI3P) on the autophagic membrane (Figure 2).The elongation of the phagophore (Figure 2B) is initiated by the production of PI3P and the recruitment of the scaffold protein WIPI2 (WD-repeat domain phosphoinositide-interacting 2).Subsequently, WIPI2 facilitates the tethering of the endoplasmic reticulum membrane and phagophore via ATG2 and supports the assembly of the ATG5-ATG12-ATG16L1 complex, along with ATG3 and ATG7.These proteins are essential for the expansion and formation of the phagophore membrane, as they provide a physical platform and facilitate the lipidation of ATG8 family proteins (LC3 (microtubule-associated protein 1 light chain 3) or GABARAP (GABA type A receptor-associated protein)) [19].The ubiquitin-like proteins LC3 and GABARAP facilitate the attachment of the cargo adaptor/receptor to the lipid membrane (specifically to phosphatidylethanolamine (PE)), acting as a binding platform [17].The protein ATG4, along with its partners ATG7 (ubiquitinactivating enzyme (E1)) and ATG3 (ubiquitin conjugation enzyme (E2)), facilitate the transformation of LC3 into its soluble form, LC3-I [20].The ATG5-ATG12-ATG16L conjugation cascade is essential for attaching soluble LC3-I to PE in the lipid membrane.This attachment leads to the generation of lipidated LC3-II, which acts as a docking site for autophagy cargo adaptors/receptors.But on the outer membrane, LC3-II promotes autophagosome maturation (Figure 2C) and lysosome merging.Autophagic cargo adaptors in the autophagosomal membrane, including p62/SQSTM1 and NRB1, selectively identify and associate with ubiquitinated cargo material [13].
The autophagosome membrane is closed by the activity of ESCRT components (endosomal sorting complex required for transport)-CHMP2 (charged multivesicular body protein 2) and VPS4 [21].The Fusion (Figure 2D) of mature autophagosome with lysosomes is initiated by SNARE (soluble N-ethylmaleimide-sensitive attachment protein receptors) superfamily proteins, including STX17, SNAP29, VAMP3, VAMP7, VAMP8, and YKT6 [14].They are both found on the autophagosome and lysosome membranes [22].The process of fusion between the autophagosome and lysosome is promoted by tethering factors, including the HOPS (homotypic fusion and protein sorting) complex (VPS11, VPS18, VPS33A, VPS39, and VPS41), PLEKHM1 (pleckstrin-homology-domain-containing family M member 1), and EPG5 [23].The tethering factors interact with GTPases, including ARL8B and RAB7, located in the lysosome membrane.Additionally, they bind to ATG8 family proteins present on the outer membrane of autophagosomes [22].After the autophagosome fuses with the lysosome, the autophagic cargo undergoes degradation (Figure 2E) mediated by lysosomal enzymes.This process causes the degradation of organelles and the release of metabolic components.
The primary purpose of mitophagy is to regulate the quality and quantity of mitochondria via the selective elimination of dysfunctional or damaged organelles [24], and it is important for embryonic development, apoptosis, and cell differentiation.The main role of mitophagy is to maintain mitochondrial quality control and homeostasis.When mitophagy is ineffective at removing damaged mitochondria, the accumulation of dysfunctional or deficient mitochondria increases, resulting in decreased OXPHOS performance and increased levels of ROS.This imbalance can disrupt metabolism, cause cellular damage, and eventually result in cell death.Improper mitophagy contributes to the development of various pathological states, such as cancer and metabolic, neurodegenerative, cardiovascular, and skeletal muscle diseases [25].Mitophagy can be activated by nutrient limitation or mitochondrial dysfunction, among which the latter is caused by different types of stress factors, such as mtDNA damage, elevated levels of mtROS, misfolded mitochondrial proteins, hypoxia, and declined mitochondrial membrane potential (MMP) [26].Mitophagy is divided into ubiquitin-dependent (PARKIN-dependent and -independent) and ubiquitinindependent (receptor-based) types.

Ubiquitin-Mediated Mitophagy
Ubiquitin-dependent mitophagy is a selective mechanism wherein mitochondria that are specifically marked with ubiquitin molecules are removed from the cell [26].The initiation of PINK1 (PTEN-induced putative kinase 1)/Parkin-mediated mitophagy occurs in response to mitochondrial stress, including mitochondrial membrane depolarization or the extreme misfolding of mitochondrial proteins (Figure 3).Mitochondrial dysfunction leads to the accumulation of the serine/threonine PINK1 kinase at the OMM, whereas under physiological conditions, the levels of PINK1 in mitochondria are typically low.The durability of PINK1 protein at the OMM depends on the activity of TOMM7 (translocase of outer mitochondrial membrane 7), Hsp70 (heat shock protein), PHB2 (prohibitin 2), and PGAM5 (mitochondrial serine/threonine protein phosphatase) [27].At a damaged OMM, PINK1 auto-activates, dimerizes, and induces cytosolic Parkin ligase (U3 ubiquitin ligase) activity via phosphorylation.The active Parkin ligase produces ubiquitin chains and tags OMM proteins, such as MFN2 (Mitofusin-2), VDAC-1 (voltage-dependent anion channel-1), and Miro (mitochondrial Rho GTPase), for mitophagy.Ubiquitinated OMM proteins provide a scaffold for the binding of autophagy adaptor proteins (also named autophagy receptor proteins).Besides Parkin ligase, other E3 ubiquitin ligases like GP78 (glycoprotein 78), MUL1 (mitochondrial E3 ubiquitin ligase 1), and SIAH1 (seven in absentia homolog 1) are also responsible for ubiquitinating mitochondrial proteins [24].The tagged mitochondria are isolated from the healthy mitochondrial network through the activity of RHOT1 (Ras homolog family member T1) [28].However, some studies have indicated that mitochondria are fragmented and separated from the ER before they can be tagged for mitophagy [29].Additionally, mitochondrial proteins that are improperly tagged with ubiquitin chains are modified by deubiquitinase (DUB) enzymes [26].accumulates on the outer mitochondrial membrane (OMM), where it undergoes phosphorylation and activation.This activation subsequently triggers Parkin ligase, which ubiquitinates mitochondrial proteins, such as MFN2 and VDAC-1.Mitochondria with polyubiquitinated OMM proteins recruit mitophagy cargo receptors/adaptors, such as NDP52 and NBR1, to their surfaces.The mitophagy cargo receptor/adaptors connect both with LC3-II, present on the phagophore membrane, and with ubiquitinated chains.This image was created on BioRender.com.

Ubiquitin-Independent Mitophagy
Ubiquitin-independent mitophagy is a process where damaged mitochondria are directed to the mitophagosome without relying on ubiquitin tagging.Instead, this process depends on the presence of mitophagy receptors/adaptors, as summarized in Table 1.These receptors/adaptors directly interact with MAP1LC3/LC3 and LC3/GABARAP, which are localized on the phagophore membrane [31].Ubiquitin-independent mitophagy receptors/adaptors, such as BNIP3 (BCL2/adenovirus E1B 19 kDa protein-interacting protein 3), BNIP3L/NIX, FUNDC1 (FUN14 Domain-Containing 1), BCL2L13 (BCL2-Like 13), FKBP8 (FKBP Prolyl Isomerase 8), and AMBRA1 (the activating molecule in BE-CLIN1-regulated autophagy 1), are directly located on the mitochondria membrane.The expression levels of these receptors are regulated by transcriptional and post-transcriptional modifications [26].Besides protein mitophagic receptors, mitochondria also exploit lipid-based receptors like cardiolipin (CL) and ceramide [30] (Table 1).CL is typically found in the IMM, where it supports the activity of ETC complexes I, III, and IV and ATP synthase.However, under mitochondrial stress, CL can translocate to the OMM [32].In the next step, PINK1 phosphorylates ubiquitin chains that are attached to OMM proteins to enhance the mitophagy process.Finally, OMM proteins marked with ubiquitin are recognized by autophagy receptors/adaptors of ubiquitin-dependent mitophagy SQSTM1/p62 (sequestosome 1), OPTN (optineurin), CALCOCO2/NDP52 (calcium binding and coiled-coil domain 2), NBR1 (neighbor of BRCA1 gene 1 protein), AMBRA1, and TAX1BP1 (Tax1 binding protein 1) [25] (Table 1).At the N-terminal arm, these receptors possess an LC3-interacting region (LIR) that enables them to interact with the MAP1LC3/LC3 (microtubule-associated protein 1 light chain 3) and LC3 protein families, which are anchored in the phagophore membrane.The mitophagy receptors/adaptors can bind to the ubiquitinated OMM proteins through their ubiquitin-binding domain, thus forming mitophagy cargo.Once the mitophagic cargo binds to the mitophagy receptor, it triggers the formation of the mitophagosome.The mitophagosome, which encapsulates the marked mitochondrium, subsequently merges with lysosomes [30].

Ubiquitin-Independent Mitophagy
Ubiquitin-independent mitophagy is a process where damaged mitochondria are directed to the mitophagosome without relying on ubiquitin tagging.Instead, this process depends on the presence of mitophagy receptors/adaptors, as summarized in Table 1.These receptors/adaptors directly interact with MAP1LC3/LC3 and LC3/GABARAP, which are localized on the phagophore membrane [31].Ubiquitin-independent mitophagy receptors/adaptors, such as BNIP3 (BCL2/adenovirus E1B 19 kDa protein-interacting protein 3), BNIP3L/NIX, FUNDC1 (FUN14 Domain-Containing 1), BCL2L13 (BCL2-Like 13), FKBP8 (FKBP Prolyl Isomerase 8), and AMBRA1 (the activating molecule in BECLIN1-regulated autophagy 1), are directly located on the mitochondria membrane.The expression levels of these receptors are regulated by transcriptional and post-transcriptional modifications [26].Besides protein mitophagic receptors, mitochondria also exploit lipid-based receptors like cardiolipin (CL) and ceramide [30] (Table 1).CL is typically found in the IMM, where it supports the activity of ETC complexes I, III, and IV and ATP synthase.However, under mitochondrial stress, CL can translocate to the OMM [32].

Chaperone-Mediated Autophagy
Chaperone-mediated autophagy (CMA) is a distinctive type of selective autophagy responsible for the lysosomal degradation of misfolded or damaged proteins.In contrast to ubiquitin-dependent/independent autophagy, during the CMA process, proteins are not enclosed in the autophagosome; instead, they are directly targeted by the chaperone Hsc70 (heat shock cognate protein 70) in the cytosol.The mechanism of CMA is categorized into distinct stages (Figure 4): 1. substrate recognition; 2. the binding of the substrate to the lysosomal membrane; 3. the multimerization of translocation complex; 4. substrate unfolding; 5. substrate translocation and degradation in the lysosomal lumen; and 6. dissociation of the translocation complex.Hsc70 recognizes CMA's substrates by binding to the KFERQ motif in target proteins [44].The function of Hsc70 is supported by various co-chaperons, including Hsp40 (heat shock protein 40), CHIP (carboxyl terminus of hsc70-interacting protein), BAG1 (Bcl2-associated athano-gene 1 protein), and HOP (hsp70-hsp90 organizing protein) [45].In addition to recognizing substrates, the complex HOP is actively engaged in protein stabilization and unfolding [46].After the substrate recognition step, Hsc70, along with the target protein, binds to the lysosomal receptor LAMP-2A (lysosome-associated membrane protein type 2A) [47].LAMP-2A forms a dynamic translocation channel via multimerization and interaction with GFAP (glial fibrillary acidic protein), which is responsible for maintaining the structure of the multimeric LAMP-2A complex in the lysosomal membrane.Consequently, the CMA substrate is unfolded and transported into the lysosomal lumen, where it undergoes immediate degradation by lysosomal proteases [48].After CMA substrate translocation, the interaction between GFAP and EF1α (elongation factor 1-α) is disrupted by GTP (guanosine triphosphate).This disturbance results in the release of EF1α to phosphorylated GFAP, which, in turn, facilitates the disassembly of LAMP-2A into its individual monomers [49].The phosphorylation of GFAP on the lysosomal membrane supports the dissociation of GFAP from the LAMP-2A multimeric complex through the dimerization of phosphorylated GFAP with unmodified GFAP.The level of GFAP phosphorylation is controlled by the activity of AKT1 (AKT serine/threonine kinase 1), which becomes active when phosphorylated by mTORC2 (mammalian target of rapamycin complex 2) and inactive when dephosphorylated by PHLPP1 (PH domain and leucine-rich repeat protein phosphatase 1) [45].
The transport of LAMP-2A to the lysosomal surface represents a crucial stage in CMA.Moreover, the level of LAMP-2A directly affects CMA activity.The translocation of LAMP-2A to lysosomal membrane is determined by the involvement of Rab-7A (Ras-related protein Rab-7A), Rab-11A, DYNC1LI2 (Dynein Cytoplasmic 1 Light Intermediate Chain 2), and RILP (Rab-interacting lysosomal protein) [45].CMA activity is regulated by the amounts of the key CMA proteins (Hsc70, GFAP, and LAMP-2A), as well as by the kinase AKT1 and circadian cycle regulators, such as BMAL1 (basic helix-loop-helix ARNT-like 1), PER1/2 (period circadian protein homolog 1/2), or RARα (retinoic acid receptor alpha) [50].Increased CMA activity is usually related to lipotoxicity (cytosolic lipid overload), starvation, hypoxia, and mitochondrial or ER stress.The elevated CMA activity is affected by the transcriptional upregulation of LAMP-2A (mostly by NFE2L2 (NFE2-Like BZIP transcription factor 2), Nrf2, and NFAT1 (nuclear factor of activated T cells) [51].
The CMA pathway supports a range of cellular processes, including the maintenance of protein quality, the regulation of the cell cycle, and the modulation of immune responses.Especially, CMA contributes to the quality control of mitochondrial proteins, such as COX IV (cytochrome c oxidase subunit 4), Tom20 (mitochondrial import receptor subunit TOM20 homolog), DJ-1 (nucleic acid deglycase), Parkin, MFN2, ATP5F1A (ATP synthase F1 subunit alpha), and VDAC1, which modulate mitochondrial function and protect the integrity of mitochondria [45].The transport of LAMP-2A to the lysosomal surface represents a crucial stage in CMA.Moreover, the level of LAMP-2A directly affects CMA activity.The translocation of LAMP-2A to lysosomal membrane is determined by the involvement of Rab-7A (Rasrelated protein Rab-7A), Rab-11A, DYNC1LI2 (Dynein Cytoplasmic 1 Light Intermediate Chain 2), and RILP (Rab-interacting lysosomal protein) [45].CMA activity is regulated by the amounts of the key CMA proteins (Hsc70, GFAP, and LAMP-2A), as well as by the kinase AKT1 and circadian cycle regulators, such as BMAL1 (basic helix-loop-helix ARNT-like 1), PER1/2 (period circadian protein homolog 1/2), or RARα (retinoic acid receptor alpha) [50].Increased CMA activity is usually related to lipotoxicity (cytosolic lipid overload), starvation, hypoxia, and mitochondrial or ER stress.The elevated CMA activity is affected by the transcriptional upregulation of LAMP-2A (mostly by NFE2L2 (NFE2-Like BZIP transcription factor 2), Nrf2, and NFAT1 (nuclear factor of activated T cells) [51].
The CMA pathway supports a range of cellular processes, including the maintenance of protein quality, the regulation of the cell cycle, and the modulation of immune responses.Especially, CMA contributes to the quality control of mitochondrial proteins, such as COX IV (cytochrome c oxidase subunit 4), Tom20 (mitochondrial import receptor subunit TOM20 homolog), DJ-1 (nucleic acid deglycase), Parkin, MFN2, ATP5F1A (ATP synthase F1 subunit alpha), and VDAC1, which modulate mitochondrial function and protect the integrity of mitochondria [45].

Role of Autophagy in Tumorigenesis
In cancer, the autophagy process serves a dual and complex function, acting either as a suppressor or initiator of tumorigenesis, depending on the type of tumor and the stage of disease advancement.On the one hand, autophagy might promote cancer suppression by abolishing oxidative stress, inhibiting cellular transformation, preventing the accumulation of damaged cellular components, and maintaining cell homeostasis [11].Transcription factors like p53, death-associated protein kinase (DAPK), tuberous sclerosis proteins 1 and 2 (TSC1/2), and phosphatase and tensin homolog (PTEN) are essential contributors to the tumor-suppressive function of autophagy [11].
On the other hand, autophagy can support tumor development and metastasis by providing nutrients to cancer cells [52], allowing cancer cells to survive under metabolic stress.Tumor oncogenes, like RAS and BRAF, promote tumor growth by upregulating the process of autophagy [11].In developing novel cancer therapies or enhancing the efficacy of chemotherapy, comprehending the involvement of autophagy at all phases of tumor formation is crucial.This knowledge contributes to the advancement of precision therapies that can effectively modulate autophagy [53].
The involvement of the autophagy activator Beclin-1 in tumorigenesis is linked to its phosphorylation level and interactions with various partner proteins [54].DAPK is a key regulator protein that contributes to the phosphorylation status of Beclin-1 and the formation of the autophagosome [55].Autophagy inhibition is achieved through the interaction of Beclin-1 with its inhibitor, BCL2.In contrast, the interaction of Beclin-1 with AMBRA1, UVRAG (UV-radiation-resistance-associated gene protein), and BIF1 (Bax interacting factor 1) disrupts the binding of Beclin-1 with BCL2, which subsequently leads to autophagy initiation [11].In solid tumors, a decrease in Beclin-1 expression is often observed and correlated with metastasis development.On other hand, in colorectal cancers and gastric carcinomas, Beclin-1 expression is elevated, resulting in enhanced autophagy.This observation has led to the suggestion that Beclin-1 promotes cell proliferation and tumorigenesis under stress conditions like hypoxia and starvation [56].Furthermore, Beclin-1 cooperates with another autophagy regulator, PTEN, which negatively controls the activity of the PI3K/AKT pathway.A reduced expression of PTEN and Beclin-1 has been observed in chemoresistant ovarian cancers [57].This discovery indicates that PTEN and Beclin-1 play roles in regulating autophagy in ovarian cancer, and their decreased expression levels contribute to reducing autophagy activity and increasing chemoresistance [58].
The modulation of autophagy by the major transcription factor p53 is determined by its subcellular localization, which determines whether cancer cells will survive or die.Nuclear p53 facilitates autophagy activation by promoting the transcription of autophagy-related genes, while cytoplasmic p53 suppresses autophagy by inhibiting autophagy regulators [11].Upon encountering cellular stress, nuclear p53 initiates autophagy through inducing the expression of DRAM (damage-regulated autophagy modulator), DAPK, and ULK1/2 [59].
Moreover, p53, through the promotion of autophagy, can increase the proliferation and resistance to chemotherapy of malignant liposarcoma cells [60].
The accumulation of autophagy cargo receptor p62 (also known as SQSTM1) is a notable feature observed in many cancers, and it is correlated with poor clinical outcomes among hepatocellular carcinoma patients [61] and increased metastasis occurrence in nasopharyngeal carcinoma.The accumulation of p62 supports tumor development and cancer cell growth via the activation of Nrf2, mTORC1, TRAF6 (tumor-necrosis-factorreceptor-associated factor 6), TNFa (tumor necrosis factor α), and NF-kB (nuclear factor kappa-light-chain-enhancer of activated B cells) [54].Consequently, an increased presence of p62 in tumors implies its involvement in promoting the development and progression of cancer.Therefore, inhibiting p62 during autophagy holds promise as a strategy for treating cancer [62].
Among mitophagy regulators, it has been observed that the tumor suppression Parkin protein encoded by the PARK2 gene is frequently deleted in colorectal, lung, breast, glioblastoma, and melanoma cancers.The absence of Parkin E3 ubiquitin ligase leads to the accumulation of dysfunctional mitochondria, resulting in elevated levels of glycolysis and ROS, reduced OXPHOS, and increased resistance to apoptosis in cells [22].
The mitochondrial kinase PINK1 is implicated in tumor suppression due to its role in detecting and removing damaged mitochondria.In certain cancers, there is a noted decrease in PINK1 expression (such as sarcomas, neuroblastomas, and leukemias), while in others, there is an increase (such as lung and breast cancers and carcinoma) [63].
Autophagy has been demonstrated to play a pivotal role in promoting drug resistance in chemotherapy-treated cancer cells.It also regulates cell migration and metastasis by affecting the interactions between cancer and healthy cells [11].Despite the complex role of autophagy in cancer, inhibiting this process can make cancer cells more sensitive to chemotherapy and enhance cell death [24].

Modulation of Mitochondria and Autophagy Exhibits Promise in Cancer Treatment
Cancer cells frequently demonstrate the capacity to reprogram their metabolism, allowing them to survive and thrive in challenging conditions, including those generated by chemotherapy [6].Targeting metabolic plasticity in cancer has been shown to significantly enhance the effectiveness of cancer therapies [64].A recent study has shown that decreased expression of mitochondrial fission regulator protein DRP1 affects metabolic plasticity and reduces the survival of breast-cancer--induced brain metastases [65].
Mitochondria primarily drive the bioenergetic adaptation that facilitates tumor growth.It is well established that mitochondrial reprogramming promotes tumor growth and cancer cell proliferation via retrograde signaling involving ROS, Ca 2+ , ATP, or TCA intermediates, which can modify gene expression [6].It has recently been identified that the knockout of MTCH1 (mitochondrial carrier 1) in cervical cancer (in HeLa cells) activates retrograde signaling through the FOXO1-GPX4 axis, leading to increased accumulation of mtROS and ferroptosis.The study in question proposes the use of MTCH1 as a candidate target for retrograde signaling pathways in cervical cancer [66].
Modifying mitochondrial metabolism (Tables 2 and 3) offers a strategy for reshaping cancer cell metabolism and combatting drug resistance.Current strategies for targeting mitochondrial function include inhibiting ETC, modulating redox balance, affecting Ca 2+ homeostasis or the apoptotic pathway, and disrupting the TCA cycle.Disruption of ETC can be achieved through the inhibition of ETC complexes I-V.The effectiveness of several complex I inhibitors is limited by issues like poor potency, toxicity, or unintended off-target actions, such as targeting rotenone and BAY 87-2243 [67].While some complex I inhibitors have failed to translate successfully to preclinical studies, others are currently being tested in clinical trials (Table 3).Phenformin, an antidiabetic drug, inhibits complex I and disrupts the redox balance (NADH/NAD+) and energetic state (AMP/ATP), resulting in AMPK activation [68].Atovaquone, used as an antimalarial drug, interferes with complex III, reducing oxygen consumption and subsequently decreasing tumor hypoxia in individuals with non-small-cell lung cancer [69].
Through the excessive activation of mitochondrial respiration, the loss of MMP can cause a breakdown in mitochondrial metabolism and ATP production, resulting in cell death.A newly identified complex IV activator, the fungal natural product ophiobolin A (OPA), significantly decreases NCI-H1703 cells' proliferation [70].Bedaquiline interferes with ATP production by targeting complex V, which lowers DA-MB-231 breast cancer cell proliferation, enhances ovarian cancer cells' sensitivity to cisplatin, and helped prevent metastasis in a xenograft model [71,72].
The disruption of mitochondrial metabolism through TCA cycle inhibition using devimistat (CPI-613), PDH, and KGDH inhibitors is being tested in patients with advanced biliary tract cancer in vitro and in a Phase Ib clinical trial, in combination with gemcitabine and cisplatin [73].Current clinical trials are investigating devimistat (CPI-613) as a monotherapy for refractory Burkitt's lymphoma/leukemia (NCT03793140) and in combination with chemotherapies for advanced pancreatic cancer (NCT03699319) and with chemoradiation for pancreatic adenocarcinoma (NCT05325281) (Table 3).
Inhibiting the apoptosis regulator BCL-2 (B-cell lymphoma-2) is one of the most extensively investigated approaches for triggering the mitochondrial apoptotic pathway in cancer therapy.Venetoclax (ABT199) was the first FDA-approved BH3-mimetic drug, originally indicated for the treatment of chronic lymphocytic leukemia [74].Subsequent studies revealed its effectiveness in treating acute myeloid leukemia.It is commonly administered either as monotherapy or in combination with monoclonal antibodies, such as rituximab, or alongside chemotherapy.The molecular action of ventoclax is driven by the activation of BAK and BAX proteins, leading to the permeabilization of the mitochondrial outer membrane and inducing apoptosis [75].Ongoing preclinical and clinical (Table 3) studies are investigating the efficacy and safety of venetoclax, both as a monotherapy and in combination with other anti-cancer drugs, in treating breast cancer (NCT03900884), myeloma (NCT05455294), lung cancer (NCT04274907), prostate cancer (NCT03751436), and solid tumors [76].
Alongside its mitochondrial function, autophagy helps facilitate cancer plasticity under nutrient deprivation conditions.Inducing autophagy can potentially prevent tumor development and growth in the early stages [77].However, in advanced stages of cancer, autophagy supports tumor growth and metastasis by supplying the necessary substrates for cell proliferation [78].The impact of autophagy activation on tumorigenesis is influenced by the degree of autophagy.A basic level of autophagy facilitates tumor growth and the development of drug resistance, while a high level of autophagy results in excessive removal of cellular components, leading to the cell death [79].Relying only on autophagy targeting is insufficient for cancer treatment.Some studies have demonstrated that combining autophagy inhibitors or activators with chemotherapy, radiotherapy, or immunotherapy is a more effective treatment strategy [77].By inhibiting autophagy, the susceptibility of cancer cells to chemotherapeutic drugs and treatments that induce apoptosis is heightened [78].Tables 2 and 3 present a range of autophagy inhibitors and activators that are being investigated in preclinical studies and ongoing clinical trials.As FDAapproved antimalarial drugs, chloroquine (CQ) and hydroxychloroquine (HCQ) are some of the most prominent autophagy inhibitors being explored in cancer therapies based on autophagy mechanisms.Through their accumulation in lysosomes and inhibition of lysosomal acidification, they interrupt the autophagosome's fusion with lysosome and change signaling and transcriptional activity [80].The antitumor effect of HCQ was increased when used in combination with monoclonal antibodies, namely, anti-PD1 (nivolumab), in advanced melanoma (Table 3, NCT04464759); inhibitor of MEK1/2 (trametinib) in pancreatic cancer (NCT03825289); a Ras/Raf/MEK/ERK signaling pathway inhibitor (sorafenib) in hepatocellular cancer (NCT03037437); and an Akt inhibitor (MK2206) in solid tumors (NCT01480154).CQ and HCQ, in addition to changing lysosomal pH, also impact the pH values of Golgi vesicles and endosomes [81].CQ derivatives are also known to target and suppress the function of PPT1 (palmitoyl-protein thioesterase 1) in melanoma cells [82].The precise mechanisms of action of CQ and HCQ remain poorly understood and extend beyond their effects on autophagy.It has been observed that CQ activates the p53 pathway, resulting in apoptosis in glioma cells [83].In clinical trials, adverse events associated with CQ and HCQ, including nausea, diarrhea, vomiting, myopathy, and cardiotoxic effects, are frequently reported [84].
Conversely, stimulating autophagy in cancer treatment can effectively impede cell proliferation and inhibit tumor growth.Among the leading autophagy inducers examined in clinical trials are the FDA-approved mTOR inhibitors rapamycin (sirolimus) and its analogue temsirolimus (CCI-779) and everolimus, which are FDA-approved for the treatment of malignancies and the prevention of transplant rejection [85].Everolimus and temsirolimus are FDA-approved drugs used to treat advanced renal cell carcinoma.Ongoing research, including preclinical and clinical trials, is exploring their efficacy as a monotherapy and in combination with other therapies (CQ, radiation, and THZ1 (cyclin-dependent kinase 7 inhibitor)) across different cancer types (bladder, colorectal, and prostate cancers and carcinoma) in vitro and in vivo.Research is focusing on everolimus, both as a standalone treatment and in combination with CQ, HCQ, AKT inhibitors 1 and 2, arsenic trioxide, or propachlor, in breast, renal, and ovarian cancer cells; various carcinoma cell lines; and mouse models.Investigations have been conducted on rapamycin in cell lines of pancreatic, cervical, and lung carcinomas; melanomas; osteosarcomas; and liposarcomas, as well as in xenograft mice models [86].Clinical trials have explored the use of rapamycin in combination with chloroquine (CQ) and hydroxychloroquine (HCQ).Current ongoing research includes a Phase I trial assessing rapamycin's combination with vorinostat for treating advanced cancers (NCT01087554), as well as a Phase I/II study evaluating its use with HCQ, metformin, dasatinib, or nelfinavir in treating relapsed prostate cancer and other solid tumors (NCT05036226).
Recently, the natural polyphenol epigallocatechin gallate (EGCG) deriving from green tea leaves has garnered interest for its ability to induce cell death through autophagy and apoptosis.EGCG is known to alter multiple cellular pathways in different types of cancer.Among the most notable pathways it effects is the RAS-Raf-MEK-ERK axis, where its action leads to the inhibition of cell proliferation and the induction of apoptosis in pancreatic cancer [87,88].Moreover, EGCG attenuated the PTEN/AKT/mTOR pathway in ovarian cancer cell lines and mouse models [89].In bladder cancer cell lines (5634 and T24), EGCG induces apoptosis through the regulation of autophagy in a dose-dependent manner.EGCG upregulates the expression of caspase 3, caspase 9, and Bax, and it also decreases BCL2 expression.Concurrently, EGCG stimulates the formation of autophagosomes and elevates the expression of the autophagy-related protein LC3II [90].

Challenges Faced in Relation to Therapies Targeting Mitochondrial and Autophagic Processes
Utilizing autophagy and mitochondrial function modulators (Tables 2 and 3) in cancer therapy shows potential in overcoming tumor plasticity and drug resistance.However, some compounds exhibit dual effects, including non-specificity and undefined molecular mechanisms of action.For instance, EGCG activates autophagy and has been shown to suppress COX-2 in prostate, colon, and skin cancers in vitro and in mouse models as well as inhibit NF-kB in a melanoma mouse model [141].In colorectal cancer (the HT-29 cell line), it triggers endoplasmic reticulum stress through the upregulation of BiP and PERK, leading to apoptosis via increased caspase-3/7 levels.In glioblastoma (the T98G and U87MG cell lines), EGCG elevates ROS levels, increases caspase 8 levels, and activates the JNK pathway [142].Metformin is an exemplary mitochondria-targeted drug, as it decreases TCA cycle activity and inhibits complex I, leading to reduced ATP production.The resulting lower ATP levels activate AMPK and inhibit mTOR, which triggered autophagy in a myeloma cancer model (the RPMI8226 and U266 cell lines and NOD/SCID mice).In contrast, in leukemic cells (HL60 and MOLM14), metformin triggers apoptosis.Additionally, metformin has the ability to inhibit the NF-kB signaling pathway [143].These examples underscore the pressing need to develop drugs that specifically target autophagy or mitochondria.
The development of autophagy inhibition methods centers on either inducing excessive autophagy or targeting the early stages of autophagy initiation [59].A potential candidate for targeting autophagy initiation, the ULK1 inhibitor 13-oxyingenol-dodecanoate (13OD), is currently undergoing preclinical research.The associated study demonstrated that 13OD effectively inhibited the proliferation of non-small-cell lung cancer cells (A549 and H460) in vitro and in BALB/c athymic nude mice by promoting autophagic cell death [144].
Autophagy inducers, notably mTOR inhibitors, face challenges due to their incomplete targeting of mTORC1.This limitation arises as mTORC1 can bypass rapalog effects through the compensatory activation of other pathways, such as PI3K/Akt.Additionally, mutations in the FKBP12-rapamycin binding domain, including an alanine-to-valine substitution at position 2034 (A2034V) and a phenylalanine-to-leucine substitution at position 2108 (F2108L), as well as the activation of mTORC2-dependent pathways, contribute to the issue [145].
Following clinical trials, it was revealed that HCQ's therapeutic effects are not mainly induced by autophagy inhibition.Rather, HCQ accumulates in endosomes, inhibits the toll-like receptor (TLR) pathway, reduces self-antigen presentation, and curbs cytokine production.The acidic nature of the tumor microenvironment negatively impacts HCQ's efficacy by restricting its cellular transport.To address this challenge and minimize toxicity, targeted drug delivery systems like nanoparticles can be utilized [146].
Researchers conducting clinical trials struggle with the challenge of identifying which cancer types and grades are autophagy-dependent, requiring them to discern the function of autophagy each specific cancer patient [59].To tackle the issue of identifying cancer's dependence on autophagy, some clinical studies employ biomarkers.A case in point is a clinical trial that evaluated glioblastoma patients' responses to combined CQ, chemotherapy, or radiotherapy by analyzing the EGFRvIII marker [147].The level of the autophagy marker p62 is influenced not only by autophagy activity but also by its role in activating antioxidant gene expression, particularly NRF2, even when autophagy is not occurring [59].
For the mitochondria-targeted BCL-2 inhibitor venetoclax, clinical trials have revealed that secondary resistance can arise in multiple myeloma patients who have undergone long-term venetoclax therapy or possess missense mutations in BCL-2 and BAX.Venetoclax treatment, whether administered as a monotherapy or in combination with chemotherapy, can cause adverse events, including nausea, diarrhea, tumor lysis syndrome, and, most commonly, neutropenia and thrombocytopenia [148].Studies investigating IDH1/IDH2 inhibitors indicate that resistance can occur in solid malignancies.It is hypothesized that this resistance arises from isotype switching, wherein patients with cytosolic IDH1 mutations develop mitochondrial IDH2 mutations after receiving IDH1 inhibitor therapy [149].
Despite their potential, the application of autophagy and mitochondria modulators in cancer treatment remains limited due to several challenges, including their lack of specificity, the development of resistance, cancer heterogeneity, and unclear molecular mechanisms underlying their actions.To address these issues, further studies are essential, especially those focused on discovering innovative drug targets and assessing synergistic combinations of drugs.Furthermore, creating autophagy-related biomarkers could help manage the variability among cancer patients and allow for more individualized treatment strategies.

Autophagy-Related Genes Hold Potential as Prognostic and Diagnostic Biomarkers for Cancer
Diagnosing and predicting the outcome of cancer in its early stages are essential for successful and effective treatment.Various types of cancer have unique autophagyrelated biomarkers that serve as prognostic indicators.Identifying these biomarkers is essential for cancer diagnosis and can help predict the effectiveness of therapies that modulate autophagy.
In regard to melanoma, the extensively studied potential autophagy-related biomarkers are LC3, p62, and Beclin-1.Immunohistochemical analysis of malignant melanomas has revealed an increased expression of LC3 and decreased expression of Beclin-1, which are correlated with poorer patient outcomes and the progression of metastasis.However, there are instances of Beclin-1 overexpression and LC3 downregulation in advanced melanoma.The prognostic biomarker p62 is upregulated in the early stages of melanoma according to the AJCC (American Joint Committee on Cancer), but its expression is downregulated in advanced metastatic tumors [150].In observational studies, these markers were validated in endometrial polyp tissue samples via immunohistochemistry (NCT04706000).Previous research on endometriosis has identified reduced levels of Beclin-1 mRNA and protein [151] (Table 4).
Analysis of mRNA expression in 52 normal and 495 tumor tissues from the Prostate Adenocarcinoma database identified mutations in ATG9B, DNAJB1 (DnaJ heat shock protein family (Hsp40) member B1), HSPB8, NKX2-3, and TP63 genes significantly associated with an increased risk of developing prostate cancer.Additionally, BNIP3, NPC1, and TP53 genes serve as prognostic autophagy biomarkers for advanced stages of prostate cancer [152].
In oral squamous cell carcinoma (OSCC), RNA sequencing and clinical screening data analysis have identified ATG12 and BID as potential prognostic autophagy-related biomarkers.Subsequent validation studies based on qRT-PCR, immunohistochemistry, and Western blot analysis have confirmed that these biomarkers are overexpressed in OSCC cell lines (SCC9, SCC15, SCC25) and tissues [153].Research employing tissue microarrays, immunohistochemistry, and Western blot analysis conducted on formalin-fixed, paraffin-embedded tissues from 352 gastric cancer patients has indicated that diminished expression of ULK1, Beclin 1, ATG3, and ATG10 is associated with improved prognosis [154].
The transcriptome profiles from the TCGA (The Cancer Genome Atlas) and GTEx (The Genotype-Tissue Expression) databases, supported by clinical data and qPCR analysis of fresh cervical cancer samples, revealed ATG4D, CD46, TP73, and HSPB8 as autophagyrelated risk biomarkers.These markers are downregulated in cervical cancer and are associated with favorable prognosis [155].An additional autophagy-related long noncoding RNA (lncRNA) involved in cervical cancer identified using a public database has established 10 lncRNAs with prognostic potential, with DBH-AS1 being the most notable.Moreover, the associated study confirmed the role of lncRNA in regulating autophagy, modulating tumor development, and altering sensitivity to treatment [156].
In regard to glioma, one well-known biomarker is VMP1.Data analyses based on various cancer genome atlases have shown that VMP1 is upregulated in high-grade gliomas, and this is associated with a worse prognosis.Suppressing VMP1 expression through CRISPR-Cas9 gene editing significantly inhibited the proliferation of LN299 cells, leading to partial autophagy as a result of disrupted autophagosome formation and the initiation of apoptosis.VMP1 has the potential to be utilized as a predictor of survival for glioma patients [157].
In regard to bladder cancer, 11 autophagy-related biomarkers have been identified as key indicators of patient survival and clinical outcomes based on information from the Human Autophagy Database and Bladder Carcinoma databases.These biomarkers are APOL1, ATG4B, BAG1, CASP3, DRAM1, ITGA3, KLHL24, P4HB, PRKCD, ULK2, and WDR45.Notably, the overexpression of ULK2 and P4HB is linked to high-risk bladder cancer.In contrast, the overexpression of APOL1, ATG4B, BAG1, DRAM1, ITGA3, KLHL24, PRKCD, and WDR45 is correlated with low-risk bladder cancer [158].A study (NCT03254888) on bladder cancer patients with confirmed histopathology employed quantitative real-time PCR to estimate ATG7 levels and used immunohistochemistry to determine LC3A levels as markers of autophagy (Table 4).
In regard to esophageal cancer, RNA-sequencing data analysis and clinical information derived from TCGA database identified DNAJB, BNIP1, VAMP7, and TBK1 (TANK binding kinase 1) as prognostic autophagy-related signatures.These biomarkers are significantly associated with overall patient survival [159].
Significant increases in autophagy and mitophagy markers, such as Beclin-1, LC-3, BNIP-3, and Parkin, were detected in breast cancer tissues compared to controls.The associated study also indicated that LC3 immunostaining was linked to younger breast cancer patients, while Parkin was associated with a history of breastfeeding [160].
An analysis of ovarian cancer gene expression profiles from the TCGA database, in conjunction with clinical data, uncovered 52 potential autophagy-related genes.LASSO-Cox analysis further revealed that FOXO1 and CASP8 are particularly promising for prognosis.Immunohistochemical analysis of tissue microarrays from 125 patients identified that elevated FOXO1 expression is linked to metastasis and a poorer prognosis in ovarian cancer [161].
Cancer prognosis and diagnosis are highly demanding disciplines owing to the diversity and intricacy of gene expression in individual patients.Each cancer patient possesses distinct genetic profiles and undergoes unique modifications in gene expression in response to cancer development.This uniqueness presents challenges in predicting cancer progression and treatment response.The heterogeneity in gene expression among cancer patients results in variation in tumor behavior and sensitivity to chemotherapy.Identifying specific prognostic biomarkers can contribute to early cancer patient diagnosis and enhance the effectiveness of personalized treatment strategies.

Conclusions
This review provides a comprehensive overview of the various functions of mitochondria within cancer cells, with a specific focus on their role in autophagy.Understanding the distinct characteristics of mitochondria in both healthy and cancerous cells, particularly in relation to autophagy, is crucial for developing more precise treatments, especially for cancer [9].Strategies for inhibiting mitochondrial function or autophagy in cancer treatment include: 1. inducing oxidative stress; 2. disrupting mitochondrial respiration by targeting Complexes I through V; 3. inhibiting non-voltage calcium channels; 4. suppressing TCA cycle enzymes; and 5. modulating autophagy through activation or inhibition [162].
Autophagy is initiated under conditions of starvation and stress, such as organelle damage and the presence of misfolded proteins [163].In cancer, autophagy plays a dual role: it can either promote tumorigenesis in certain cancers or suppress tumor development in others.Additionally, autophagy plays a role in the development of drug resistance and metastasis [12].Modulating autophagy in cancer cells holds promise for cancer treatment.Autophagy inhibitors like chloroquine and hydroxychloroquine, as well as autophagy activators such as temsirolimus and rapamycin, have demonstrated efficacy in disrupting tumor growth, especially when combined with chemotherapy, according to both preclinical and clinical studies [164].Despite the potential of mitochondrial function or autophagy modulators, their application is limited by several factors, including a lack of specificity, incomplete targeting due to mutations at binding sites, adverse events, and the development of secondary resistance.
Moreover, the precise diagnosis of specific cancer types is as crucial as the development of effective treatments.Early-stage cancer diagnosis significantly enhances the likelihood of successful treatment.Autophagy-related biomarkers are valuable for both cancer diagnosis and prognosis.This review also provides an overview of unique autophagy biomarkers across different types of cancer in pre-clinical and clinical studies.

Figure 1 .
Figure 1.Overview of mitochondrial functions.Mitochondria perform several essential functions within the cell, including ATP production; reactive oxygen species (ROS) generation and elimination through superoxide dismutase (SOD), NADPH oxidase (NOX), catalase (CAT), glutathione peroxidase (GSH-Px), or thioredoxin peroxidase (TRX-Px); mitochondrial communication; and regulation of cell death.This image was created on BioRender.com.

35 Figure 3 .
Figure 3. PINK1/Parkin-dependent mitophagy.Under conditions of mitochondrial stress, PINK1 accumulates on the outer mitochondrial membrane (OMM), where it undergoes phosphorylation and activation.This activation subsequently triggers Parkin ligase, which ubiquitinates mitochondrial proteins, such as MFN2 and VDAC-1.Mitochondria with polyubiquitinated OMM proteins recruit mitophagy cargo receptors/adaptors, such as NDP52 and NBR1, to their surfaces.The mitophagy cargo receptor/adaptors connect both with LC3-II, present on the phagophore membrane, and with ubiquitinated chains.This image was created on BioRender.com.

Figure 3 .
Figure 3. PINK1/Parkin-dependent mitophagy.Under conditions of mitochondrial stress, PINK1 accumulates on the outer mitochondrial membrane (OMM), where it undergoes phosphorylation and activation.This activation subsequently triggers Parkin ligase, which ubiquitinates mitochondrial proteins, such as MFN2 and VDAC-1.Mitochondria with polyubiquitinated OMM proteins recruit mitophagy cargo receptors/adaptors, such as NDP52 and NBR1, to their surfaces.The mitophagy cargo receptor/adaptors connect both with LC3-II, present on the phagophore membrane, and with ubiquitinated chains.This image was created on BioRender.com.

Table 2 .
Synthetic inducers and inhibitors of mitochondrial function and autophagy.

Table 3 .
Investigated drugs targeting autophagy and mitochondrial pathways in ongoing cancer clinical trials.

Table 4 .
Observational research on cancer patients derived from clinical trial database.