OR2H2 Activates CAMKKβ–AMPK–Autophagy Signaling Axis and Suppresses Senescence in VK2/E6E7 Cells

Olfactory receptors are expressed in multiple extra-nasal tissues and these ectopic olfactory receptors mediate tissue-specific functions and regulate cellular physiology. Ectopic olfactory receptors may play key roles in tissues constantly exposed to odorants, thus the functionality of these receptors in genital tissues is of particular interest. The functionality of ectopic olfactory receptors expressed in VK2/E6E7 human vaginal epithelial cells was investigated. OR2H2 was the most highly expressed olfactory receptor expressed in VK2/E6E7 cells, and activation of OR2H2 by aldehyde 13-13, a ligand of OR2H2, increased the intracellular calcium and cAMP concentrations. Immunoblotting demonstrated that activation of OR2H2 by aldehyde 13-13 stimulated the CAMKKβ–AMPK–mTORC1–autophagy signaling axis, and that these effects were negated by OR2H2 knockdown. AMPK is known to regulate senescence; consequently, we investigated further the effect of aldehyde 13-13 on senescence. In H2O2-induced senescent cells, activation of OR2H2 by aldehyde 13-13 restored proliferation, and reduced the expression of senescence markers, P16 and P19. Additionally, aldehyde 13-13 induced apoptosis of H2O2-induced senescent cells, compared with non-senescent normal cells. In vivo, aldehyde 13-13 increased the lifespan of Caenorhabditis elegans and budding yeast. These findings demonstrate that OR2H2 is a functional receptor in VK2/E6E7 cells, and that activation of OR2H2 activates the AMPK–autophagy axis, and suppresses cellular aging and senescence, which may increase cellular health.


Introduction
Olfactory receptors (ORs), part of the G protein-coupled receptor (GPCR) superfamily, are primarily expressed in the cilia of olfactory sensory neurons where olfactory perception is initiated upon odorant binding to ORs.These receptors are also ectopically expressed RT-PCR and qPCR.OR1D2, OR2J3, OR2B6, and OR2H2 were expressed in VK2/E6E7 cells (Figure 1a).Among these, OR2H2 displayed the most significant expression.Immunocytochemistry illustrated that OR2H2 was localized to the cell membrane and the perinuclear region of the cytosol (Figure 1b).Approximately 13% of the OR2H2 signal overlapped with the phalloidin signal, indicating a significant presence of OR2H2 protein in the plasma membrane (Figure 1b, right panel).In second messenger assays, aldehyde 13-13 (a ligand for OR2H2) notably boosted intracellular calcium levels, unlike propionic acid (a ligand of OR51E2) and lactic acid (a ligand of Olfr78) (Figures 1c,d and S1).We subsequently delved deeper into the functionality of OR2H2 in VK2/E6E7 cells.Confirming earlier findings, aldehyde 13-13 instigated a robust intracellular Ca 2+ response in VK2/E6E7 cells (Figure 1c).When VK2/E6E7 cells were continuously exposed to aldehyde 13-13 (300 µM), there was a consistent decline in Ca 2+ levels, hinting at desensitization of the OR2H2-calcium signaling pathway (Figure 1d).We then explored whether the second messengers generated by aldehyde 13-13 were dependent on OR2H2.In cells where the OR2H2 gene was knocked down using OR2H2 siRNA, OR2H2 expression diminished by approximately 80% without affecting other ORs shown in Figure 1a.The OR2H2 siRNA left VK2/E6E7 cell viability unchanged (Figure 2A,B).While aldehyde 13-13 significantly upregulated intracellular cAMP and Ca 2+ concentrations, these effects were negated in cells with OR2H2 knocked down (Figure 2C,D).Collectively, these findings indicate that the impacts of aldehyde 13-13 on VK2E6E7 cells are mediated through OR2H2.

Results
2.1.Increases the Intracellular Ca 2+ and cAMP Levels in VK2/E6E7 Cells We began by examining ectopic OR expression in VK2/E6E7 cells.Based on GTEx analysis (https://gtexportal.org), ORs were chosen, and their expression was validated via RT-PCR and qPCR.OR1D2, OR2J3, OR2B6, and OR2H2 were expressed in VK2/E6E7 cells (Figure 1a).Among these, OR2H2 displayed the most significant expression.Immunocytochemistry illustrated that OR2H2 was localized to the cell membrane and the perinuclear region of the cytosol (Figure 1b).Approximately 13% of the OR2H2 signal overlapped with the phalloidin signal, indicating a significant presence of OR2H2 protein in the plasma membrane (Figure 1b, right panel).In second messenger assays, aldehyde 13-13 (a ligand for OR2H2) notably boosted intracellular calcium levels, unlike propionic acid (a ligand of OR51E2) and lactic acid (a ligand of Olfr78) (Figures 1c,d and S1).We subsequently delved deeper into the functionality of OR2H2 in VK2/E6E7 cells.Confirming earlier findings, aldehyde 13-13 instigated a robust intracellular Ca 2+ response in VK2/E6E7 cells (Figure 1c).When VK2/E6E7 cells were continuously exposed to aldehyde 13-13 (300 µM), there was a consistent decline in Ca 2+ levels, hinting at desensitization of the OR2H2calcium signaling pathway (Figure 1d).We then explored whether the second messengers generated by aldehyde 13-13 were dependent on OR2H2.In cells where the OR2H2 gene was knocked down using OR2H2 siRNA, OR2H2 expression diminished by approximately 80% without affecting other ORs shown in Figure 1a.The OR2H2 siRNA left VK2/E6E7 cell viability unchanged (Figure 2A,B).While aldehyde 13-13 significantly upregulated intracellular cAMP and Ca 2+ concentrations, these effects were negated in cells with OR2H2 knocked down (Figure 2C,D).Collectively, these findings indicate that the impacts of aldehyde 13-13 on VK2E6E7 cells are mediated through OR2H2.

Aldehyde 13-13 Increased the Intracellular Ca 2+ Level by Activating Multiple Calcium Channels
Intracellular Ca 2+ levels can be elevated either by influx from external sources or by releasing stored intracellular Ca 2+ from organelles such as the endoplasmic reticulum or mitochondria.To discern the origin of the Ca 2+ surge following aldehyde 13-13 treatment,

Aldehyde 13-13 Increased the Intracellular Ca 2+ Level by Activating Multiple Calcium Channels
Intracellular Ca 2+ levels can be elevated either by influx from external sources or by releasing stored intracellular Ca 2+ from organelles such as the endoplasmic reticulum or mitochondria.To discern the origin of the Ca 2+ surge following aldehyde 13-13 treatment, we conducted a calcium imaging test under Ca 2+ -free conditions.The ratiometric calcium imaging revealed no amplitude change during these calcium-free conditions.This suggests that the rise in intracellular Ca 2+ levels due to aldehyde 13-13 is not reliant on extracellular calcium but potentially originates from the internal calcium reservoir (Figure 3A).To pinpoint this source, VK2/E6E7 cells were simultaneously treated with Ca 2+ inhibitors and aldehyde 13-13.The Ca 2+ boost instigated by aldehyde 13-13 diminished in cells cotreated with an adenylyl cyclase III inhibitor (SQ22536), a PLC inhibitor (U73122), a SERCA inhibitor (thapsigargin), and a CNG channel inhibitor (L-cis diltiazem) (Figure 3B-E).Thus, aldehyde 13-13 amplifies intracellular Ca 2+ concentrations in VK2/E6E7 cells by engaging multiple Ca 2+ channels.we conducted a calcium imaging test under Ca 2+ -free conditions.The ratiometric calcium imaging revealed no amplitude change during these calcium-free conditions.This suggests that the rise in intracellular Ca 2+ levels due to aldehyde 13-13 is not reliant on extracellular calcium but potentially originates from the internal calcium reservoir (Figure 3A).

Activation of OR2H2 Induces the Calcium-CaMKKβ-AMPK Signaling Pathway
We next explored the signal transduction pathways influenced by OR2H2.In a phosphokinase array analysis evaluating the phosphorylation levels of 43 kinases, aldehyde 13-13 significantly enhanced the phosphorylation of AMPKα1 (Figure S2).Given that calcium signaling can trigger various components including CAMKKβ and considering that aldehyde 13-13 boosted AMPK phosphorylation in kinase array assays, CAMKKβ became our primary focus.CAMKKβ acts as an upstream kinase for AMPK.Upon aldehyde 13-13 stimulation, immunoblotting demonstrated the enhanced phosphorylation of both CaMKKß (an upstream kinase of AMPK) and AMPKα1, signifying OR2H2 activation (Figures 4A,B and S3a,b).AMPK plays a pivotal role in regulating cellular energy metabolism and homeostasis [18].Its activation is considered a prospective therapeutic target for metabolic disorders [19] and aging [20].AMPK exhibits diverse biological functions, predominantly activating the autophagy pathway through the phosphorylation inhibition of mTORC1 [21].Given that S6K and S6 are downstream signaling components of mTORC1, their phosphorylation was also examined.Immunoblotting revealed a significant decrease in phosphorylation levels of mTORC1, S6K, and S6 (a target of S6K) in VK2/E6E7 cells post aldehyde 13-13 treatment (Figures 4C-E and S3c-e).The ratios of phosphorylated-to-total mTOR, S6K, and S6 were notably diminished.Consequently, OR2H2 activation by aldehyde 13-13 stimulates the CaMKKß-AMPK-mTORC1 signaling pathway.

Activation of OR2H2 Induces Autophagy Pathways and Autolysosome Formation
The initiation of the AMPK-mTORC1 signaling route may induce cellular autophagy [14].Immunoblotting demonstrated an increased LC3-II to LC3-I ratio-a primary autophagosome formation marker-in cells treated with aldehyde 13-13 (Figures 5A and  S4), suggesting autophagy amplification upon OR2H2 activation.We assessed further the influence of aldehyde 13-13 on autophagic flux in VK2/E6E7 cells.Post-transfection with the mRFP-mGFP-LC3 tandem fluorescence-tagged vector, autolysosome generation was observed.This tandem fluorescence-tagged LC3 allows the differentiation of acidic

AMPK plays a pivotal role in regulating cellular energy metabolism and homeostasis [18].
Its activation is considered a prospective therapeutic target for metabolic disorders [19] and aging [20].AMPK exhibits diverse biological functions, predominantly activating the autophagy pathway through the phosphorylation inhibition of mTORC1 [21].Given that S6K and S6 are downstream signaling components of mTORC1, their phosphorylation was also examined.Immunoblotting revealed a significant decrease in phosphorylation levels of mTORC1, S6K, and S6 (a target of S6K) in VK2/E6E7 cells post aldehyde 13-13 treatment (Figures 4C-E and S3c-e).The ratios of phosphorylated-to-total mTOR, S6K, and S6 were notably diminished.Consequently, OR2H2 activation by aldehyde 13-13 stimulates the CaMKKß-AMPK-mTORC1 signaling pathway.

Activation of OR2H2 Induces Autophagy Pathways and Autolysosome Formation
The initiation of the AMPK-mTORC1 signaling route may induce cellular autophagy [14].

OR2H2-Dependent-AMPK-Autophagy Signaling Pathway Mediates Suppression of Cellular Senescence
We undertook OR2H2 knockdown experiments to validate the dependency of the CaMKKβ-AMPK-autophagy signaling on OR2H2.The OR2H2 mRNA level diminished by 80% in VK2 cells treated with OR2H2 siRNA (Figure 6a).In such conditions, aldehyde 13-13 did not affect the phosphorylation levels of CAMKKβ and AMPK, nor did it alter the LC3-II to LC3-I ratio in VK2/E6E7 cells (Figures 6b-d and S5a-c).This indicates that the activation of the CAMKKβ-AMPK-autophagy axis by aldehyde 13-13 is intrinsically linked to OR2H2 in VK2/E6E7 cells.

OR2H2-Dependent-AMPK-Autophagy Signaling Pathway Mediates Suppression of Cellular Senescence
We undertook OR2H2 knockdown experiments to validate the dependency of the CaMKKβ-AMPK-autophagy signaling on OR2H2.The OR2H2 mRNA level diminished by 80% in VK2 cells treated with OR2H2 siRNA (Figure 6a).In such conditions, aldehyde 13-13 did not affect the phosphorylation levels of CAMKKβ and AMPK, nor did it alter the LC3-II to LC3-I ratio in VK2/E6E7 cells (Figures 6b-d and S5a-c).This indicates that the activation of the CAMKKβ-AMPK-autophagy axis by aldehyde 13-13 is intrinsically linked to OR2H2 in VK2/E6E7 cells.

OR2H2 Activation Restored Senescence Induced by H2O2
Autophagy is a pivotal mechanism that counters cellular aging by upholding protein cellular homeostasis and discarding malfunctioning organelles and proteins [22].The inhibition of cellular aging typically correlates with rejuvenated cell proliferation and curtailed cellular senescence [23].Crucially, AMPK activation has been recognized to inhibit cellular senescence through multiple avenues.AMPK phosphorylates and restrains p27kip1, a key player in inducing apoptosis and senescence [15].Moreover, AMPK combats senescence via the activation of SIRT1 [16].In light of this, we examined the effect of aldehyde 13-13, which stimulates AMPK through OR2H2, on cellular senescence.
To delve deeper into OR2H2's influence on cellular aging and senescence, we observed the repercussions of aldehyde 13-13 on senescent VK2/E6E7 cells.These cells underwent senescence induction by oxidative stress (H2O2, 300 µM) for 3 days, with a preceding incubation with aldehyde 13-13 to discern its anti-senescent capabilities.Notably, OR2H2 expression tripled in senescent cells compared to their non-senescent counterparts (Figure 7A), implying heightened sensitivity of senescent VK2/E6E7 cells to aldehyde 13-13.

OR2H2 Activation Restored Senescence Induced by H 2 O 2
Autophagy is a pivotal mechanism that counters cellular aging by upholding protein cellular homeostasis and discarding malfunctioning organelles and proteins [22].The inhibition of cellular aging typically correlates with rejuvenated cell proliferation and curtailed cellular senescence [23].Crucially, AMPK activation has been recognized to inhibit cellular senescence through multiple avenues.AMPK phosphorylates and restrains p27kip1, a key player in inducing apoptosis and senescence [15].Moreover, AMPK combats senescence via the activation of SIRT1 [16].In light of this, we examined the effect of aldehyde 13-13, which stimulates AMPK through OR2H2, on cellular senescence.
To delve deeper into OR2H2's influence on cellular aging and senescence, we observed the repercussions of aldehyde 13-13 on senescent VK2/E6E7 cells.These cells underwent senescence induction by oxidative stress (H 2 O 2 , 300 µM) for 3 days, with a preceding incubation with aldehyde 13-13 to discern its anti-senescent capabilities.Notably, OR2H2 expression tripled in senescent cells compared to their non-senescent counterparts (Figure 7A), implying heightened sensitivity of senescent VK2/E6E7 cells to aldehyde 13-13.We also gauged the influence of aldehyde 13-13 on the proliferation capacity of senescent cells.A 1 h pre-treatment with aldehyde 13-13 nearly completely restored their proliferative potential, as denoted by Ki-67 immunocytochemistry, a cell proliferation marker (Figure 7B).Additionally, aldehyde 13-13 markedly lowered the expression of cellular senescence indicators, P16 INK4a and P21, in senescent cells (Figures 7C and S6).H2O2-induced senescence amplified the expression of senescence-associated ßgalactosidase and induced changes in cell morphology (Figure 7D).However, aldehyde 13-13 administration ameliorated the senescent morphological phenotype and decreased the number of cells positive for senescence-associated ß-galactosidase (Figure 7D).Thus, OR2H2 activation by aldehyde 13-13 appears to rejuvenate cell proliferation and mitigate the H2O2-induced senescence phenotype.

Aldehyde 13-13 Selectively Induced Apoptosis in Senescent Cells
Accumulation of senescent cells contributes to chronic diseases, tissue dysfunction, age-related ailments, and organ aging [24].Reducing the number of these cells might enhance tissue function and lower the risk of developing age-related diseases.Some senolytic compounds, like UBX0101, selectively target senescent cells by interfering with the p53 and MDM2 interaction [25].We subsequently examined the apoptotic effect of aldehyde 13-13 on senescent cells.Using flow cytometric analysis with Annexin V staining We also gauged the influence of aldehyde 13-13 on the proliferation capacity of senescent cells.A 1 h pre-treatment with aldehyde 13-13 nearly completely restored their proliferative potential, as denoted by Ki-67 immunocytochemistry, a cell proliferation marker (Figure 7B).Additionally, aldehyde 13-13 markedly lowered the expression of cellular senescence indicators, P16 INK4a and P21, in senescent cells (Figures 7C and S6).H 2 O 2induced senescence amplified the expression of senescence-associated ß-galactosidase and induced changes in cell morphology (Figure 7D).However, aldehyde 13-13 administration ameliorated the senescent morphological phenotype and decreased the number of cells positive for senescence-associated ß-galactosidase (Figure 7D).Thus, OR2H2 activation by aldehyde 13-13 appears to rejuvenate cell proliferation and mitigate the H 2 O 2 -induced senescence phenotype.

Aldehyde 13-13 Selectively Induced Apoptosis in Senescent Cells
Accumulation of senescent cells contributes to chronic diseases, tissue dysfunction, age-related ailments, and organ aging [24].Reducing the number of these cells might enhance tissue function and lower the risk of developing age-related diseases.Some senolytic compounds, like UBX0101, selectively target senescent cells by interfering with the p53 and MDM2 interaction [25].We subsequently examined the apoptotic effect of aldehyde 13-13 on senescent cells.Using flow cytometric analysis with Annexin V staining (Figure 8A), we found that the proportion of Annexin V positive cells remained unchanged in non-senescent cells treated with aldehyde 13-13.In contrast, the ratio increased significantly in senescent cells, suggesting aldehyde 13-13 might preferentially induce apoptosis in senescent cells compared to non-senescent ones (Figure 8A).(Figure 8A), we found that the proportion of Annexin V positive cells remained unchanged in non-senescent cells treated with aldehyde 13-13.In contrast, the ratio increased significantly in senescent cells, suggesting aldehyde 13-13 might preferentially induce apoptosis in senescent cells compared to non-senescent ones (Figure 8A).To understand this effect further, we analyzed the apoptotic marker, caspase 3, in both cell types through immunocytochemistry.In non-senescent cells, both the expression of P16 INK4a (a senescence marker) and caspase-3 levels remained unaffected by aldehyde 13-13 (Figure 8B).Thus, the colocalization of caspase-3 and P16 appeared consistent.However, in senescent cells, while P16 INK4a expression markedly increased, caspase-3 levels similarly rose.Notably, aldehyde 13-13 significantly amplified the colocalization of caspase-3 and P16 in these senescent cells (Figure 8B).These results indicate that aldehyde 13-13 boosts apoptosis in senescent cells, with negligible effects in their non-senescent counterparts.
The decrease in senescent cells might enhance tissue and overall organismal function, potentially impacting lifespan.Therefore, we investigated the influence of aldehyde 13-13 on the lifespan of C. elegans and budding yeast.Both organisms were treated with either ethanol or 10 mM aldehyde 13-13 at 20 °C.Remarkably, aldehyde 13-13 extended the lifespan of C. elegans by approximately a week in comparison to controls (Figure S7a).In budding yeast, aldehyde 13-13 doses (ranging from 100 to 500 µM) notably lengthened lifespan, as evidenced by propidium iodide staining (Figure S7b) and a colony-forming To understand this effect further, we analyzed the apoptotic marker, caspase 3, in both cell types through immunocytochemistry.In non-senescent cells, both the expression of P16 INK4a (a senescence marker) and caspase-3 levels remained unaffected by aldehyde 13-13 (Figure 8B).Thus, the colocalization of caspase-3 and P16 appeared consistent.However, in senescent cells, while P16 INK4a expression markedly increased, caspase-3 levels similarly rose.Notably, aldehyde 13-13 significantly amplified the colocalization of caspase-3 and P16 in these senescent cells (Figure 8B).These results indicate that aldehyde 13-13 boosts apoptosis in senescent cells, with negligible effects in their non-senescent counterparts.
The decrease in senescent cells might enhance tissue and overall organismal function, potentially impacting lifespan.Therefore, we investigated the influence of aldehyde 13-13 on the lifespan of C. elegans and budding yeast.Both organisms were treated with either ethanol or 10 mM aldehyde 13-13 at 20 • C. Remarkably, aldehyde 13-13 extended the lifespan of C. elegans by approximately a week in comparison to controls (Figure S7a).In budding yeast, aldehyde 13-13 doses (ranging from 100 to 500 µM) notably lengthened lifespan, as evidenced by propidium iodide staining (Figure S7b) and a colony-forming unit assay (Figure S3c).These findings collectively suggest that aldehyde 13-13 enhances the lifespan of both budding yeast and C. elegans.

Discussion
Ectopic olfactory receptors perform varied functions across diverse organs and tissues [5,26,27].Given that genital organs are consistently exposed to odorants, ectopic olfactory receptors might influence intracellular signaling pathways and associated physiological processes in these organs.In this study, we delved into the role of OR2H2 in VK2/E6E7 human vaginal epithelial cells.
Currently, three extant studies discuss the functionality of ectopic OR2H2, pointing to its tissue-specific roles.In human myoblasts, OR2H2 elevates the intracellular calcium concentration and diminishes myoblast fusion via Phosphoinositide 3-kinase signaling [9].In the thyroid gland, OR2H2 expression decreases in malignant cells, compared to surrounding healthy tissues.Aldehyde 13-13 inhibits the proliferation of thyroid cancer cells [28].The single nucleotide polymorphism of OR2H2, rs123388, is linked to celiac disease in patients from Indian and Dutch populations [29].This polymorphism, along with five others, is associated with immune functions and Toll-like receptor signaling pathways [29].Such findings indicate the significance of OR2H2 in gut and immune cells.Furthermore, we discerned a new function of OR2H2 in VK2/E6E7 cells.OR2H2 activation by aldehyde 13-13 energized the Ca 2+ -CAMKKβ-AMPK-autophagy signaling pathway, curbing cellular senescence via a senolytic effect (Figure 9).unit assay (Figure S3c).These findings collectively suggest that aldehyde 13-13 enhances the lifespan of both budding yeast and C. elegans.

Discussion
Ectopic olfactory receptors perform varied functions across diverse organs and tissues [5,26,27].Given that genital organs are consistently exposed to odorants, ectopic olfactory receptors might influence intracellular signaling pathways and associated physiological processes in these organs.In this study, we delved into the role of OR2H2 in VK2/E6E7 human vaginal epithelial cells.
OR2H2 activation stimulated autophagy.Metrics such as the LC3-II-to-LC3-I ratio, MDC staining, autophagic flux analysis, and transmission electron microscopy all depicted enhanced autophagy and the progression of autophagic turnover from the autophagosome to autolysosome in VK2/E6E7 cells.Autophagy stands at the crossroads of metabolic and proteostatic signaling, dictating key aging mechanisms and organism lifespan [34].A decline in autophagic activity is believed to lead to the buildup of damaged organelles and macromolecules with aging, whereas sustaining adequate autophagic activity aids in life extension [35].AMPK spurs autophagy either directly or indirectly through mTORC1 suppression or SIRT-1 activation.Indeed, AMPK oversees the aging process via an interconnected signaling network [36].
AMPK is a central regulator of energy metabolism and homeostasis, influencing the aging process through interactions with several signaling networks [37].Enhanced AMPK activity potentially promotes healthspan and lifespan by mitigating cellular stress.This enhancement is achieved by activating signaling molecules such as FoxO/DAF-16, Nrf2/SKN-1, and SIRT1, stimulating the autophagic pathway via mTOR signaling, and restraining proinflammatory responses by inhibiting NF-κB signaling [36].As AMPK activity diminishes with age, its increased activity might extend the lifespan of simpler organisms.
Aldehyde 13-13 extended the lifespan of both C. elegans and budding yeast, potentially through the AMPK-autophagy pathway.However, neither C. elegans nor budding yeast have OR2H2 homologs.As such, pinpointing the target receptor and the signaling mechanisms of aldehyde 13-13 requires further exploration.We hypothesize that in organisms like C. elegans and yeast, aldehyde 13-13 might counteract aging through analogous (rather than homologous) mechanisms compared to the OR2H2-dependent pathway in human cells.However, the specific anti-aging action of aldehyde 13-13 on C. elegans and yeast remains elusive.In humans, OR2H2, being a receptor for aldehyde 13-13, might offer therapeutic avenues for mitigating the aging of human vaginal epithelial cells.This is evidenced by the fact that Ca 2+ and cAMP signaling via aldehyde 13-13 was specifically observed in OR2H2-expressing VK2/E6E7 cells.This potential therapeutic approach could extend to other human tissues expressing OR2H2, a possibility we aim to probe further.
AMPK maintains cellular energy balance and combats senescence [38,39].For instance, aging skeletal muscle stem cells (MuSCs) exhibit diminished autophagy, augmented apoptosis, and reduced phosphorylation of AMPK and its downstream target, p27 Kip1 [15].Activating AMPK in aged MuSCs in vitro curtailed apoptosis, boosted proliferation, and enhanced transplantation efficiency in vivo.Additionally, the AMPK/p27Kip1 pathway activation lowered senescence markers in older cells, partially relying on p27 Kip1 phosphorylation.Hence, the AMPK/p27 Kip1 pathway might modulate the autophagy/apoptosis equilibrium in aged MuSCs, serving as a prospective target for enhancing muscle regeneration in older adults.Our results indicate that the OR2H2-AMPK-autophagy pathway activation diminishes cellular senescence in VK2/E6E7 cells.To the best of our knowledge, this constitutes the pioneering assertion that ectopic olfactory receptors can impede aging and cellular senescence.

Cell Culture
VK2/E6E7 cells (ATCC, CRL-2616) were purchased from the American Type Culture Collection (ATCC, VA, USA), and cultured in keratinocyte-serum free medium (Gibco, New York, USA, 17005042), supplemented with 0.1% human recombinant epidermal growth factor, 0.3% bovine pituitary extract, and 0.4 mM calcium chloride as instructed in the manufacturer's protocol.Culture medium was renewed every 2-3 days.Cells were grown in 37 • C with 5% CO 2 .All compounds except L-Cis diltiazem (Abcam) and aldehyde 13-13 (Henkel) were prediluted in DMSO.L-Cis diltiazem was prediluted in distilled water and aldehyde 13-13 in ethanol.All compounds were diluted 1:1000 in growth medium or Ringer's solution and applied to VK2/E6E7 cells.All dilutions of aldehyde 13-13 were prepared fresh before use.

RNA Extraction and RT-PCR
Total cellular RNA was extracted with Total RNA extraction reagent RNAiso Plus (1 mL, Takara Bio, 9109, Japan) according to the manufacturer's instructions.Complementary DNA was synthesized from 1 µg RNA with ReverTra Ace ® RT Master Mix kit (Toyobo, Osaka, Japan, FSQ-301) according to the manufacturer's instructions.One µg of cDNA was then used as a template for PCR reactions and specific primers were designed by the Primer-BLAST designer program (NCBI, Bethesda, MD, USA).RT-PCR was performed with EmeraldAmp ® GT PCR Master Mix reagent according to the manufacturer's instructions.The RT-PCR products were analyzed by agarose gel electrophoresis (3%) and image analysis was obtained by using a ChemiDoc touch imaging system with the Image Lab 5.2 software (Bio-Rad, Redmond, WA, USA).L32 was used to normalize the data.

Real Time qPCR
After a 24 h treatment in 6-well plates, total cellular RNA was extracted using the RNAiso Plus reagent (Takara Bio, Shiga, Japan), following the manufacturer's guidelines.Complementary DNA (cDNA) was synthesized from 1 µg of RNA using the ReverTra Ace ® RT Master Mix kit (FSQ-301; Toyobo, Japan), again adhering to the manufacturer's protocol.An amount of 1 µg of the resultant cDNA was utilized as a template for the polymerase chain reaction (PCR).Specific primers were crafted using the Primer-BLAST designer tool (NCBI, Bethesda, MD, USA).The cDNA was then subjected to PCR using the iQ5 i-Cycler system (Bio-Rad Laboratories, Hercules, CA, USA) and the Thunderbird SYBR ® qPCR Mix reagent (T00PS-201; Takara Bio).Amplification parameters for the cDNA included an initial 30 s denaturation at 95 • C, 40 cycles of 10 s denaturation at 95 • C, 20 s annealing at 59 • C, and 20 s extension at 68 • C. The fluorescent signal was quantified automatically post each PCR cycle.Gene expression was determined from the threshold cycle (Ct value), and L32 was employed for normalization.The oligonucleotide sequences can be found in Supplementary Table S1.

OR2H2 Immunocytochemical Staining
Immunocytochemical staining was carried out using immunofluorescence microscopy.VK2/E6E7 cells were placed on coverslips inside a 24-well plate, containing 500 µL of cell culture medium, and incubated at 37 • C in a 5% CO 2 environment.Upon reaching 80% confluence, the medium was discarded, and the cells were rinsed with PBS.Postfixation in ice-cold acetone, cells were treated with both primary (1:100, anti-OR2H2; Antikorperonline.de) and secondary antibodies (1:1000, goat anti-rabbit 546; Thermo Fisher, Carlsbad, CA, USA).Subsequently, cells were exposed to Alexa Fluor phalloidin 488 (1:200, Thermo Fisher) for 45 min at ambient temperature with gentle agitation.The cells were then sealed with Immu-Mount solution (Thermo Fisher) and inspected under an LSM 510 Meta Confocal Microscope (Carl Zeiss, Jena, Germany) employing a 40× oil immersion objective and the Leica Application Suite X Software.The specificity of the antibodies utilized was previously ascertained by rho-tagged transfection of Hana3A cells [40].

Calcium Imaging and Calcium Inhibitor Treatments
Intracellular calcium concentration changes were monitored using the fluorescent dye Fura-2-acetoxylmethyl ester (Fura-2/AM; Invitrogen).VK2/E6E7 cells were cultured in 35 mm dishes and incubated in growth medium containing 3 µM Fura-2/AM for 30 min at 37 • C, protected from light.Next, growth medium was replaced with Ringer's solution.Aldehyde 13-13 and calcium inhibitors were dissolved in Ringer's solution (1:1000) and applied directly to the cells.In desensitization experiments, the cells were stimulated repetitively with aldehyde 13-13 (300 µM) for 2 min while control cells were treated with vehicle (ethanol in Ringer's solution) repeatedly for 2 min.In experiments under calciumfree conditions, cells were stimulated with aldehyde 13-13 (500 µM) for 3 min, then washed for 3 min with Ringer's solution.Cells were then treated with calcium-free Ringer's solution for 7 min, and then aldehyde 13-13 was added for 3 min.A third application of aldehyde 13-13 was performed for 3 min.In experiments with calcium channel inhibitors, cells were stimulated with aldehyde 13-13 (500 µM) for 3 min.After 2 min washing with Ringer's solution, the cells were stimulated with the calcium channel inhibitors.Subsequently, aldehyde 13-13 and inhibitors were co-applied for 3 min.A third application was also prepared under normal conditions after a 2 min wash-out step.Calcium channel inhibitors were incubated under the following conditions: SQ 22536 (10 µM) for 10 min; L-cis diltiazem (100 µM) for 3 min; U 73122 (5 µM) for 5 min; thapsigargin (5 µM) for 25 min.Intracellular calcium flux was observed using a DMI, 6000CS inverse microscope (Leica, Wetzlar, Germany), and calcium-dependent fluorescence changes were detected using a 10-fold fluorescence objective.Fluorescence emission intensities (340 and 380 nm) were detected by a DFX 360FX CCD camera (Leica).Regions of interest (ROIs) were analyzed using Advanced Fluorescence software LASX Office 1.4.5 27713 (LAS AF; Leica).

Phosphokinase Array
The human phosphokinase array kit by RnD systems was applied to investigate the phosphorylation of 43 different kinases under the influence of aldehyde 13-13 stimulation for an incubation time of 30 min.Before starting the array, according to the manufacturer's instructions, protocol cells were cultivated in 75 cm 2 culture flasks until a confluence of 90% was achieved.Medium was exchanged with fresh medium containing the diluted aldehyde 13-13 in a concentration of 500 µM.The control was treated with ethanol (<0.1%).After incubation, medium was aspirated, cells were covered with PBS and manually detached with a cell scraper.The detached cells were then subsequently taken up in the PBS and centrifuged for 10 min at 1000 rpm and 4 • C. The cell pellets thus obtained were then lysed in RIPA buffer and their protein concentration was determined using the Pierce TM BCA protein assay kit.The total amount of protein was 250 µg for the treated and untreated samples.The evaluation of the membrane was performed by the chemiluminescence System Fusion SL 3500-WL.The intensity of the individual array dots was analyzed with the program Image J and a microarray plugin and normalized to the control.

OR2H2 Knockdown
For mRNA interference of OR2H2, VK2 cells (4 × 10 5 ) were seeded in six-well plates and transfected with a siRNA against OR2H2 (Cat No. sc-95450; Santa Cruz Biotechnology, Inc.) using Lipofectamine 2000 according to the manufacturer's instructions.Briefly, cells were cultured with siRNA and Lipofectamine 2000 in Opti-MEM reduced-serum medium (Cat No. 32985070; Gibco, New York, NY, USA).After incubation for 5 h at 37 • C in a CO 2 atmosphere, medium was removed, and cells were incubated for 19 h in serum-containing medium at 37 • C. To verify transfection, VK2 cells transfected with fluorescein-conjugated control siRNA (Cat No. SN1021; Bioneer, Dae-Jeon, Republic of Korea) were harvested.Intracellular fluorescence intensity was measured using a flow cytometer equipped with an FL1 detector (BD Biosciences, Franklin Lakes, NJ, USA).

Cell Viability Assay
The viability of siRNA-transfected VK2/E6E7 cells was assessed using a 2,5-diphenyl-2H-tetrazolium bromide (MTT) assay [41].Cells were seeded at a density of 1 × 10 4 cells per well in 96-well culture plates and were allowed to adhere overnight.The following day, the culture medium was discarded and replaced with a medium containing 10% MTT (Sigma Aldrich).Cells were then incubated for 3 h at 37 • C. Afterward, the MTT solution was carefully removed from each well, and dimethyl sulfoxide (DMSO; Bio Basic Inc., Markham, ON, Canada) was added to dissolve the formazan crystals.The absorbance of each sample was subsequently measured at 570 nm using a microplate spectrophotometer (Multiskan Go; Thermo Fisher Scientific).

Immunoblot Analysis
Total cellular proteins were extracted using radioimmunoprecipitation assay buffer supplemented with Halt protease and phosphatase inhibitor reagent (Thermo Fisher Scientific, Carlsbad, CA, USA).Total cellular proteins were centrifuged for 20 min at 12,000 rpm to obtain the soluble protein fraction.Protein concentration was measured using a protein assay dye reagent concentrate (Bio-Rad).Denatured proteins were run on a sodium dodecyl sulfate-polyacrylamide gel, and transferred to nitrocellulose membranes (GVS Filter Technology, Morecambe, UK).The membranes were blocked in TBS with 5% (w/v) non-fat dried milk for 1 h at room temperature.The primary antibodies were diluted in TBS-Tween 20 (0.1%) with 5% (w/v) non-fat dried milk.The secondary antibodies were diluted in TBS with 0.1% Tween-20.Immunoblot images were obtained using the ChemiDoc Touch Imaging System and analyzed with Image Lab 5.2 software (Bio-Rad).Protein levels were normalized with β-actin after stripping the identical blot using stripping buffer (Dyne Bio, CBS3180, Seong-Nam, Republic of Korea).

mRFP-GFP-LC3 Puncta Formation Assay
VK2/E6E7 cells (2 × 10 5 ) were seeded in a six-well confocal plate.After 24 h, cells were transfected with 1.5 ng of mRFP-GFP-LC3 plasmid using DharmaFECT transfection reagent (Horizon Discovery, Cambridge, UK) as per the manufacturer's instructions and incubated for 48 h.Next, cells were treated with ethanol (control) or 500 µM aldehyde 13-13 for 30 min.Cells were washed once with PBS and fixed with 4% paraformaldehyde for 10 min.mRFP and GFP fluorescent puncta were observed under an LSM510 META confocal microscope and images were analyzed with LSM700 version 3.2 software (Carl Zeiss, Jena, Germany).

Monodansylcadaverine Staining Assay
VK2/E6E7 cells were seeded in a black or clear 96-well plate at 1 × 10 4 per well.After 24 h, cells were treated with ethanol, rapamycin (100 nM), or aldehyde 13-13 (500 µM) for 30 min and autophagy vacuoles were stained using a monodansylcadaverine (MDC) staining kit (Cayman, Ann Arbor, MI) as per the manufacturer's protocol.Autophagy vacuoles were detected under a fluorescence microscope (Nikon Eclipse Ti) and images were analyzed using NIS-elements F software (Nikon Instruments, Inc., New York, NY, USA).

Autophagy Analysis by Transmission Electron Microscopy
VK2 cells (5 × 10 6 ) were cultured in 175T flasks for 24 h and treated with aldehyde 13-13 (500 µM) for 30 min.For TEM, cells were fixed with Karnovsky's fixative and stored at 4 • C overnight.Cells were post-fixed with 1% osmium tetroxide and stained with 0.5% uranyl acetate overnight followed by dehydration in an ethanol gradient.The cells were infiltrated with Spurr's resin overnight and visualized using a JEM1010 electron microscope at 120 kV (JEOL, Tokyo, Japan).

Annexin V and Propidium Iodide Staining
Cells were seeded in a six-well plate at 3 × 10 5 /well and grown for 24 h.Proliferating cells were treated with vehicle and 40 µM aldehyde 13-13.Senescent cells were cotreated with 200 µM H 2 O 2 plus vehicle and aldehyde 13-13.Next, cells were stained and incubated with 3 µL Annexin-V-FITC (BD Biosciences, CA, USA) and 10 µL propidium iodide (BD Biosciences, CA, USA) for 20 min and apoptosis analysis was performed using Accuri C6 Plus FACS (BD Biosciences).

Measurement of Chronological Lifespan by PI Staining and Flow Cytometry
Yeast cells were harvested by centrifugation, washed by resuspending in 1 mL of phosphate-buffered saline (PBS) and incubated for 20 min at 30 °C after adding 5 µL of PI solution (1 mg/mL, Sigma Aldrich).Stained cells were analyzed using a flow cytometer (FACS Verse; Becton Dickinson) with excitation at 488 nm and emission at 585 nm.Approximately 20,000 cells were analyzed per sample, and data were analyzed using Cell Quest software v3.3 (Becton Dickinson).

Colony-Forming Unit Assay of Budding Yeast
A colony-forming unit (CFU) assay was performed to determine yeast viability.Yeasts were harvested, serially diluted in PBS, counted using a hemocytometer, and 200 cells were spread onto YPD agar and incubated at 30 • C until colony formation.

Caenorhabditis elegans (C. elegans) Longevity Assay
C. elegans strains were cultured on fresh NGM plates for 2-3 generations without starvation, and lifespan analysis was conducted at 20 • C. Worms were synchronized by isolating eggs from gravid adults using hypochlorite and NaOH.When worms reached the L4 stage, 2 -deoxy-5-fluorouridine (FUdR, 0.6 mM) was added to prevent internal hatching.Aldehyde 13-13 (10 mM) was added to each well along with OP50 on the first day of the lifespan assay.Ethanol (0.1%) was vehicle in the control group.Wells containing > 15 worms were excluded from the analysis because of the risk of dietary restriction.Worm movement was used to determine whether the animals were alive or dead.Survival curves were analyzed by the log-rank (Mantel-Cox) method.

Statistical Analysis
Results are means ± standard error of the mean (SEM).To generate dose-response curves, SigmaPlot 10.0 was used, and curves were fitted using the Hill three-parameter equation.Significance was examined by two-tailed unpaired t-test.Data were subjected to oneway ANOVA followed by Tukey's HSD test or Student's t-test for multiple or two-group comparisons.Different letters indicate a significant difference at p < 0.05 (ANOVA).

Conclusions
In non-senescent cells, aldehyde 13-13 heightened autophagy by AMPK activation and, in senescent cells, increased cell proliferation while inducing apoptosis, thus reducing senescence (Figure 9).Our data from VK2/E6E7 cells suggest that aldehyde 13-13 might enhance cellular health and counteract aging in the human vaginal epithelium through AMPK activation.AMPK appears to hold pivotal roles in cellular senescence and apoptosis.For instance, in mouse embryonic fibroblasts, removing AMPKα2 accelerates cellular senescence and cell cycle arrest triggered by oxidative stress-induced senescence [42].Activation of AMPK by specific molecules can drive cancer cell apoptosis.This process stimulates apoptosis by inhibiting AKT and COX-2, repressing mTORC1, and modulating P53 and P21.Our cumulative data show that aldehyde 13-13 activates OR2H2 in VK2/E6E7 cells, induces the AMPK-autophagy pathway, curtails cellular senescence while promoting

Figure 1 .
Figure 1.OR2H2-mediated increase in intracellular Ca 2+ level in VK2/E6E7 cells: (a) Expression of OR2H2 and other ORs in VK2/E6E7 cells determined by RT-PCR."-" represents a negative control without reverse transcriptase during cDNA synthesis.Experiments were conducted in triplicates, denoted as 1, 2, and 3 in the gel images.(b) OR2H2 expression in VK2/E6E7 cells observed through