Abstract
Aging is a primary risk factor for cognitive impairment and exacerbates multiple biological processes in the brain, including but not limited to nutrient sensing, insulin signaling, and histone deacetylation activity. Therefore, a pharmaceutical intervention of aging that targets distinct but overlapping pathways provides a basis for testing combinations of drugs as a cocktail. Our previous study showed that middle-aged mice treated with a cocktail of rapamycin, acarbose, and phenylbutyrate for 3 months had increased resilience to age-related cognitive decline. This finding provided the rationale to investigate the transcriptomic and molecular changes within the brains of mice that received this cocktail treatment or control treatment. Transcriptomic profiles were generated through ribonucleic acid (RNA) sequencing, and pathway analysis was performed by gene set enrichment analysis to evaluate the overall RNA message effect of the drug cocktail. Molecular endpoints representing aging pathways were measured using immunohistochemistry to further validate the attenuation of brain aging in the hippocampus of mice that received the cocktail treatment, each individual drug or control. Results showed that biological processes that enhance aging were suppressed, with an increased trend of autophagy in the brains of mice given the drug cocktail. The molecular endpoint assessments indicated that treatment with the drug cocktail was overall more effective than any of the individual drugs for relieving cognitive impairment by targeting multiple aging pathways.
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Introduction
Aging is a complex process involving the change of multifactorial pathways in all organs of the body including the brain. Aberrant progression of several critical pathways accelerates biological aging. Pathways including mammalian target of rapamycin (mTOR) signaling, insulin signaling, and histone deacetylation [1] are respectively and individually targeted by rapamycin (Rap), acarbose (Acb), and phenylbutyrate (Pba), with each drug shown to have anti-aging effects in mice [2,3,4,5,6]. A combination of these three drugs as a cocktail would be expected to result in a more robust outcome on preventing or slowing aging in the brain due to targeting multiple aging pathways [7].
Rap is an antibiotic clinically approved for treating organ transplant patients and neoplastic conditions [8, 9]. It has a high oral bioavailability and readily crosses the blood brain barrier. Rap blocks mTOR1, a protein shown to integrate signals from growth factors and nutrients to control protein synthesis [10]. Mechanistically, Rap downregulates mTOR1 signaling, leading to a phenocopy of caloric restriction [11]. Previous studies demonstrated that Rap feeding increased lifespan even when started late in life in both male and female mice [12, 13]. Acb is a common type 2 diabetes medication used for glucoregulatory control by delaying the digestion of complex carbohydrates. Specifically, Acb reversibly inhibits α-glucosidases within the intestinal brush border and promotes postprandial blood glucose regulation [14]. A previous study showed long-term treatment with Acb in heterogeneous background mice extended both median and maximum lifespan [4]. Pba is clinically approved as an ammonia scavenger for urea cycle disorders in children and acts as a broad inhibitor to class I and II histone deacetylases, which enhance histone acetylation and protein folding as well as decrease endoplasmic reticulum stress [15]. Extensive studies have demonstrated that increases in histone acetylation globally elevate transcription, which can be beneficial at old age as it contributes to the reversion of age-dependent decline in stress response, deoxyribonucleic acid (DNA) repair, and other genes involved in the maintenance of homeostasis [15, 16]. However, it is noteworthy that, unlike Rap and Acb, which have been shown to extend lifespan in various models, Pba did not demonstrate an increase in lifespan in mice [17].
Middle-aged mice treated for 3 months with a drug cocktail consisting of Rap, Acb, and Pba showed improvements in multiple aspects of health span including significant delays in the appearance of cognitive impairment and enhanced motor coordination [18]. In this study, we showed that mice treated with the drug cocktail had significantly better performance, with a more robust effect than any individual drug. It was therefore posited that the drug cocktail was able to retard brain aging by targeting multiple biological processes. While behavioral and physiological evidence was provided in prior studies, effects of the drug cocktail treatment on the specific processes and biological pathways have not yet been identified and evaluated. To investigate the pathways and molecular targets of brain aging in mice treated with drug cocktail or control, multivariate discriminant analysis was conducted for this study.
In order to identify age-associated pathways altered by the cocktail in the brain, transcriptomic profiles were explored through RNA sequencing. We report that the drug cocktail targeted mTOR1 signaling, insulin signaling, and histone deacetylase binding, which represent three major pathways of aging. Additional pathways of aging were also observed to be targeted by the drug cocktail including DNA damage, inflammation, senescence, and autophagy. Validation of these transcriptomic endpoints was done using immunohistochemistry to demonstrate expression levels of corresponding proteins.
Methods
Mouse brain tissue
All tissues used for this study were obtained from archived brain samples of a National Institute on Aging (NIA) funded preclinical drug study, which compared aging phenotypes between the drug cocktail diet treated C57BL/6 mice with mice receiving individual drug diet or control diet [18]. In this study, both female and male mice received cocktail diet, each individual drug or placebo (control) chow. Treatment began at 20 months of age and lasted for 3 months until 23 months of age (Fig. 1). Mice treated with the drug cocktail were consistently cognitively similar to 8-month-old untreated mice compared to older mice treated with each individual drug or untreated older mice.
Nonfasted mice were euthanized via carbon dioxide asphyxiation followed by decapitation. All procedures were approved by the University of Washington IACUC as previously reported (Jiang et al., 2022). Brains were harvested and collected within 2 min of decapitation. Brains were sectioned sagittally through the midline. The parietal-temporal lobe from the left sagittal hemisphere was extracted into a sterilized vial and snap-frozen using liquid nitrogen before being transferred to a −80 °C freezer for long-term storage. The right sagittal hemisphere was fixed in 10% neutral buffered formalin (NBF) for 72 h then embedded in paraffin wax through the University of Washington Department of Comparative Medicine’s Histology Lab.
RNA-seq
Total RNA was extracted from homogenized parietal-temporal lobe tissue of three randomly chosen drug cocktail-treated mice and three control mice using RNeasy kits (Qiagen, Redwood City CA). RNA purity was measured by Nanodrop spectrophotometer, and RIN value was obtained through 2100 Bioanalyzer. Library construction and sequencing were done through Quick Biology Inc. (Monrovia CA), using the high throughput genome sequencing platform NovaSeq 6000 with 15M paired reads. In brief, the raw RNA-seq data (SRA database PRJNA1012002) went through FASTQ quality control and cleanup and was aligned to the University of California San Diego (UCSD) C57BL/6 mice RNA data bank for further analysis.
Quantitative reverse transcription PCR (q-PCR)
RNA preparation for q-PCR was performed in the same manner as for RNA-seq. cDNA samples were generated by OligodT (High-capacity cDNA Reverse Transcription Kit; Thermo-Fisher Cat. 4368813) reverse transcription using 5ng RNA following the manufactural standard protocol. qPCR was carried out using SYBR Green Master Mix (PowerTrack SYBR Green Master Mix, Thermo-Fisher Cat. A46109) and primer pairs. β-actine was selected as a house-keeping gene for quantification, and all q-PCR results were analyzed through the ΔΔCt method. Primer sequences are listed as follows: Cdkn2a (p16Ink4a) Fwd 5′-CCCAACGCCCCGAACT-3′, Cdkn2a (p16Ink4a) Rev 5′-GCAGAAGAGCTGCTACGTGAA-3′; β-actine Fwd 5′-CACCATTGGCAATGAGCGGTTC-3′, β-actine Rev 5′-AGGTCTTTGCGGATGTCCACGT -3′.
Gene set enrichment analysis (GSEA)
The DESeq2 R package [19] was used for preparing differential expression transcriptome data across all sequencing cohorts. GSEA (RRID:SCR_003199) is a useful tool to interpret high throughput expression studies and identify insights into biological pathways underlying a given phenotype [20, 21]. The GSEA algorithm scores a gene set according to how the genes in it represent increases or decreases on average in response to the regulation strength. The groups of pathways selected for GSEA analysis were predefined by previous studies [1] as major pathways of mammalian aging. Reference gene sets were extracted through Gene Ontology (GO) or Kyoto Encyclopedia of Genes and Genomes (KEGG) and Gene Ontology Molecular Function (GOMF) databases with strong validation from previous literature. For GSEA, mouse gene symbols were remapped to human gene orthologs. The GSEA analysis was done using GSEA software [20, 21] version 4.2.1, and the database was derived from the Molecular Signatures Database v5.0 [20, 22]. GSEA was based on the K-S test which weighs each observed gene within the gene set based on a given cumulative density function.
Immunohistochemistry (IHC)
Brain tissues were randomly selected from each group. Brains from 8-month-old mice were measured for each tested endpoint as an untreated young control. Four-micrometer formalin-fixed paraffin-embedded unstained slides were used for staining. Slides were rehydrated with xylene and a series of decreasing concentrations of ethanol in water. Slides then went through 20 min of heat-mediated antigen retrieval (98 °C) in citric acid buffer (pH 6.0). Slides stained with P21 as primary antibody were immersed in ethylenediaminetetraacetic acid (EDTA) buffer (pH 8.0) for antigen retrieval. Sections were then blocked with endogenous peroxidase plus 3% H2O2, serum, avidin, and biotin blocking reagents (HRP-DAB Cell & Tissue Staining Kit, R&D Systems, Minneapolis MN) and washed in Tris-buffered saline (TBS) with 0.1% Tween 20 (TBST) in between each blocking step. Sections were then incubated in primary antibodies diluted in TBST solution overnight in a 4 °C humidified chamber. The dilution concentration for each antibody is as follows: HDAC2 (rabbit polyclonal to HDAC2, Abcam, Boston MA, Cat. ab1793, RRID: AB_305706) 1:500, MCP1 (rabbit polyclonal to MCP1, Novus Biologicals, Centennial CO, Cat. NBP1-07035, RRID: AB_1625612) 1:200, TNFα (mouse monoclonal to TNFα, Abcam, Cat. ab1793, RRID: AB_302615) 1:400, ATG5 (rabbit polyclonal anti-ATG5, Novus Biologicals, Cat. NB110-53818, RRID: AB_828587) 1:500, IL6 (rabbit polyclonal to IL-6, Abcam, Cat. ab208113, RRID: AB_2927421) 1:400, P21 (rabbit monoclonal to p21, Abcam, Cat. ab188224, RRID: AB_2734729) 1:50, and γH2AX (rabbit monoclonal to gamma H2A.X, Abcam, Cat. ab26350, RRID: AB_470861.) 1:500. Slides were rinsed thoroughly before incubating in a biotinylated secondary antibody for 30 min at room temperature. After the washing step, sections were incubated with conjugated high sensitivity streptavidin horseradish peroxidase for 30 min followed by washing steps. 3,3′-diaminobenzidine chromogen was applied to slides for 20 min until the desired intensity of staining was reached. Slides were then dehydrated and mounted for imaging and analysis.
QuPath analysis
IHC slides were photographed under a Nikon Eclipse microscope with a Nikon D7100 camera. All photos were taken under a magnification of ×40 for capturing the entire area of the hippocampus across brain tissue slides from five randomly chosen mice per treatment group. Qupath (RRID:SCR_018257) version v2.0 was used for positive stained cell identification and optical density quantification [23]. The background staining threshold red green blue (RGB) values were calibrated consistently on sections treated with the same primary antibody regardless of specimen cohort conditions. The hippocampus was annotated with the polygon wand tool to selectively measure the staining expression within the desired region. Cellular parameters for positive staining detection were fixed based on antibody detection properties. Detected cells were calibrated and quantified by RGB-based superpixel clustering. The quantification indicated the average optical density for each detectable cell within the annotated region. An intensity heat map reflecting the staining quantification was generated for visualization purposes. Heat map gradients were adjusted to represent the intensity level across all stained slides that received the same primary antibody.
Statistics
All numerical data analyses were conducted in Prism (GraphPad Software, La Jolla CA, RRID:SCR_002798). Two-way analysis of variance (ANOVA) followed by Tukey’s post hoc test was used to compare the population difference between cohorts. p-value ≤ 0.05 was considered statistically significant and presented as mean ± standard of mean (SEM). For GSEA, lists of ranked genes based on a score calculated by the K-S test as −log10 of p-value multiplied by fold-change, either upregulated or downregulated. Enrichment score (ES) was calculated by the difference between 0 and the extremes of the entire ranked gene list. The normalized enrichment scores reflected default parameters with ES over the average of positive to negative extremes within the gene set [20].
Results
The brains from mice treated with a cocktail of Rap, Acb, and Pba showed downregulation of transcriptomic profiles targeted by each individual drug
The parietal-temporal lobe with hippocampus from mice treated with cocktail or control chow was randomly selected for RNA-seq. Total RNA that was purified from homogenized tissue with hippocampus was utilized. Three pathways associated with each individual drug were suppressed significantly in the brains of mice that received the drug cocktail (Fig. 2).
The Rap-medicated reduction on mTOR1 signaling was reflected by the enhanced expression of downregulating genes. As an anabolic signaling kinase, active mTOR1 translates to rapid cell growth and proliferation. Emerging studies support the idea that lower mTOR1 activity leads to decreased nutrient signaling and extends longevity [24]. The overall insulin signaling referenced to the KEGG database was negatively regulated by the cocktail through enrichment of downregulating or suppressing genes. Insulin signaling is one of the most conserved aging-controlling pathways in evolution [24,25,26]. In addition to the beneficiary effect from Rap, Acb promotes glucoregulatory control and improves glucose homeostasis and insulin sensitivity. Current evidence suggests that interventions that constitutively decreased insulin signaling may prevent or reverse the adverse effects associated with aging [27]. Here, induced downstream effectors were seen in the histone deacetylase binding pathway for cocktail-treated mice. Pba targets epigenetic function by inhibiting histone deacetylation, which silences genes that play a protective role in maintaining systemic as well as neuronal function. Downregulated histone deacetylation alters accessibility of chromatin and allows DNA-binding proteins to interact with exposed sites to activate gene transcription and downstream cellular function [28, 29].
Altered regulation of transcriptomic profiles representing multiple pathways of aging was observed in the brains of mice treated with the drug cocktail
Five pathways associated with each individual drug were altered in the brains of mice that received the drug cocktail (Fig. 3A). Brains from treated mice showed a downregulated pattern of DNA repair, suggesting a reduced tendency for DNA damage (Fig. 3B). The DNA repair pathway from the GO database includes both up- and down-stream genes involved with DNA repair that makes this an ideal illustration for addressing the level of DNA damage [30]. The innate immune sensing pathway with interferon-γ as a downstream effector was chosen to represent primary inflammatory response in the brain [31]. This pathway was downregulated in the brains of mice treated with the drug cocktail (Fig. 3C).
Normal cell division is halted when cellular senescence occurs. As senescence accumulates with increasing age, an elevated expression of both systemic and local senescence-associated secretory phenotype (SASP) is observed in neuronal cells [32]. The production of reactive oxygen species (ROS) often promotes cells into senescent phase [33]. ROS and SASP pathways are commonly designated to measure upstream and downstream transcriptional targets of senescence. Both pathways were downregulated in the brains of mice treated with the cocktail. However, only the ROS pathway was significant (Fig. 3D, E). The GSEA analysis for SASP was referenced with the exclusive Reactome gene database which led to fewer genes presented within the cluster causing fewer hits from the testing groups. Even with a nominal p-value greater than 0.05, the enrichment plot exhibited a heavily skewed downregulating trend with a distinctive normalized enrichment score of −1.76.
The GSEA data in our study indicated an upregulated trend for autophagy with data skewed upwards for mice receiving the drug cocktail (Fig. 3F). However, the nominal p-value was not significant at the 0.05 level. Genomic heat map interpretation suggested that the K-S ranking for the autophagy pathway may be affected by internal variance within the treatment cohort.
Protein expression levels of aging pathways corresponded to transcriptomic profiles in brains from mice treated with the drug cocktail
Images of IHC stains were digitally processed through Qupath for heat map demonstration and optical density quantification. The intensity results showed that brains from cocktail-treated mice had significantly less expression of γH2AX and HDAC2 while Pba only suppressed the expression of HDAC2 (Fig. 4A, B). HDAC2 is a class I histone deacetylation protein that participates in the DNA damage response as it is rapidly recruited to DNA damage sites to promote hypo-acetylation [34]. γH2AX refers to the X isoform of the histone H2A which resides closely with DNA as a part of the nucleosome. Phosphorylation of γH2AX is an early repair response to the detection of double-strand breaks or replication stress. The accumulation of HDAC2 and γH2AX in brain tissue has often been referred to as a surrogate marker of DNA damage [35].
Reduced levels of all three inflammatory molecules were observed for mice treated with the drug cocktail. Rap alone reduced the level of MCP-1 and TNF-alpha as Pba alone only reduced MCP-1 (Fig. 4C–E). General inflammation can be assessed by MCP-1, a pro-inflammatory cytokine that selectively recruits glial cells in the CNS [36]. IL-6 is secreted by parenchymal macrophages in the CNS and is critical for the progression of inflammatory disorders of neural tissue [37]. TNF-alpha is a pro-adhesive inflammatory factor that upregulates NF-κB. Increased activation of TNF-alpha induces both acute and chronic neuroinflammation [31]. Notably, treatment with Rap and Pba altered the expression of most of the tested biomarkers independently. However, neither of these two treatments affected the expression of P21, a marker associated with cellular senescence (Fig. 4G). The combination treatment uniquely downregulated P21 expression, indicating a synergistic or additive effect that is not replicated by any individual compound.
Biomarkers for senescence were decreased in the brain of cocktail-treated mice, and no effect was observed in other treatment cohorts (Fig. 4F, G). P16 and P21 are endpoints for identifying senescence phenotypes in murine models [36]. P21 is a downstream effector of P53 transcription factor and acts as a primary mediator for downstream cell cycle arrest. P16 is essential for oncogene-induced senescence and a cyclin-dependent kinase inhibitor that slows cell division by preventing the progression of the cell cycle from the G1 phase to the S phase [1]. P16 was measured through q-PCR due to the lack of validated commercially available antibody for IHC in the mouse brain. ATG5, a common biomarker for measuring autophagy, binds with beclin and promotes macroautophagy induction [38]. ATG5 levels were increased in the brain tissue of both cocktail and Rap-treated mice (Fig. 4H).
Heatmaps based on regional optical density provided additional insight on the distribution of staining within the hippocampus region. While five mouse samples were analyzed per treatment group, these IHC images presented (Fig. 5) were randomly selected from a single mouse representative of each treatment group to visually exemplify typical findings. Staining intensity was visualized by a color gradient, where red represents high levels and blue represents low levels (Fig. 5). The heatmap paralleled the quantitative data generated from positive superpixel analysis.
HDAC2 and γH2AX, protein markers associated with DNA damage and repair, observed a stark contrast in expression levels between the young untreated mice, which show minimal expression indicative of less DNA damage, and the old untreated mice, which display heightened expression levels as denoted by warmer colors, suggesting increased DNA damage or repair activity characteristic of aging. However, in the old cocktail-treated group, there is a notable shift towards the cooler spectrum for γH2AX, aligning with the expression patterns observed in the young untreated mice, hinting at the treatment’s efficacy in mitigating DNA damage. Similarly, the effect of treatment is also visible in HDAC2, affecting different regions within the hippocampus.
In terms of the inflammatory markers MCP1, IL6, and TNFα, the young untreated mice exhibit relatively low levels of these markers, whereas old untreated mice show an expected increase, consistent with an age-related pro-inflammatory state. Intriguingly, the old mice that received the cocktail treatment exhibit much lower expression of these inflammatory markers, closely resembling the young untreated profile, which suggests a substantial anti-inflammatory effect of the cocktail treatment.
When examining senescence marker P21 and autophagy-associated marker ATG5, we see a low expression of P21 in young untreated mice and a drastic increase in the old untreated mice. The old cocktail-treated mice, however, show reduced P21 expression, implying that the treatment might be influencing cellular mechanisms to retard senescence. Meanwhile, ATG5 levels, which are moderately expressed in young untreated mice and decline with age, seem to be restored in the old cocktail-treated mice, indicating a rejuvenation of autophagic processes often compromised during aging.
Discussion
Age-related cognitive decline in the brain is characterized by the progressive loss of physiological integrity. This deterioration can lead to early stages of neurodegenerative conditions such as Alzheimer’s disease and other dementias, affecting millions of older people [39]. Currently, aging is a subject of scientific scrutiny involving the aggravation of multiple different, but interconnected biological processes. Targeting multiple factors that contribute to the progression of aging will likely provide a more robust attenuation of age-related cognitive dysfunction than any single drug [7]. Significant improvement of cognitive performance was observed in middle-aged mice treated for 3 months with a drug cocktail composed of Rap, Acb, and Pba [18]. Selection of these specific drugs for a multiplex approach was based on their well-established roles in promoting health span and prolonging lifespan in mice [4, 11, 15]. Phenotypic improvement observed from this preclinical study suggested the drug cocktail may be targeting multiple pathways associated with aging.
The comparison of mechanistic pathways in the brains from mice receiving drug cocktail versus control was evaluated through GSEA on RNA-seq data. The results showed that the drug combination alleviated the aberrant progression of age-associated pathways not only directly targeted by each drug but also extensively relevant to overall cocktail effects. Molecular endpoints that manifested among tested aging pathways were further analyzed between all treatment cohorts. Quantification of IHC digital imaging provided additional evidence that the cocktail treatment showed a more comprehensive effect on ameliorating common aspects of aging compared to the administration of each individual drug in the cocktail.
A set of pathways has been considered to characterize the process of aging. Several of these pathways are involved in dysregulated nutrient sensing, enhanced insulin signaling intensity, and epigenetic alterations. Activation of mTOR1 signaling, insulin signaling, and histone deacetylase binding pathways can easily antagonize these three biological processes. Emerging studies suggest that Rap, Acb, and Pba can directly target these pathways in various mammalian models [7]. Our results indicated that all three pathways were downregulated in the brain of cocktail-treated mice at the transcriptomic level. Furthermore, cocktail treatment suppressed the aggravation of several other common aging hallmarks including DNA damage, inflammation, and senescence. DNA damage caused by changes to chromatin organization can be mediated through increasing acetylation of histones, suggesting Pba may decrease DNA double-strand breaks or replication stress [40]. mTOR implicates genome integrity maintenance, and it has been demonstrated that active mTOR1 expression interplays with DNA damage response systems and promotes growth and survival for cells undergoing constitutive DNA damage [30]. This mechanism aligned with our observation that mice with suppressed mTOR1 signaling and histone deacetylase binding also showed decreased DNA damage level.
mTOR1 is one of the key regulators for chronic inflammatory response as it controls inflammation-associated cell proliferation and migration. Rap as an anti-proliferative mTOR1 inhibitor was proven to prevent endothelial cell overgrowth and is considered a potential reagent for suppressing the primary immune response [41]. Acb was observed to lower glucose excursions and interfere with neuro-inflammatory reactions [42]. This provides the rationale for both Rap and Acb contributing to a lower level of inflammation. Rap was found to suppress the downstream complexes of mTOR1 signaling including NF-κB [43], STAT3 [44], and Akt signaling [45], hence reducing cellular senescence [1, 46]. Increasing evidence implicates cellular senescence in tissue is associated with dysregulated insulin regulation [47], which suggests that Acb may contribute to reducing the senescence-associated inflammatory response. Moreover, DNA damage is parallel to the production of senescence-associated inflammatory cytokines [15], which hints to a potential senescence-suppressing effect from the administration of Pba.
Autophagy, one of the main activities of the principal proteolytic system implicated in protein quality control, declines with aging. Rap can restore the autophagic flux and enhance autophagy by restoring mitochondrial and lysosomal functions [48]. The phenocopy of caloric restriction from Rap and antihyperglycemic effect from Acb are also known to increase autophagy activation [1]. Interestingly, a strong trend of upregulated autophagy was observed in the brains of mice that received the cocktail.
IHC assessment of age-related molecular endpoints provides insight into how drug treatment can effectively target the expression of specific biomarkers within the brain. Data from this study showed a consistently significant alleviation of expression levels in HDAC2, γH2AX, MCP-1, IL-6, TNF-alpha, and P21 from mice treated with the cocktail compared to expression levels in control mice. The results shed light on the impact of each individual drug on these molecular endpoints. Specifically, Rap was shown to significantly alter MCP-1, TNF-alpha, and ATG5 levels, whereas Pba was shown to decrease HDAC2 and MCP-1 levels. Acb alone was not associated with a reduction in any of the targeted markers, yet its inclusion in the cocktail appears to have enhanced the overall efficacy of the cocktail.
A notable observation was the unique modulation of P21 by the cocktail, absent in the monotherapies, suggesting that the combined drugs engage additional biological pathways not influenced by rapamycin or phenylbutyrate alone. This effect could result from a synergistic interaction, where the collective action of the drugs is greater than the sum of their individual effects. These findings imply that the cocktail has a synergistic advantage, offering a more comprehensive approach to modulating age-related biomarkers than any single agent.
All three drugs involved in the cocktail are Food and Drug Administration (FDA)—approved for clinical conditions in people and considered safe with little or no adverse effects. A geropathology assessment in mice from a previous preclinical study using this drug combination showed that the cocktail treatment decreased age-related lesions in all major organs without showing any histology findings related to drug toxicity or abnormal clinical pathology [18].
In conclusion, the framework demonstrated in our study of mapping the alleviating effects of a cocktail of Rap, Acb, and Pba, applied to aging-associated pathways and molecular endpoints, provided a cross-sectional perspective of associated changes in the brains of middle-aged mice (Fig. 6). The observations suggest the cocktail is an encouraging blueprint for designing future drug combinations for preventing, reversing, or delaying age-related cognitive impairment and decreasing the risk for the development of more severe degenerative conditions such as Alzheimer’s disease.
Data availability
All RNA-sequencing data has been uploaded to the SRA database. It will be released upon the publication of the manuscript. The reference number is PRJNA1012002.
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This work was supported by National Institutes of Health grants R01 AG057381 (Ladiges and Darvas, coPI’s), R56 AG058543 (Ladiges PI), and R01 AG057381 (Ladiges PI).
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Jiang, Z., He, Q., Wezeman, J. et al. A cocktail of rapamycin, acarbose, and phenylbutyrate prevents age-related cognitive decline in mice by targeting multiple aging pathways. GeroScience 46, 4855–4868 (2024). https://doi.org/10.1007/s11357-024-01198-w
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DOI: https://doi.org/10.1007/s11357-024-01198-w