Molecular Mechanisms of Inflammation in Sarcopenia: Diagnosis and Therapeutic Update

Sarcopenia is generally an age-related condition that directly impacts the quality of life. It is also related to chronic diseases such as metabolic dysfunction associated with diabetes and obesity. This means that everyone will be vulnerable to sarcopenia at some point in their life. Research to find the precise molecular mechanisms implicated in this condition can increase knowledge for the better prevention, diagnosis, and treatment of sarcopenia. Our work gathered the most recent research regarding inflammation in sarcopenia and new therapeutic agents proposed to target its consequences in pyroptosis and cellular senescence. Finally, we compared dual X-ray absorptiometry (DXA), magnetic resonance imaging (MRI), and ultrasound (US) as imaging techniques to diagnose and follow up on sarcopenia, indicating their respective advantages and disadvantages. Our goal is for the scientific evidence presented here to help guide future research to understand the molecular mechanisms involved in sarcopenia, new treatment strategies, and their translation into clinical practice.


Introduction
Population aging and obesity have become enormous problems for public health, challenging healthcare systems. In 2019, the United Nations Population Prospects and the World Population Ageing indicated that, by the year 2050, the number of people over 60 years will have increased from 1 in 11 individuals to 1 in 6 individuals [1,2]. This situation forces us to have a new social, health, and economic perspective on the elderly [3,4]. One of the many conditions related to aging is sarcopenia, defined by the World European Working Group in Older People 2 (EWGSOP2) as a progressive skeletal muscle disease prone to dramatic outcomes such as falls, fractures, physical disability, and mortality [4,5]. Sarcopenia is characterized by a massive decline in muscle mass and function [6,7] that begins between 30 and 40 years of age, with a 3-8% gradual muscle fiber decline every decade until the 60's, when the loss compromises the individual's life [8]. Although sarcopenia is usually related to aging, in primary sarcopenia, there are other risk factors, such as cancer, obesity (sarcopenic obesity), rheumatic diseases, and malnutrition, that lead to secondary sarcopenia [9]. A lack of physical activity or a sedentary lifestyle leads to secondary sarcopenia in earlier life stages [10,11].
The characterization of sarcopenia is essential for clinical care practice. According to the EWGSOP2, not only low muscle mass but also low muscle quality, strength, and physical performance are now accepted as new criteria in the disease diagnosis [5]. Sarcopenia is a multifactorial disease with a wide variety of factors that contribute to its onset, such as lifestyle, physical activity, nutritional habits, reduced satellite cells (myogenic stem cell), changes in muscle protein homeostasis, anabolic resistance, neuromuscular dysfunction, among others.
The EWGSOP2, Asian Working Group for Sarcopenia (AWGS), and other worldwide organizations have established the clinical and research guidelines that help to understand, prevent, detect early, and treat sarcopenia and its dramatic consequences [5,12]. To date there have been no US Food and Drug Administration (FDA)-approved medications for sarcopenia, so therapeutical approaches to overcome sarcopenia could lead to better intervention in healthy aging [13]. Our objective is to provide a molecular perspective on the inflammatory and energetic processes that underlie sarcopenia, analyze non-invasive and low-cost diagnostic tools for early diagnosis, and increase the understanding of treatment.

Inflammation in Sarcopenia 2.1. Inflammaging in Sarcopenia
Aging and lipid metabolism are correlated with the increase in dysfunctional systemic levels of inflammatory molecules (chronic low-grade inflammation) known as "inflammaging" [14,15], which leads to tissue degeneration and pathogenesis in age-related diseases (type 2 diabetes, osteoarthritis, and sarcopenia) [14,16,17]. Inflammaging is especially connected to sarcopenic obesity, supported by alterations in glucose metabolism, insulin resistance, and oxidative stress, along with exacerbating the production of inflammatory cytokines [18][19][20]. In addition to inflammaging, primary and secondary sarcopenia are also correlated with alterations in lipid metabolism [21]; replacing type II muscle fibers with fat is one of the most prominent characteristics of the disease, contributing to muscle contraction atrophy [22]. The principal inflammatory molecules involved in inflammaging are TNF-α, IL-6, IL-1, and chemokines, which promote the infiltration of inflammatory cells to deteriorate muscle via NF-κB [23]. Lifestyle habits such as physical activity and diet profoundly impact primary and secondary sarcopenia [24,25]; for example, it is well known that a sedentary lifestyle increases the risk of many chronic diseases, including sarcopenia [26]. Moreover, exercise attenuates muscle loss by decreasing the activation of NF-κB [27,28]. Furthermore, diet and nutrition play an important role in the onset of sarcopenia; for example, saturated fat can activate the innate immune system, leading to pro-inflammatory molecule production (IL6 and TNF-α), which, over time, causes insulin resistance [29]. Inflammation triggered by certain foods can be measured by the Dietary Inflammation Index (DII), where higher values of DII represent a greater probability of inflammation. This DII score has been used to establish the inflammatory potential of food; a high DII has been associated with the development of musculoskeletal diseases, including sarcopenia [30]. Therefore, a diet rich in vegetables and fruits is recommended to reduce the risk [31]. In a rat model, a high-fat diet (HFD) caused the accumulation of long-chain fatty acids such as linoleic acid, stearic acid, and vaccenic acid, as well as an increase in the chemokines RANTES, MCP-1, and MIP-2, causing low-grade inflammation and decreased muscle quantity and quality-distinct attributes of sarcopenia [32,33]. The accumulation of palmitic acid derived from a lifestyle with dietary imbalance reduces Akt phosphorylation causing insulin resistance and impairs muscle regeneration [34][35][36]. Moreover, palmitic acid leads to inflammation and cell death by increasing the inflammatory cytokine TNF-α [37], which reveals the lipotoxic effect of high levels of this saturated fatty acid.
In contrast, omega-3 polyunsaturated fatty acids (such as alpha-linolenic acid (ALA), eicosapentaenoic acid (EPA), and docosahexaenoic acid (DHA)) decrease the adverse effects of sarcopenia by reducing inflammation [38] and improving muscle strength and function in older adults with little effect on muscle mass [39]. In fact, eicosapentaenoic has been shown to have benefits against muscular atrophy caused by palmitic acid accumulation. EPA treatment under lipotoxic stress caused by palmitic acid reduced the rate of muscle protein loss related to the expression of MyoD, myogenin, IGF-II, and IGFBP-5 [37]. These findings support omega-3 polyunsaturated fatty acid administration as a potential therapeutic tool to reduce muscle loss and inflammation linked to accumulated fatty acids in secondary sarcopenia. Likewise, DHA has also recently been found to modulate the ubiquitin-proteasome and the autophagy-lysosome systems, potentially improving muscle integrity and function by decreasing proteolysis and inflammation for sarcopenia [40].
Some saturated fatty acids can enhance the signaling pathways involved in the inflammation of macrophages [41]. NF-κB expression, linked to the deregulation of lipid metabolism, is relevant because it activates the NLRP3 inflammasome multiprotein complex that generates a network of immune responses related to local and systemic inflammation [42]. Different signals can lead to the activation of the NLRP3 inflammasome and cause sarcopenia; for example, metabolic dysregulation due not only to obesity but also to insulin resistance [43] leads to hyperglycemia and muscle atrophy via the WWP1/KLF15 pathway [44]. This pathway could be used as a therapeutic target for muscle atrophy and sarcopenia developed by obesity and insulin resistance [45].

Pyroptosis Contributes to Sarcopenia Development
The inflammation-induced activation of the NLRP3 inflammasome can trigger cell death, a process known as pyroptosis [46]. NLRP3 activates the axis caspase-1, which acts upon its substrate gasdermin D (GSDMD), cleaving it [47] and causing multiple membrane pores. These pores allow ion flux and the release of ATP, HMGB1 (high-mobility group box-1), and interleukin (IL)-1β into the cell, provoking membrane rupture and, ultimately, cell death/pyroptosis [48][49][50]. The NLRP3 inflammasome and pyroptosis contribute to muscle dysfunction through a decline in the glycolytic potential and myofiber size [44]. The perspective of the NLRP3 inflammasome reveals the necessity of finding new therapeutical approaches to attenuate inflammation and pyroptosis in sarcopenia.
A recent approach is the administration of BMP-7 (bone morphogenetic protein 7), which, in mice, showed the potential to attenuate pyroptosis, inflammation, and muscle atrophy in diabetic muscle myopathy via the inhibition of the HMGB-1 protein. HMGB-1 protein is a potent signaling molecule for inflammation and a key initiator in pyroptosis that binds RAGE or TLR4 and activates other pro-inflammatory factors [51]. Mice with muscle atrophy triggered by the administration of dexamethasone (Dexa) were treated with phlorotannin dieckol (DK) from the brown algae Ecklonia cava (ECE) extract. They showed a reduction in protein levels in HMGB-1, NF-κB, and TLR4, key molecules in NLRP3 inflammasome formation (Figure 1) [52]. These therapeutic alternatives offer an alternative to attenuate the effects of inflammation and pyroptosis in sarcopenia.

Inflammaging and Mitochondria
Mitochondrial dysfunction is a common state in sarcopenia related to inflammation [53]. Therefore, mitochondrial quality and homeostasis control are essential to prevent muscle damage. To maintain mitochondrial quality and homeostasis, damaged mitochondria must be removed via mitophagy (organelle-specific autophagy). Conversely, the accumulation of damaged mitochondria and decreased mitophagy are related to sarcopenia [54,55] and are a source of mitochondrial damage-associated molecular patterns mDAMPs (such as mitochondrial DNA (mtDNA), N-formyl peptides, and some lipid spe-

Inflammaging and Mitochondria
Mitochondrial dysfunction is a common state in sarcopenia related to inflammation [53]. Therefore, mitochondrial quality and homeostasis control are essential to prevent muscle damage. To maintain mitochondrial quality and homeostasis, damaged mitochondria must be removed via mitophagy (organelle-specific autophagy). Conversely, the accumulation of damaged mitochondria and decreased mitophagy are related to sarcopenia [54,55] and are a source of mitochondrial damage-associated molecular patterns mDAMPs (such as mitochondrial DNA (mtDNA), N-formyl peptides, and some lipid species such as cardiolipin).
Interestingly, inflammation and mDAMPs synergistically contribute to sarcopenia [56]; for example, mDAMPs can activate the Toll-like receptor (TLR) pathway and trigger NF-κB signaling, thus increasing the expression of IL-6 and TNF-α [57]. Damaged mitochondria can activate the NLRP3 inflammasome, triggering the expression of the proteolytic cytokines IL-18 and IL-1β and enhancing inflammation, likely causing pyroptosis ( Figure 1) [58]. These reports highlight the importance of the interconnection between mitochondrial dysfunction, triggering potent inflammatory responses that contribute to sarcopenia. In the next section, we analyze mitochondrial morphology and lipid alterations related to sarcopenia development.

Senescence and Its Role in Sarcopenia
Recently, the relevance of cellular senescence in sarcopenia has gained attention due to its relation with inflammaging. Cellular senescence is the permanent cell cycle arrest in response to various stress stimuli or signals that compromise genomic integrity, preventing the proliferation of damaged cells [59]. In addition to cell cycle arrest, cellular senescence is characterized by a highly active metabolic state, telomere shortening, increased ROS, persistent DNA damage, the expression of diverse genes, and the secretion of inflammatory molecules partially regulated by NF-κB, such as IL-1α, IL-6, and IL-8, causing the senescence-associated secretory phenotype (SASP). Over time, this phenotype contributes to the clearance of the same senescent cells by the immune system since accumulation could result in chronic inflammation and changes in the cell microenvironment [59][60][61].
The accumulation of senescent cells in muscle correlates with sarcopenia pathophysiology because of the secretion of inflammatory molecules, and the increase in protein degradation results in muscle fiber thinning [62][63][64]. On the one hand, cellular senescence affects the functionality and number of satellite cells (SCs, specific muscle stem cells), which play a fundamental role by switching from their normal quiescent state with a low metabolic rate to an active state to proliferate, differentiate, and form new muscle fibers [65,66]. Subsequent cellular senescence could limit the ability of SC to regenerate and maintain itself by the overexpression of p16 (INK4a), which is the primary inducer of cell cycle arrest in cellular senescence [65]. On the other hand, the SASP significantly contributes to sarcopenia via inflammaging, where the persistent levels of IL-6 harm muscle integrity and function, causing muscle degradation and atrophy [67]. Given the consequences of cellular senescence in muscle degeneration, it is necessary to find new therapeutical strategies to attenuate cellular senescence and its SASP. New approaches have emerged since 2015, when Kirkland's work group demonstrated the selective depletion of senescent cells in adipose tissue accompanied by decreasing levels of IL-6, IL-8, and CCL2. The precise depletion was achieved by a new type of drugs named senolytics, which include dasatinib and quercetin; the combined treatment can extend the lifespan of aging mice and improve their muscular strength and exercise capacity (Table 1) [68,69]. Preliminary reports suggested that new drugs such as senolytics recover muscular function. In this context, the compound 25HC-an oxygenated derivate of cholesterol that inhibits the CRYAB (Alpha beta-crystallin) protein, which is upregulated in senescent cells-showed significant effects in skeletal muscle. 25HC inhibits the expression of IL-6, a known contributor to muscle atrophy in sarcopenia, attenuating the loss of muscle mass associated with aging in mice and human cultures (Table 1) [70]. Another preliminary report suggested the use of a 5-fluorouridine (5FUR) derivate; 5FURGal kills human senescent cells with multiple benefits such as enhancing cognitive function, lifespan extension, and improvement of muscle tissue and satellite cells (Table 1) [71]. Overall, the connection between SASP and NLRP3 provides a scenario where therapeutic targets against senescent cells (senolytics) and/or the NLRP3 inflammasome could prevent muscle degeneration and sarcopenia, killing two birds with one stone. and MuRF1 Higher intake of Vitamin C has a positive correlation with higher muscle mass

Mitochondrial Homeostasis in Sarcopenia
Mitochondria play a crucial role in muscle health, function, and homeostasis by acting as cellular energy communicators, regulating intracellular calcium concentrations, and modulating cell proliferation [53]. Therefore, mitochondrial quality and homeostasis control are essential to prevent muscle damage.

Mitochondrial Plasticity and Lipotoxicity in Sarcopenia
Mitochondrial functionality depends on the morphological plasticity regulation between the coordination of two events: (1) Mitochondrial fusion, which allows mitochondrial interconnection, signal transmission, and metabolite exchange, is associated with the high utilization of muscle capacity and the regulation of oxidative metabolism and is accompanied by the simultaneous expression of Mfn2 and Opa1 proteins [88].
(2) The opposite event is mitochondrial fission, wherein mitochondrial fragmentation is evident, controlling the correct segregation of daughter cells, targeting defective mitochondria for mitophagy elimination and the protein expression of Drp1 and Fis1 [88,89]. Diverse authors have shown a mitochondrial fusion/fission imbalance phenotype in aged mice [55,90]. According to Del Campo, this imbalanced state is observed before sarcopenia is completely developed, contributing to the notion that this preserved phenotype in mitochondrial functionality plays a pivotal role in the pathophysiology of sarcopenia [90]. Earlier this year, the mitochondrial uncoupling agent BAM15 (a protonophore of the respiratory chain) was demonstrated to decrease mitochondrial fission by lowering the expression of Fis1; as a result, increased muscle mass and function, mitochondrial biogenesis quality control, and OXPHOS activity were observed, accompanied by the attenuation of inflammation in sarcopenic mice. These findings provide a new perspective on mitochondrial dynamics in sarcopenia and possible new therapeutical targets [73].
Other mitochondrial disturbances associated with sarcopenia include high sustained levels of triglycerides due to disproportionate diacylglycerol, resulting in a metabolic shift and causing low levels of phosphatidylethanolamine [91,92]. Phosphatidylethanolamine is a key phospholipid for membrane fluidity, inducing a persistent fusion-like phenotype in mitochondrial morphology-this persistent morphological state is a known contributor to sarcopenia development (Figure 1) [91,93]. In sarcopenia, lipid metabolism dysregulation is widespread. Excess triglyceride and HDL are strongly correlated with sarcopenia [94,95]. Furthermore, unbalanced lipid components directly impact mitochondrial morphology and functionality [91]. These mitochondrial changes are major factors that contribute to the age-dependent muscle degeneration observed in sarcopenia [96].

Alterations in Energy Metabolism Implicated in Sarcopenia
Understanding the metabolome in sarcopenia could significantly contribute to determining its pathophysiology and treatment. In recent years, diverse metabolomic profiles have been performed, mainly in the skeletal muscle of mice, showing a general perspective on metabolites that could serve as novel targets to diagnose and treat sarcopenia.
Regarding age-related energy dysfunction, a genome-wide transcriptional analysis in individuals of diverse ethnicities with sarcopenia showed mitochondrial energy dysfunction as a major disruption accompanied by an impaired OXPHOS system. As a result, NAD + levels, the principal regulator of REDOX balance, were reduced significantly; likewise, its activity was notably decreased, revealing the essential role of mitochondria in appropriate muscle function independently of ethnicity [97].
On the subject of glycerophospholipids (GPLs) in the gastrocnemius and soleus of FBN-aged rats (Fischer/brown Norway rat model of aging), the metabolic analysis showed a reduction in carnitine [98]. Low levels of carnitine were associated with cardiomyopathy, muscle weakness [99], and mitochondrial dysfunction [100]. Carnitine is an important amino acid essential for energy metabolism due to its role in the mitochondrial β-oxidation of fatty acids. In recent years, low carnitine levels have been associated with secondary sarcopenia triggered by conditions such as chronic liver disease, liver cirrhosis, and gastrointestinal cancer [101][102][103]. Recently, carnitine levels have been used as a sarcopenic biomarker [103] and a potential candidate to delay muscle deterioration [102,104]; therefore, these metabolomic alterations in FBN-aged rats could be extrapolated to humans with sarcopenia.
Polyamines are biomolecules composed of multiple amino groups interacting with diverse molecules such as DNA, RNA, and ATP at physiological conditions [105], par-ticipating in cell growth and protein synthesis [106]. In early 2006, a reduction in total polyamine levels in the muscle of aged mice was described [107]. Recently, metabolomic analyses in aged mice have shown both a notorious reduction in spermidine and spermine and a lower expression of S-adenosylmethionine decarboxylase [108]. In mice, spermidine, in combination with exercise, reduced the muscular atrophy and sarcopenia via the AMPK-FOXO3a pathway, which resulted in autophagy activation, promoted myogenesis, and reduced D-gal apoptosis [109].
Thus, energy metabolism dysfunction is essential in the pathogenesis of sarcopenia. Knowing the molecular targets participating in the disruption could lead to new therapeutic strategies for sarcopenia.

Biological Therapy Interventions
Biotherapeutic approaches for sarcopenia could provide a reliable perspective for therapeutic intervention for sarcopenia. One attractive candidate to target sarcopenia is Myostatin (MSTN), a member of the transforming growth factor-beta (TGF-β) superfamily and a potent negative regulator of muscle growth and differentiation [110]. In recent years, diverse strategies in designing monoclonal antibodies against MSTN have shown a significant increase in muscle mass and moderate improvement in muscle function in clinical trials-such as the case of landogrozumab. Other evaluations in individuals with sarcopenia are currently underway [74,75]. For example, another MSTN inhibitor, trevogrumab, enhances muscle mass and function in young and old mice. Meanwhile, others (Stamulumab, Domagrozumab, a novel anti-myostatin peptide PINTA-745, and an anti-myostatin adnectin RG6206) increase muscle mass but fail to improve physical strength in clinical trials [75].
Other interesting therapeutical approaches for sarcopenia treatment are testosterone and androgen modulators. Testosterone deficiency is clinically associated with sarcopenia and obesity [76]. Testosterone interacts with the androgen receptor (AR), leading to its nuclear translocation to regulate myogenic expression [77]. In clinical trials, testosterone supplementation showed increased muscle mass and strength in older men. However, studies were terminated due to secondary cardiovascular effects, prostatic hyperplasia, and urinary symptoms [111,112]. Therefore, combined strategies to reduce secondary effects have been proposed as a solution, such as exercise or the combination with finasteride that impedes prostatic hyperplasia [113].
As many therapeutical approaches fail to improve muscular strength and function (e.g., some MSTN inhibitors), researchers have seriously considered other drugs that simulate the effects of physical activity on activated protein kinase (AMPK) signaling as attractive targets for sarcopenia, for example, metformin, a common type II diabetes treatment. Metformin activates AMPK [114] and modulates diverse biological processes for muscle, such as glucose uptake, fatty acid oxidation, protein metabolism, autophagy, and mitochondrial function [115]; it also decreases the development of sarcopenia by reducing the inflammatory response by NF-κB [116]. Preliminary trials with metformin combined with exercise have improved resistance training in healthy older adults [78,79].

Natural Compounds
Natural compounds with anti-aging effects have been tested for sarcopenia treatment, such as ursolic acid and pentacyclic triterpene acid fruits, including apple peels and tomatidine (a steroidal alkaloid derived from green tomatoes), which increase the quality of muscle mass and grip strength of mice by reducing the activity of ATF4, a mediator of age-related muscle atrophy [80].
Plant flavonoids are important as dietary compounds because of their activities in maintaining good health; in this regard, we want to reference flavanols, the main constituents of cocoa beans. Flavanols such as epicatechin have delayed skeletal muscle degeneration in aged mice by reversing the age-altered expression of extracellular matrix peroxisome proliferator-activated receptors (PPARs), which are master regulators for lipid and glucose homeostasis in muscle [81,82]. Furthermore, epicatechin from cocoa beans improves physical performance consistently with the modulation of biomarkers of sarcopenia by decreasing FoxO1A and MuRF1, regulators of muscle degradation [83]. Epicatechin has also been shown to have anti-inflammatory effects in diverse cell types, such as hepatic and glial cells, but this effect remains to be proved in sarcopenia [117,118].

Vitamins
Vitamin D deficiency and low physical activity strongly correlate with muscle mass, strength, physical performance, and sarcopenia [119]. Some authors have suggested vitamin D as a regulator of mitochondrial health and possible implications in satellite cells activity for muscle regeneration [84]. However, the effects of vitamin D can be indirect in muscle function via its relationship with serum calcium and phosphorus [120,121]. Recent studies have demonstrated that the depletion of vitamin D receptors in mice myocytes directly impacts muscle size and strength, demonstrating the participation of signaling vitamin D in muscle function and size [85]. Another work group showed the increased expression of MuRF1 (Muscle RING-finger protein-1) and FOXO3a in mice with limited physical activity and vitamin D deficiency, implying a synergistic effect of vitamin D, physical activity, and muscle protein degradation in sarcopenia [122]. These studies recommend vitamin D supplementation and physical activity to fight against sarcopenia.
Vitamin C aids carnitine and collagen biosynthesis [123,124] and has a significant and positive association with muscle. Vitamin C deficiency in mice stimulates the upregulation of ubiquitin ligases, such as atrogin1/muscle atrophy F-box (MAFbx) and MuRF1 [125]. Other recent studies have demonstrated that a higher vitamin C intake is positively correlated with a higher muscle mass in men and women [86,87]. These findings are relevant to future treatments and the prevention of sarcopenia.

Imaging Based on Inflammation as an Approach for Detection and Follow-Up of Sarcopenia
As mentioned above, diverse factors lead to muscle degeneration manifested as a loss of muscle fibers and mass. The sooner sarcopenia diagnosis is established, the easier it is to prevent more health impairments; that is why diagnosis needs reliable and combinable methods for clinical practice. According to EWGSOP2, diagnosis for sarcopenia should follow a step-by-step procedure starting with a validated measure of muscle strength, commonly by grip strength. If grip strength is lower than the reference, sarcopenia should be considered a probability [126]. The next step in diagnosing sarcopenia is measuring muscle mass and quality [5]. For this approach, there are many tools and techniques, each with its respective flaws or limitations. Currently, there is no single reliable universal tool for clinical practice. In this section, we compare the different tools to diagnose sarcopenia.
Clinical visualization methods represent excellent tools to support the diagnosis and monitoring of various pathological conditions, including sarcopenia [127][128][129]. Biopsy has long offered the visualization of the morphological changes in muscle, the infiltration of adipose cells, and fibrous tissue, among other aspects related to muscle quality; therefore, muscle biopsies have been commonly used to diagnose sarcopenia [130]. However, biopsy is an invasive procedure that can cause discomfort and requires posterior wound care; additionally, a relatively larger sample may be required, and the method is unsuitable for people on anticoagulant treatments (Table 1) [131]. In this regard, imaging tools offer a non-invasive option to evaluate muscle integrity and real-time visualization, which provide the personalized and precise determination of muscle quality.
The various imaging tools can precisely identify vulnerable people before the development of sarcopenia or the early stages of the condition, thus allowing early treatment.
Dual X-ray absorptiometry (DXA) has become one of the most common tools to quantify body composition (BC). For sarcopenia diagnosis, this method is based on X-ray transmission across the body at two different spectra, visualizing either bone or soft tissue (e.g., fat mass and lean mass) [132]. This tool estimates muscle mass by linking the appendicular lean soft tissue (ALST) and total-body SM mass in an equation [133]. The use of DXA to measure muscle mass is controversial, while some authors use DXA as a reference tool to diagnose sarcopenia because of its validation versus other more expensive imaging methods such as computer tomography (CT) or magnetic resonance imaging (MRI). Furthermore, the radiation exposure is much lower than in CT [134]. Others point out that using DXA as a reference/gold standard is still premature because of discrepancies related to hydration, thickness of soft tissues, and unclear mathematical equations and algorithms used for the estimation of muscle mass leading to cumulative variations and dangerous expectations in sarcopenia diagnosis [135].
Another imaging tool that can help analyze muscle integrity and sarcopenia is magnetic resonance imaging (MRI), which is based on the atomic distribution of the body because of a strong magnetic field [136,137]. The organization of the atoms can vary according to the nature of the molecules; this allows the recognition of diverse tissues based on their magnetic attributes [138]. The MRI is the most advanced tool for identifying sarcopenia and is considered the gold standard for muscle mass quantification, showing muscular quality and fat [5,139]. The MRI variation methods accompanied by nuclear polarization have shown a significant intensification of the MRI signal, allowing the visualization of free radical species in tissues [140]. Dynamic nuclear polarization-magnetic resonance imaging (DNP-MRI) is a variation of the above-described technique used to explore real-time REDOX fluctuation states under local muscle inflammation; this is a magnificent MRI approach to follow up pathologies in real time where inflammation plays a fundamental role (Table 2). However, some disadvantages of MRI and its variations are the high costs and restricted accessibility [141], which is why it is not yet a daily technique used worldwide.
Since MRI is not always an option in the identification and follow-up of sarcopenia, ultrasound (US) can be used since it provides some advantages. First, US is a much more acceptable tool in terms of costs, accessibility, portability, and patient/analyst ease; second, this imaging tool offers a significant degree of image resolution, allowing a good evaluation of muscular integrity quantification and inflammation [142]. US is based on sound waves that the human ear cannot detect (a frequency between 200 kHz and 1.5 MHz) and provides a signal to visualize the size structure of diverse organs and tissues [143]. The use of US has increased exponentially in recent years to diagnose and follow up on various musculoskeletal conditions, including those related to muscle degeneration associated with inflammation and/or restricted mobility [144]. Recent reports have provided standardization and recommendation for the better operation of US to evaluate diverse muscle mass parameters in more than 30 different muscles, taking advantage of the vast presence of US in clinical practice [145][146][147]. These US muscular parameters are considered "ultrasound biomarkers for sarcopenia" and include muscle thickness, echo intensity, pennation angle, fascicle length, contrast-enhanced assessment of vascularization, and the cross-sectional area, among others. One of the most used parameters is the echo intensity, which expresses the muscle quality in terms of structural changes caused by an increase in intramuscular fat infiltration and connective tissue, which results in a higher echo intensity of the muscle in question; it has also been noted that echo intensity is higher in muscle from older than younger people [148,149]. Likewise, US helps to determine the microstructural characteristics of muscle by measuring the pennation angle and fascicle length, as decreased values of these parameters are observed in sarcopenia [150].
One of the main challenges for US to be at the same level as MRI (the gold standard imaging tool) in sarcopenia is the universal standardization of the quantitative and ensembled (and not alone) parameters of muscular changes among diverse muscles to evaluate individuals with sarcopenia. Nonetheless, US might positively impact the daily clinical practice for the early identification and follow-up of this disease (Table 2).
Other non-imaging tools are used to measure the muscle mass in sarcopenia diagnosis, such as bioimpedance analysis (BIA) [151]. This technique is based on an electric current through the body, where the tissues rich in water and electrolytes let electric currents pass more easily than adipose tissue. BIA flaws are influenced by many factors, such as age, hydration, and different devices [152,153]. Thus, this tool should only be used when there is limited access to better options [154].

Conclusions
From a public health point of view, sarcopenia is a dangerous condition that compromises muscle integrity and directly impacts the quality of life of several groups of individuals, mainly elderly people or those with risky lifestyle behaviors [5,161]. Categorizing sarcopenia into primary or secondary is important to prevent, diagnose, and treat this condition [162]. However, it is not an easy task because the dynamics of sarcopenia depend on many factors that can be intrinsic or extrinsic, such as age, sex, physical activity, dietary intake, comorbidities, etc. [5]. The complex dynamics make it difficult to determine between primary and secondary sarcopenia. Primary sarcopenia is always associated with chronological aging and is exacerbated by diseases or other lifestyle factors and leads to secondary sarcopenia, which is the muscle loss for other causes involved in addition to aging [162].
More information about the molecular basis, onset, and diagnosis of sarcopenia can be used for the better prevention and treatment of the disease. Our work comprises some of the most recent information regarding inflammatory molecular mechanisms underlying sarcopenia; additionally, we reviewed different imaging tools to help diagnose and follow up on the disease.
Aging and metabolic diseases, such as obesity and type II diabetes, are accompanied by a state of chronic inflammation. One of the diverse mechanisms known to contribute to the onset of sarcopenia is the slight but persistent increase in inflammatory mediators such as IL-1β, IL-6, and TNF-α that simultaneously impact muscle metabolism, causing wasting and loss via the mTOR pathway [163][164][165]. One event that exacerbates the inflammatory state in sarcopenia is senescence via its associated secretory phenotype (SASP). The release of soluble factors such as pro-inflammatory cytokines and chemokines has a paracrine effect on neighbor cells, reinforcing the microenvironment of chronic inflammation and cellular senescence. Another factor involved in the onset of sarcopenia is mitochondrial dysfunction, which brings a series of alterations at different levels; for example, the abnormal mitochondrial morphology caused by an impaired lipid metabolism entails the stiffness of membranes and increases reactive oxygen species in muscle degeneration. Additionally, mitochondria have a close relationship with inflammatory processes that could be exacerbated to cause pyroptosis. Mitochondrial dysfunction in sarcopenia can be expressed as differential patterns depending on the class of muscle with altered levels of intermediates that participate in energetic metabolism, i.e. the significant decrease in REDOX regulators and some cofactors essential for the complete glucose oxidation that enhances muscle deterioration. Therefore, strategies directed to decrease the inflammatory state, the clearance of senescent cells in sarcopenia, or the attenuation of mitochondrial dysfunction (Table 1)

Conflicts of Interest:
The authors declare no conflict of interest.