Lipid Metabolic Alterations in KRAS Mutant Tumors: Unmasking New Vulnerabilities for Cancer Therapy

KRAS is one of the most commonly mutated genes, an event that leads to development of highly aggressive and resistant to any type of available therapy tumors. Mutated KRAS drives a complex network of lipid metabolic rearrangements to support the adaptation of cancer cells to harsh environmental conditions and ensure their survival. Because there has been only a little success in the continuous efforts of effectively targeting KRAS-driven tumors, it is of outmost importance to delineate the exact mechanisms of how they get rewired, leading to this distinctive phenotype. Therefore, the aim of this review is to summarize the available data acquired over the last years with regard to the lipid metabolic regulation of KRAS-driven tumors and elucidate their specific characteristics in an attempt to unravel novel therapeutic targets.


Introduction
Altered metabolism is a well-established hallmark of cancer as a response of tumor cells to the continuously changing environmental conditions such as reduced oxygen availability (hypoxia) and nutrient deprivation. Lipid metabolism is a field of study that has recently been in the limelight, as its dysregulation allows cancer cells to meet their high energy and growth demands. One of the most commonly mutated gene in human cancer is the small GTPase RAS. KRAS-driven tumors, shift their metabolism towards a more anabolic profile by upregulating the expression of multiple rate-limiting enzymes involved in key metabolic processes essential for survival. With this metabolic shift, KRAS-driven tumors not only are able to produce key lipid mediators establishing an immunosuppressive tumor microenvironment (TME), but are also able to take full advantage of exogenous lipids produced by the TME such as fatty acids (FAs) prostaglandins and other lipid mediators, thus maintaining a vicious cycle that allows tumor growth and metastasis. Therefore, mutated KRAS, which is mostly encountered in pancreatic, lung and colorectal cancers, is considered a synonym for highly aggressive, resistant to conventional therapies tumors, thus leading to a devastatingly poor patient survival. Despite continuous effort, the GTPase has not been successfully targeted yet, with the only bright exception being the recent FDA approval of sotorasib (AMG 510), a small molecule targeting directly KRAS G12C . Thus, it is of outmost importance that we unravel unique characteristics of these tumors that could potentially be used as therapeutic vulnerabilities. To this end, in this review, we summarize and discuss the recent insights in the deregulation of lipid metabolism of KRAS-driven tumors, as well as the interplay between specific lipids and key cancer machineries.

Fatty Acid Uptake, Biosynthesis, and Degradation
The highly conserved process of FA synthesis incorporates carbons from acetyl-CoA into growing FAs, thus providing the cell with the required substrate for cell growth signaling, membrane building, and energy storage. In the 50 s, a seminal observation was made directly linking lipid biogenesis and cancer. Medes et al. described that tumor cells For FA synthesis to take place unobstructed, vital secondary metabolites are required, which become available through glycolysis. Therefore, attenuating the glycolytic machinery could prove to be beneficial by restricting not only the energy supply, but also the availability of indispensable, for lipid generation, metabolites. In this direction, the importance of glucose transporters in Kras-driven lung adenocarcinomas has been investigated, revealing that in a Kras LSL-G12D/WT ;Trp53 flox/flox lung adenocarcinoma mouse model concomitant deletion of the glucose transporters Glut1 and Glut3, significantly decreases tumor progression [18]. On a similar note, pharmacologic inhibition of an alternative glucose transport system, the sodium-dependent glucose transporter Sglt2, delayed the development of lung adenocarcinomas [19]. Taking into account the fact that compounds for Sglt2 inhibition are already being used in the clinic to treat diabetes, it is realistic to say that targeting the lipid metabolism of cancer cells through the glycolytic pathway may become possible in the near future for the subset of patients with tumors that are heavily dependent on glycolysis.
Several key enzymes of the FA synthesis process undergo transcriptional regulation by sterol regulatory element-binding protein 1 (SREBP1), including FASN [20,21]. Mutant KRAS regulates SREBP1 mainly by upregulating the PI3K/Akt/mTOR signaling pathway [22] As expected, SREBP1 has been found upregulated in KRAS mutant PDAC patients and its expression correlates with poorer prognosis [23]. NSCLC cells also exhibit increased SREBP1 levels; however, a novel, non-canonical role has recently been attributed to the gene, as it was shown that its ablation inhibits tumor growth, not by affecting lipogenesis, but by altering mitochondrial function and impairing oxidative phosphorylation [24]. Similarly, in CRC cells, genetic inhibition of either SREBP1 or SREBP2 leads to reduced tumor initiation and growth in vitro and in vivo, accompanied by decreased oxidative phosphorylation and glycolysis levels [25]. Hence, it would undoubtedly be of interest to investigate whether SREBP, apart from its well-established role in FA and cholesterol synthesis, is also directly regulating genes involved in mitochondrial function in a setting of KRAS-driven tumorigenesis.
On the other side of the spectrum, FA degradation by β-oxidation (FAO) is responsible for energy supply and NADPH production. For years, the synthesis and degradation of FAs were considered as two mutually exclusive cellular processes. The tide has turned over the last decade, and we are now at a point where it is accepted that both pathways can, in fact, be active concomitantly and independently [26,27]. FAO is tightly regulated by carnitine palmitoyltransferase 1 (CPT1), an enzyme that couples FAs with carnitine to enable their translocation to the mitochondria. Increased FAO levels directly correlate with accelerated progression and therapy resistance in KRAS-driven tumors. This phenotype can be established via multiple mechanisms. In KRAS mutant NSCLC, FAO is facilitated by the upregulation of long-chain acyl-CoA synthetase 3 (ACSL3), the enzyme responsible for activating free FAs, allowing tumor cells to meet the increased ATP demand [2]. Moreover, loss of REDD1 in KRAS mutant NSCLC not only increases FAO, but also allows cancer cells to cope with increased reactive oxygen species (ROS) by boosting ROS detoxifying systems [7]. Interestingly, both ACSL3 upregulation and REDD1 loss exhibit enhanced uptake of lysophospholipids and lipid storage. Notably, in a Kras G12D -driven PDAC mouse model, inhibition of FAO reduces the tumor-initiating potential of a dormant, oncogene ablation-resistant, population of tumor cells that is often linked to relapse [28]. In colorectal cancer, elevated FAO is associated with extracellular FA-mediated AMPK activation, an event that strongly favors FAs as the main mitochondrial substrate for energy production [4]. Conversely, we recently reported that in hypoxic KRAS mutant tumors, phospholipase C γ1 (PLCγ1) is suppressed, a phenomenon leading to impaired mitochondrial fitness and decreased FAO, which boosts tumor growth [29]. Taken together, these results highlight the level of metabolic heterogeneity among hypoxic and normoxic KRAS mutant tumors and the imperative need to carefully characterize them on a single-cell level in our pursuit of designing effective therapeutic strategies.
Taken altogether, targeting the lipid synthesis and degradation machinery in a KRASmutated context is a complicated concept, as there are multiple aspects to be considered ( Figure 1). However, targeting the enzymes and pathways involved in FA scavenging and utilization will surely set the ground for developing new cancer treatments.
tumors, phospholipase C γ1 (PLCγ1) is suppressed, a phenomenon leading to impaired mitochondrial fitness and decreased FAO, which boosts tumor growth [29]. Taken together, these results highlight the level of metabolic heterogeneity among hypoxic and normoxic KRASmutant tumors and the imperative need to carefully characterize them on a single-cell level in our pursuit of designing effective therapeutic strategies.
Taken altogether, targeting the lipid synthesis and degradation machinery in a KRAS-mutated context is a complicated concept, as there are multiple aspects to be considered ( Figure 1). However, targeting the enzymes and pathways involved in FA scavenging and utilization will surely set the ground for developing new cancer treatments.

Autophagy
The role of autophagy in cancer initiation and progression, as well as therapeutic targeting has been extensively described in many excellent reviews [30,31], but the general consensus is that its complex function acts in favor of the tumors. In KRAS-driven malignancies, the autophagic machinery is commonly upregulated [32]. However, tumor initiation and progression are affected differently, with the former being inhibited and the latter promoted by autophagy. Indeed, in a Kras G12D -driven PDAC mouse model, genetic ablation of autophagy results in increased tumor initiation, however, these tumors are lacking the ability to progress into adenocarcinomas, thus leading to improved survival irrespective of the p53 tumor suppressor status [33]. In Kras G12D -driven NSCLC, loss of autophagy via Atg7 deletion before lung tumor onset did not affect tumor growth, while blocked tumor progression in mice with preexisting lung cancer [34].
In PDAC cells, an interesting crosstalk has been unveiled between pancreatic stellate cells (PSCs) and cancer cells. In a nutrient-deprived context, PDAC cells stimulate autophagy in PSCs, and this leads to secretion of alanine. Alanine is then uptaken by PDAC cells

Autophagy
The role of autophagy in cancer initiation and progression, as well as therapeutic targeting has been extensively described in many excellent reviews [30,31], but the general consensus is that its complex function acts in favor of the tumors. In KRAS-driven malignancies, the autophagic machinery is commonly upregulated [32]. However, tumor initiation and progression are affected differently, with the former being inhibited and the latter promoted by autophagy. Indeed, in a Kras G12D -driven PDAC mouse model, genetic ablation of autophagy results in increased tumor initiation, however, these tumors are lacking the ability to progress into adenocarcinomas, thus leading to improved survival irrespective of the p53 tumor suppressor status [33]. In Kras G12D -driven NSCLC, loss of autophagy via Atg7 deletion before lung tumor onset did not affect tumor growth, while blocked tumor progression in mice with preexisting lung cancer [34].
In PDAC cells, an interesting crosstalk has been unveiled between pancreatic stellate cells (PSCs) and cancer cells. In a nutrient-deprived context, PDAC cells stimulate autophagy in PSCs, and this leads to secretion of alanine. Alanine is then uptaken by PDAC cells and used as alternative fuel for the TCA cycle, thus sustaining mitochondrial oxygen consumption and lipid synthesis and promoting growth during tumor initiation, but not progression [35]. The complexity of the interplay between tumor cells and the TME has also been elegantly shown in a recent work revealing that, upon induction of autophagy as a response to oxidative stress, KRAS G12D protein is secreted from PDAC cells and uptaken by macrophages. This event further stimulates FAO, promotes pro-tumor macrophage M2 polarization and facilitates tumor progression [36]. The above results suggested that inhibition of autophagy could be highly effective in suppressing PDAC growth. However, this was not the case as clinical trials observed limited to no efficacy of hydroxychloroquine, an orally administered FDA-approved autophagy inhibitor [37].
When it comes to the control of lipid metabolism, autophagy seems to be critical for maintaining fat and glycogen stores in mice both during fasting and fed state. Indeed, systemic Atg7 ablation leads to depletion of white adipose tissue in mice [34]. Moreover, inhibition of autophagy in CRC cells thwarts their ability to use FAs and hinders their proliferation, suggesting that mutant KRAS controls lipid fate by modulating the autophagic machinery [4]. Similarly, our group found that autophagy is crucial for the turnover of lipids from intracellular lipid stores (i.e., lipid droplets) in KRAS mutant pancreatic cancer. In a lipid-deprivation context, autophagy increases to provide cancer cells with the necessary lipids in KRAS mutant tumors, but not in healthy lung tissue. Indeed, concurrent extracellularly derived lipid depletion and autophagy inhibition increases cell death and suppresses PDAC progression [38]. Therefore, lipid deprivation could be exploited to render KRAS mutant PDAC tumors responsive to autophagy inhibitors.

The ATX-LPA Signaling Axis
Lysophosphatidic acid (LPA) is a phospholipid consisting of a glycerol backbone, a phosphate group and a FA chain that can vary in length and saturation [39]. LPA acts through LPA receptors, which are G-protein-coupled receptors, thus initiating signaling cascades involved in key cellular processes such as proliferation, survival, cytoskeletal changes, and calcium signaling [40,41]. LPA is produced mainly through two different pathways. Firstly, LPA can be generated via conversion of lysophosphatidylcholine (LPC) by autotaxin (ATX), a secreted glycoprotein that has lysophospholipase D (lysoPLD) activity [42]. Alternatively, phosphatidic acid (PA) can get deacylated by phospholipase A 1 or A 2 (PLA 1, PLA 2 ) [43].
Numerous in vitro and in vivo studies suggest that alterations in the levels of LPA or its receptors are involved in tumorigenesis. By far the largest body of research, with regard to the LPA signaling axis, focuses on LPA1 and LPA3 receptors. It has been shown that in PDAC cells treated long-term with cisplatin, the activity of LPA1 and LPA receptors increased cell motility and invasion capacity, as well as MMP-2 activation [44]. These advantages could be ablated by LPA1 and LPA3 receptor knockdown, indicating that the two receptors strongly contribute to the malignant phenotype that cells acquire during tumor progression in PDAC. The same work also suggested that increased cell motility of the long-term cisplatin treated cells is, at least in part, regulated by extracellular LPA produced by ATX [44]. On a similar note, PANC-R9 cells (a highly invasive cell line established from PANC-1 pancreatic cancer cell line) were found to have higher expression levels of LPA1 receptor compared to the parental cell line, while the expression level of LPA3 receptor was decreased. Interestingly, the invasive capacity was amplified by LPA only in the PANC-R9 cells, an event that was accompanied with increased expression level of ATX [45]. Recently, it has been revealed that PDAC cells uptake FAs and particularly LPC derived from PSCs, which they then use either for membrane synthesis, or as precursors to produce signaling lipids, mainly LPA, through ATX-mediated LPC hydrolysis. Of note, ATX is overexpressed in human PDAC and its inhibition, either genetically or pharmacologically, suppressed tumor growth in an orthotopic PDAC mouse model [46]. LPA has also been involved in PDAC cell chemotaxis and metastasis in vivo [47]. Key player of this regulation is the Neural Wiskott-Aldrich Syndrome Protein (N-WASP), which drives LPA1 receptor recycling and prevents its degradation. Overall, these findings imply that the two LPA receptors, as well as LPA per se, may have a direct impact in tumor aggressiveness and resistance to drugs and their targeting could simultaneously thwart multiple hallmarks of cancer, while sparing normal cells.
The connection between the expression of LPA receptors and drug resistance has also been investigated in a CRC setting. DLD1 cells that underwent long term treatment with fluorouracil (5-FU) exhibit a robust increase in the expression levels of LPA1 receptor.
Conversely, cisplatin treatment led to a markedly elevated expression of LPA6 receptor [48]. Using the same CRC cell line model, Shida et al. showed that LPA through LPA1 receptor stimulates cell migration, proliferation, adhesion, and the secretion of both VEGF and -in a dose dependent manner-IL-8, boosting their metastatic potential. The mechanism of LPA-induced IL-8 secretion, included degradation of IκBα and consequent activation of NF-κB [49].
Similarly, in a Kras G12D -driven lung adenocarcinoma mouse model, genetic deletion of ATX or LPA1 receptor suppressed lung tumorigenesis, confirming a pro-tumorigenic role of LPA signaling also in this context [50]. Notably, ATX was recently found to modulate also the TME because it can have a chemorepulsive action on tumor-infiltrating lymphocytes and circulating CD8+ T cells [51].
Taken altogether, it is becoming evident that KRAS-driven tumors heavily rely on the ATX-LPA signaling axis to acquire and maintain their aggressive and often therapy resistant phenotype. The mechanisms through which this is achieved seem to be cell line dependent and dictates further research. The heterogeneity in the expression pattern of LPA receptors across the different cancer types acts once more as a reminder that a "one size fits all" approach cannot be applied when planning a treatment strategy. It remains to be investigated why certain tumors rely on different LPA receptors, or their inhibition, to promote functions that will allow their propagation.

The Role of Polyunsaturated Fatty Acids (PUFAs) and Cholesterol
In view of the dependency of KRAS-driven tumors on exogenous lipids, when designing approaches to target lipid signaling it is important to consider the impact of the different extracellularly derived lipids on KRAS mutant cancer cells. During the last decades, a strong link between diet and cancer has been established, with high fat diet promoting tumor initiation, progression and, eventually, poorer survival [52]. Intriguingly, high calorie diet-induced obesity which leads to hypertrophic tumor-associated adipocytes in mouse and human PDAC setting, seems to increase the incidence and accelerate tumorigenesis by increasing inflammation [53][54][55]. However, in Kras G12D -driven lung cancer, a high calorie diet dampens tumor progression if given before tumor onset, by causing defective unfolded protein response (UPR) and unresolved endoplasmic reticulum (ER) stress, but increases tumor burden when administered after tumor onset [56]. Whether the timing of high calorie diet is important for tumor development and the exact underpinning mechanisms remain to be investigated, however, ER chaperones are unveiled as an attractive way to selectively target KRAS-driven lung tumors.
Although the role of specific FAs in different human cancer types is not fully unraveled yet, it is becoming clear that a high uptake of ω-3 PUFAs, such as docosahexaenoic acid (DHA) and eicosapentaenoic acid (EPA), can reduce the risk of initiation and progression of some cancers including colorectal, prostate, and breast cancer (Figure 2) [57][58][59][60][61]. In fact, Collet et al. initially proposed a direct reduction of RAS localization to the plasma membrane by DHA [62]. However, it was later shown that incorporation of DHA and EPA into the plasma membrane phospholipids suppresses phosphatidic acid-dependent oncogenic KRAS-driven effector interactions (i.e., ERK signaling), thus suppressing hyperproliferation of cancer cells in vitro and in vivo [63]. Therefore, DHA rises as a promising compound that could be used to treat RAS-driven cancers.

Figure 2.
The effect of ω-3 and ω-6 PUFAs on tumor progression. ω-3 PUFAs, such as DHA or EPA, can exert an anti-tumor effect. Increased dietary uptake of these lipids has been linked to decreased inflammatory status and tumorigenesis. This is achieved through inhibition of pro-proliferative mechanisms, including the ERK pathway, inhibition of angiogenesis and decrease of the metastatic capacity. Conversely, these pathways are boosted by a diet rich in ω-6 PUFAs, such as arachidonic acid (AA).
Accumulating data obtained from both in vitro and in vivo studies point towards a direct cytotoxic effect of certain PUFAs on cancer cells [64][65][66]. This is because certain phosphoglycerolipids (mainly phosphatidylethanolamines) containing polyunsaturated acyl chains are subjected to either oxidation by ROS or selective oxygenation by lipoxygenases (LOX), a process named lipid peroxidation, which leads to ferroptosis (an irondependent, non-apoptotic cell death induced by the accumulation of lipid hydroperoxides) [67][68][69]. Therefore, KRAS mutant tumors are equipped with potent antioxidant systems to be able to overcome the cytotoxic effects of PUFAs and generally survive in the presence of high ROS levels [70]. In this context, the glutathione peroxidase 4 (GPX4) is an important ferroptosis regulator as it converts toxic lipid hydroperoxides to non-toxic lipid alcohols at the expense of glutathione (GSH) [71]. This dependency exposes a cancer cell vulnerability, in which inhibition of GPX4 either directly or indirectly with erastin (a compound which inhibits the import of cystine, leading to GSH depletion and inactivation of GPX4) results in excessive lipid peroxidation causing cancer cell death [72]. Indeed, with the view of the ongoing effort to develop drugs that can efficiently target KRASmutated cancer cells, there are many recent reports that successfully leveraged the ferroptosis machinery to promote cell death in KRAS-driven tumors [73][74][75].
Furthermore, PUFAs activate PPARs, alter the expression pattern of oncogenes or oncosuppressors, and induce DNA damage [76][77][78]. With certainty, gaining better insight into the different cell functions that PUFAs can rewire will be a huge step forward in our efforts to design novel compounds and effectively tackle hard to treat malignancies.
As stated above, KRAS mutant cancer cells can induce the transcription of SREBPs, promoting cholesterol synthesis and uptake [22]. Moreover, increased LDL-R expression has been observed in all stages of KRAS mutant pancreatic cancer and is associated with increased disease recurrence rates. LDL-R silencing reduces the proliferative and clonogenic capacity of PDAC cells established from Pdx1-Cre;LSL-Kras G12D ;Ink4a/Arf flox/flox tumors [79]. LDL-R depletion also improves the response of cells to gemcitabine and leads to tumor regression, shedding light to not only an appealing target for therapeutic exploitation, but also to a potentially effective way of sensitizing cancer cells to conventional treatment regiments [79]. In sharp contrast, treatment with statins (drugs that lower LDL blood levels) accelerates PDAC growth of Pdx1-Cre;LSL-Kras G12D ;Trp53 flox/flox mice through TGF-β induction and epithelial to mesenchymal transition (EMT) activation, but dramatically Accumulating data obtained from both in vitro and in vivo studies point towards a direct cytotoxic effect of certain PUFAs on cancer cells [64][65][66]. This is because certain phosphoglycerolipids (mainly phosphatidylethanolamines) containing polyunsaturated acyl chains are subjected to either oxidation by ROS or selective oxygenation by lipoxygenases (LOX), a process named lipid peroxidation, which leads to ferroptosis (an iron-dependent, non-apoptotic cell death induced by the accumulation of lipid hydroperoxides) [67][68][69]. Therefore, KRAS mutant tumors are equipped with potent antioxidant systems to be able to overcome the cytotoxic effects of PUFAs and generally survive in the presence of high ROS levels [70]. In this context, the glutathione peroxidase 4 (GPX4) is an important ferroptosis regulator as it converts toxic lipid hydroperoxides to non-toxic lipid alcohols at the expense of glutathione (GSH) [71]. This dependency exposes a cancer cell vulnerability, in which inhibition of GPX4 either directly or indirectly with erastin (a compound which inhibits the import of cystine, leading to GSH depletion and inactivation of GPX4) results in excessive lipid peroxidation causing cancer cell death [72]. Indeed, with the view of the ongoing effort to develop drugs that can efficiently target KRAS mutated cancer cells, there are many recent reports that successfully leveraged the ferroptosis machinery to promote cell death in KRAS-driven tumors [73][74][75].
Furthermore, PUFAs activate PPARs, alter the expression pattern of oncogenes or oncosuppressors, and induce DNA damage [76][77][78]. With certainty, gaining better insight into the different cell functions that PUFAs can rewire will be a huge step forward in our efforts to design novel compounds and effectively tackle hard to treat malignancies.
As stated above, KRAS mutant cancer cells can induce the transcription of SREBPs, promoting cholesterol synthesis and uptake [22]. Moreover, increased LDL-R expression has been observed in all stages of KRAS mutant pancreatic cancer and is associated with increased disease recurrence rates. LDL-R silencing reduces the proliferative and clonogenic capacity of PDAC cells established from Pdx1-Cre;LSL-Kras G12D ;Ink4a/Arf flox/flox tumors [79]. LDL-R depletion also improves the response of cells to gemcitabine and leads to tumor regression, shedding light to not only an appealing target for therapeutic exploitation, but also to a potentially effective way of sensitizing cancer cells to conventional treatment regiments [79]. In sharp contrast, treatment with statins (drugs that lower LDL blood levels) accelerates PDAC growth of Pdx1-Cre;LSL-Kras G12D ;Trp53 flox/flox mice through TGF-β induction and epithelial to mesenchymal transition (EMT) activation, but dramatically decreases tumor progression in Pdx1-Cre;LSL-Kras G12D ;Trp53 wt/flox mice, potentially due to a TGF-β-mediated, p53-dependent apoptosis initiation [80,81]. Nevertheless, one could argue that disrupting cholesterol uptake by cancer cells or thwarting LDL-R expression can be a promising therapy, at least for a subset of patients, that deserves further investigation.

Lipid Mediators of Inflammation
Inflammation has been linked with the initiation and progression of cancer, by enabling the tumor to acquire hallmark properties [82][83][84][85][86][87][88]. In adult mice, both chronic pancreatitis and mutated KRAS are required to induce preneoplastic lesions and PDAC [89], suggesting that inflammation is important to drive tumorigenesis in mice. Indeed, shift of the TME into a more tumor-permissive state, impediment of anti-tumor immunity, and enhancement of pro-tumorigenic signaling are commonly observed after chronic inflammation status [90]. Furthermore, KRAS mutant cancer cells produce inflammatory lipid mediators, establishing an inflammatory microenvironment [90]. In this well-orchestrated process, a pivotal role is played by different lipid molecules that act either as pro-or anti-inflammatory autacoids. The former comprise, among others, prostaglandins and leukotrienes [91]. On the other hand, specialized pro-resolving lipid mediators (SPMs) are produced locally by either epithelial, or immune cells and act as local hormones, binding to their specific receptors and thus initiating resolution of inflammation and tissue restoration [92]. From that perspective, SPMs have been shown to be able to modulate angiogenesis, stimulate efferocytosis, and mitigate the inflammatory response [91].
Unresolved inflammation and consequently increased risk of cancer initiation can be due to either sustained production of pro-inflammatory mediators, or lack of pro-resolving activity. It is therefore reasonable that targeting the inflammatory machinery attracted a lot of scientific attention as a promising therapeutic approach to combat cancer.

The Pro-Inflammatory Front: Prostaglandins
Prostaglandins, which derive from ω-6 PUFAs, namely arachidonic acid, act in a tumor promoting way both by directly activating signaling pathways, which control cancer cell proliferation, anchorage-independent growth, migration, apoptosis and angiogenesis, and by establishing an immunosuppressive TME ( Figure 2) [93,94]. Despite extensive research, the exact molecular mechanisms through which tumor growth is promoted remain elusive. However, this is slowly changing, particularly with regard to prostaglandin E 2 (PGE 2 ) and how its biosynthesis pathway is involved in many different aspects of cancer progression (Table 1).
In a CRC orthotopic mouse model, PGE 2 increased the invasiveness and metastatic capacity of cancer cells by elevating the expression levels of miR675-5p, which in turn binds to p53 mRNA and prevents its translation [95]. In contrast, in a clinical study conducted by Zhang et al., a robust decrease in serum concentration of PGE 2 and its product, 20-hydroxy-PGE 2, were observed in CRC patients compared to the healthy cohort [96].
Accumulation of PGE 2 can be due to either increased biosynthesis, or decreased degradation through 15-hydroxyprostaglandin dehydrogenase (15-PGDH), the enzyme responsible for degrading prostaglandins. In Kras G12D -driven lung adenocarcinomas, the production of prostaglandins PGE 2 , PGD 2 , and PGI 2 is greatly increased compared to healthy lungs. This increase is ACSL3 dependent as Kras G12D ;Acsl3 −/− lung tumors evidence impaired prostaglandin production. Increased prostaglandin synthesis requires sufficient amounts of their precursor arachidonic acid. How KRAS mutant cancer cells manage to sustain such high levels of arachidonic acid to be able to sustain the prostaglandin production is not well understood. Notably, the lysophosphatidylinositol-acyltransferase 1 (LPIAT1), which is involved in reacylation of phospholipids with specificity for arachidonic acid, is overexpressed in KRAS mutant lung cancer [97]. We recently shed light to this mechanism by determining that ACSL3 channels arachidonic acid to LPIAT1 to boost the pool of arachidonic acid-bound phosphatidylinositol (PI) and consequently accommodate the high prostaglandin production rates [97]. Alternatively, the strongly upregulated miR-574-5p directly antagonizes CUGBP1, a negative regulator of PGE synthase-1 (PGES-1), allowing the expression of an alternative PGES-1 3 UTR variant, increasing PGE 2 production and promoting lung tumor growth in vivo [98].
In PDAC, 15-PGDH expression is inversely correlated with ALDH1, a well described cancer stem cell (CSC) marker and pharmacological inhibition of 15-PGDH leads to the expansion of the ALDH1-positive PDAC cells in vitro and in vivo [99]. Moreover, interleukin-1β-mediated decrease of 15-PGDH is often observed in PDAC and is associated with poor prognosis [100].
The arachidonic acid/PLA 2 /COX2/PGE 2 synthesis pathway can also get stimulated in cancer cells by the TME. In this context, IL-6 is secreted by macrophages in the TME, an event that induces the translocation of β-catenin from the cytoplasm to the nucleus, leading to EMT and increased invasiveness of lung cancer cells [101]. Once produced, PGE 2 upregulates the levels of PD-1 in infiltrating CD8 + T cells via EP2 and EP4, resulting in immune tolerance in the lung cancer TME [102]. Lastly, further highlighting the complexity of the prostaglandins production pathway, a recent study using an in vitro KRAS mutant NSCLC model showed that, unlike COX2, inhibition of PGES creates a pro-cell death state which coincides with accumulation of sphinganine and dihydroceramide C16:0, two sphingolipid species associated with cancer cell death [103]. Therefore, these data suggest that KRAS mutant cancer cells crosstalk with the TME to sustain their high prostaglandin demand, leading to tumor progression and invasion.
Taken together, the above data underscore the therapeutic potential of suppressing prostaglandin production not only in cancer cells but also in components of the TME.

Pro-Resolving Lipid Mediators
The most thoroughly investigated SPM is lipoxin A4 (LXA 4 ), an anti-inflammatory metabolite derived from AA. In pancreatic cancer, LXA 4 is associated with attenuated cancer cell invasion and metastasis by inhibiting KRAS-induced ROS production, as well as ERK/MMPs and TGF-β1 signaling pathways [104,105]. Furthermore, LXA 4 can modulate different elements of the TME in various cancer models. In CRC, LXA 4 has a tumor suppressing role by targeting, at least in part, regulatory B-cells and as a result facilitating the activity of CD8 + cytotoxic T cells in the TME [106].
In addition to LXA 4 , resolvins also have therapeutic potential. In a pancreatic cancer model, RvD1 did not only modify the TME by supporting the cytotoxic activity of NK cells, but it also induced tumor cell apoptosis [107]. In a lung cancer setting, RvD1 and RvD2 suppressed the TGF-β1-induced EMT in vitro, further supporting the fact that these lipid mediators exert key anti-tumor functions that can also be independent of their antiinflammatory properties [108].
A few years back, aspirin was in the spotlight about its potential anti-tumor effects. What sets aspirin apart from other NSAIDs is the fact that, apart from blocking prostaglandins synthesis by inhibiting the pro-inflammatory COX pathway, is also responsible for stimulating the production of anti-inflammatory mediators, such as aspirin-triggered lipoxins (AT-LXs) and resolvins (AT-RvDs), albeit rather weakly [109,110]. In fact, treatment with AT-LXA 4 , or AT-RvDs strongly reduces tumor growth in a Lewis lung carcinoma cell (LLC; KRAS G12C mutated) -derived lung cancer mouse model, by negatively regulating the secretion of pro-inflammatory cytokines including macrophage migration inhibitory factor (MIF), plasminogen activator inhibitor-1 (PAI-1), and C-C motif chemokine ligand 2 (CCL2) and stimulating macrophage phagocytosis of tumor cell debris [111]. The substantially lower concentration required to achieve these effects means that by directly targeting the resolvin pathways, the aspirin-induced toxicity and immunosuppression no longer poses a limitation (Table 1).

Conclusions
Over the last years, a growing body of evidence substantiated the key role of lipid metabolism in carcinogenesis. Thus, it is now widely accepted that cancer cells display differential regulation of lipid metabolism, thus affecting tumor progression, invasion, and metastasis through an extremely dynamic and complex signaling network. Against this backdrop, developing novel drugs that will successfully target lipid metabolism, to prevent or efficiently treat cancer, is an attractive prospect. Therefore, understanding how cancer cells adapt their metabolism to meet their high energy and biosynthetic needs is of outmost importance. For instance, even though FA synthesis and FAO were once considered as mutually exclusive, it is nowadays known that both cellular processes can, in fact, be concomitantly active.
KRAS-driven cancers are notorious for their aggressiveness and resistance to therapy. It is therefore tempting to speculate that they bear a specific lipid metabolic "fingerprint", the identification of which will allow us to efficiently target them. It is becoming apparent that apart from synthesizing lipids de novo, those tumor cells are also able to uptake lipids, sometimes even by stimulating their secretion from the surrounding tissue, underscoring once more the importance of detailed investigation of the TME. The excellent work of various research groups that was summarized in this review, indicates that tumors bearing oncogenic KRAS rewire their lipid metabolism in such a tissue-and context-specific way that allows them to adapt to any conditions. This is manifested in many different cellular functions, including FA synthesis, FAO, autophagy, and inflammation. It is evident that in our pursuit of a better understanding of these tumors, we need to evaluate the available preclinical and clinical data not only in a tissue-, but also oncosuppressor-and time-specific manner.