AbstractObjectiveThe types and functions of lipids involved in glioblastoma (GB) are not well known. Lipidomics is a new field that examines cellular lipids on a large scale and novel aplication of lipidomics in the biomedical sciences have emerged. This study aimed to investigate the potential of blood lipids for use as biomarkers for the diagnosis of GB via untargated lipidomic approach. Gaining a deeper understanding of lipid metabolism in patients with GB can contribute to the early diagnosis with GB patiens and also development of novel and better therapeutic options.
MethodsThis study was performed using blood samples collected from 14 patients (eight females and six males) and 14 controls (eight females and six males). Lipids were extracted from blood samples and quantified using phosphorus assay. Lipid profiles of between patients with GB and controls were compared via an untargeted lipidomics approach using 6530 Accurate-Mass Q-TOF LC/MS mass spectrometer.
ResultsAccording to the results obtained using the untargeted lipidomics approach, differentially regulated lipid species, including fatty acid (FA), glycerolipid (GL), glycerophospholipid (PG), saccharolipid (SL), sphingolipid (SP), and sterol lipid (ST) were identified between in patients with GB and controls.
INTRODUCTIONGlioblastoma (GB) is the most common and aggressive primary intracranial mass lesion observed in adults. Despite there being multimodal therapies against it, the average survival is approximately 12-14 months [4]. Normal cells primarily rely on mitochondrial oxidative phosphorylation, which typically has a relatively low glycolytic rate, to generate the energy needed for cellular processes. In contrast, energy production in cancer cells is mainly dependent on glycolysis followed by lactic acid fermentation. This phenomenon, termed as the “Warburg effect,” has long been recognized as the critical metabolic difference between cancer and normal cells [3,29].
Rapidly proliferating cells also exhibit alterations in lipid metabolism, and increased lipogenesis is considered another metabolic characteristic of cancer cells. Accordingly, glioma tissues have been shown to have increased lipid synthesis, and nuclear magnetic resonance studies have demonstrated a correlation between the lipid resonance spectrums of GB extracts and the degree of malignancy [11,35]. Cancer cells utilize exogenous fatty acids (FAs) for growth and increased de novo lipid synthesis [19]. Lipids, including FAs, triglycerides (TAGs), and phospholipids (PLs), are the mediators of signal transduction involved in numerous physiological responses. However, the mechanism by which lipids play a role in the development and progression of brain tumors is still unclear. Studies investigating brain tissues of patients with GB have shown that lipid droplets (LDs) that are not observed in normal brain tissues are highly abundant in tumor tissues; however, the types and functions of the lipids involved in GB are not well known [33]. A better understanding of lipid metabolism can contribute to the development of novel treatment modalities for GB. Given the critical role of lipids in cell membrane formation and signal transduction, identifying the key players involved in the reprogramming of lipid metabolism will enable the development of novel therapeutic strategies and possible biomarkers for GB.
Lipidomics is a branch of science that focuses on the types of lipids and biological roles of proteins involved in lipid metabolism and function, including their complete characterization and gene regulation analysis [24]. Exploratory lipidomics can be classified into three types according to the analytical objective : focused lipidomics (lipid profiling), targeted lipidomics (targeted lipid analysis), and untargeted lipidomics (universal lipid profiling) [36,42]. Briefly, lipidomics involves the identification and quantification of lipids in biological systems [9]. Studies have shown that certain diseases (e.g., Alzheimer’s disease, schizophrenia, bipolar disorder, multiple sclerosis, chronic kidney failure, and cystic fibrosis) and cancers (e.g., prostate, insulin growth factor receptor-2 (IGFR-2)- positive metastatic breast, and colorectal cancers) are closely related to changes in lipid ratio and that some lipid molecules are associated with the development of certain diseases [1,8,10,13,17,22,24,25,28,30,34,37,39,41,43,44]. The outcomes of the studies suggest that alterations in the lipid profiles of different lipid types specific to different diseases can be used as biomarkers for that disease.
In our study, lipids isolated from blood samples obtained from patients with GB were investigated for the first time using an untargeted lipidomics approach to evaluate the potential of lipid species that vary between healthy individuals and patients with GB for use as biomarkers.
MATERIALS AND METHODSThis study was approved by University Ethics Committee of Sivas Cumhuriyet University (approval number : 2020-06/02, date of approval : November 6, 2020). The patients who presented to the brain and neurosurgery clinic with a preliminary diagnosis of an intracranial mass and were diagnosed with GB (World Health Organization grade IV) via pathological examination were included in this study. A control group comprising age- and sex-matched healthy individuals who did not have any chronic diseases and did not use any medications were included. Blood samples were collected from patients and controls (Table 1).
Sample collectionOf the 1-mL blood sample, 500 µL was immediately mixed with 1 mL of methanol:water (1.0 : 0.4 volume/volume [v/v]) and then placed stored at -80°C until lipid extraction was performed as described below.
Bligh and Dyer method of blood lipid extractionLipids were extracted using chloroform and methanol according to the Bligh and Dyer method [6]. Briefly, blood samples suspended in 1.25 mL of methanol and 1.25 mL of chloroform were subjected to lipidomics analysis. Tubes were vortexed for 30 seconds, allowed to sit for 10 minutes on ice, and centrifuged (213×g; 5 mintues), and the bottom chloroform layer was transferred to a new test tube. The extraction steps were repeated for a second time, and the obtained chloroform layers were combined. The chloroform layers were dried under nitrogen, reconstituted with 50 µL of methanol : chloroform (3 : 1 v/v), and stored at -80°C until further analysis.
Lipid phosphorus assayLipid phosphorus was quantified using the phosphorus assay2). First, 400 µL of sulphuric acid (5 M) was added to the extracted lipids (10 µL), and the solution was heated in a glass test tube at 180-200°C for 1 hour. Next, 100 µL of 30% H2O2 was added to the tube while vortexing, and the tube was heated at 180-200°C for 1.5 hours. A reagent (4.6 mL; 1.1 g ammonium molybdate tetrahydrate + 12.5 mL sulphuric acid + 500 mL double distilled water) was added and vortexed, followed by the addition of 100 µL of 15% ascorbic acid and vortexing. The solution was heated for 7-10 minutes at 100°C, and a 150-µL aliquot was used to measure the absorbance at 830 nm.
Quadrupole time-of-flight liquid mass spectrometer (Q-TOF LC/MS) : electrospray ionisation mass spectrometry (ESI-MS)-based lipid analysisLipid extract samples (500 pmol/µL) were prepared by reconstitution in chloroform:methanol (2 : 1, v/v). ESI-MS was performed as described previously [18,26,39] using an Agilent Technologies 6530 Accurate-Mass Q-TOF LC/MS mass spectrometer (Agilent Technologies, Santa Clara, CA, USA) with a dry nitrogen gas flow rate of 8 L/min at 350°C and a nebulizer pressure of 30 psi. The scanning range was from 200 to 1000 mass/charge (m/z) ratio for 5 µL of the sample scanned in positive and negative ion mode for 2.5 minutes with a mobile phase of acetonitrile : methanol : water (2 : 3 : 1) in 0.1% ammonium formate. As described previously [32], qualitative identification of individual PL molecular species was based on their calculated theoretical monoisotopic mass values, subsequent MS/MS analysis, and their level normalized to either the total ion count or the most abundant PL. Fragmentation was performed using an Agilent Technologies 6530 Accurate-Mass Q-TOF LC/MS mass spectrometer equipped with an ESI source. The direct injection feature of the HPLC system (Agilent Technologies) was used to introduce the analyte. The dry nitrogen gas flow rate was 8.0 L/min at 350°C. ESI-MS analysis spectrums in positive and negative ion modes were obtained using Agilent Technologies 6530 Accurate-Mass Q-TOF LC/MS mass spectrometer. A tentative ID was assigned based on the m/z ratio and the LIPID MAPS database [20].
Statistical analysisMultivariate principal component analysis (PCA) was performed using MetaboAnalyst 5.0 (https://www.metaboanalyst.ca) [21]. Automatic peak detection and spectrum deconvolution was performed using a peak width set at 0.5. Data were normalized to the sum, and scaled to the Z-value. Analysis parameters consisted of interquartile range filtering and sum normalization without the removal of outliers from the dataset. Features were selected based on volcano plot analysis and were further identified using MS/MS analysis. Significance for the volcano plot analysis was determined based on a fold change threshold of 2.00 and p≤0.05. Following identification, the total ion count was used to normalize each parent lipid level, and the change in the relative abundance of that lipid species as compared to its control was determined. This is the standard method for lipidomics analysis as reported in previous studies [18,26].
RESULTSThe data obtained from ESI-MS analysis were analyzed using the parameters presented in the Materials and Methods section via MetaboAnalyst 5.0 and Lipid Maps databases. Figs. 1A and B, 2A (for positive ion mode) and Figs. 3A and B, 4A (for negative ion mode) represented that the whether there was a difference between the GB and control groups via multivariate analyses, such as PCA, partial least squares discriminant analysis (2D-PLS-DA), and OrthoPLSDA analysis. PCA is the most used explorative multivariate method. PCA is generally preferred for purposes of data reduction. The primary goal of PCA is to explain the variation in the original data using a reduced space, defined by variables called principal components (PC1 and PC2), which retain most of the relevant information from the original data. The ideal situation occurs when control and treated samples appear far enough to be completely distinguished. The 2D-PLS-DA analysis of the targeted acquired data (Figs. 1B and 3B) resulted in better model separation compared to the PCA model (Figs. 1A and 3A) created from the blood samples. The score plots of the 2D-PLS-DA from untargeted lipidomics were clearly clustered between GB patients (green) and control (red) groups. Further, t-test was performed (Fig. 1C for positive ion mode; Fig. 3C for negative ion mode). Assuming a fold change threshold of 2.0 and a pvalue of 0.05, lipid types (detected by t-test) that differed between the two groups were identified using this changing ratio (fold change; Fig. 1D for positive ion mode; Fig. 3D for negative ion mode). Volcano plot, which numerically gives the m/z ratios of lipid types varying between groups, was obtained by combining the t-test and the logarithm of the fold change graphs (Fig. 1E for positive ion mode; Fig. 3E for negative ion mode). The m/z ratios obtained from the volcano plot were interpreted using the Lipid Maps database, and the classes of lipid types corresponding to these m/z ratios were determined using MS-MS validation (Tables 2 and 3). Orthogonal projections to latent structures (OPLS) has a similar predictive capacity compared to PLS and improves the interpretation of the predictive components and of the systematic variation (Figs. 2A and 4A) [27]. In particular, OPLS modeling of single responses only requires one predictive component.
Table 2 presents the corresponding lipid classes in the Lipid Maps database of 32 significantly altered (p<0.05) m/z ratios obtained from the volcano plot data. Fig. 2B shows the variable importance projection (VIP) scores of the lipid types that were significantly different (p<0.05) between patients with GB and controls, with m/z ratios obtained from the volcano plot on the Y-axis. The levels of 17 and 15 lipid types were found to be higher (shown in red) and lower (shown in blue), respectively, in patients with GB than in controls. Table 3 presents the corresponding lipid classes in the Lipid Maps database of 30 significantly altered (p<0.05) m/z ratios obtained from the volcano plot data. Fig. 4B shows the VIP scores of the lipid species found to be different between patients with GB and controls, with m/z ratios obtained from the volcano plot on the Y-axis. The levels of 20 and 10 lipid types were found to be higher (shown in red) and lower (shown in blue), respectively, in patients with GB than in controls. These lipid types with increased and decreased levels due to GB are predicted as lipid biomarkers for GB.
DISCUSSIONGB is the most common and rapidly progressing malignant form of primary brain tumors of the central nervous system. It is characterized by a poor prognosis [31]. It is highly invasive, and despite the current treatment options, improved survival rates have not been reported over the past two decades. Biomarkers can be considered as diagnostic, prognostic, or therapeutic indicators of a disease. New approaches and technologies based on system biology have the potential to identify biomarkers that can be used as new therapeutic targets for GB. Identification of cancer-specific biomarkers and detection of tumors from easily accessible samples, such as bodily fluids (e.g., blood, urine, or saliva), will be a significant advance in the field of neuro-oncology [14,16]. There is an immense need to advance the use of biomarkers in the field of neuro-oncology as current imaging systems often fail to provide adequate information about relapsing tumor growth or the actual biological status of either the primary or recurrent tumor. This lack of knowledge leads to a fairly uniform treatment regimen for every patient, precluding an individualized approach for the management of the disease and the assessment of individual responses to treatment.
Lipids stored in tumor cells are thought to play a number of critical roles during nutritional stress, including energy production, membrane biogenesis, cellular signaling, and nutrient transport [38]. In addition to other functions, lipids essentially act as structural components of cellular membranes. Lipids can be detected in brain tissues due to cell membrane destruction and necrosis of malignant brain tumors, such as GB. Lipidomics analyses revealed the accumulation of five major lipid classes in GB, predominantly ceramides, total polar lipids (TPLs), diacylglycerol (DAGs), TAGs, and sphingomyelins (SMs). In previous studies, higher amounts of different types of PLs were observed in the serum of patients with various primary brain tumors. Similarly, under lipid-restricted growth conditions, cancer cells have been reported to exhibit an increased dependence on de novo FA synthesis to maintain their growth and survival. In a study by Taïb et al. [33], multiple changes in the lipidomics profiles of cells primarily including PLs, DAGs, and TAGs were demonstrated in response to the absence of serum lipids. Accordingly, they proposed that alterations in lipid types may indicate putative metabolic pathways that mediate cell growth in GB. Additionally, they reported that GB cells alter their lipid composition as an adaptation mechanism in response to exogenous monounsaturated long chain FAs (e.g., oleic acid) through increased TAG accumulation and FA esterification and oxidation. Oleic acid also stimulates GB proliferation through a mechanism involving monoacylglycerol lipase [33]. Examination of brain tissues collected from patients with GB shows that LDs are abundant in tumor tissues but are not found in normal brain tissues [33]. Taïb et al. [33] treated U138 GB cells with oleic acid to investigate how FAs are utilized by GB cells and assess their role in GB proliferation. This treatment induces the accumulation of perilipin-2-coated LDs containing TAGs enriched in C18 : 1 FAs and an increase in FA oxidation. Interestingly, oleic acid also increased glucose utilization and proliferation of GB cells. In contrast, the pharmacological inhibition of monoacylglycerol lipase reduced GB proliferation. Hence, it was suggested that monounsaturated FAs increase GB proliferation through triglyceride metabolism, indicating a novel LD-mediated pathway that may be a therapeutic target for GB. Hu et al. [15] orally administered carbon-13 (13C) FAs to mice using a gastric probe and reported a significant 13C increase in gliomas and a minor 13C increase in capillary endothelial cells of the normal brain tissue. These results were supported by a previous study showing the disruption of the blood-brain barrier in an experimental brain metastases model [40]. Moreover, lipids containing FAs, TAGS, and PLs have been implicated as mediators of signal transduction involved in several physiological reactions [23]. Circulating lipid types have not been extensively studied as putative biomarkers in patients with GB; however, 24S-hydroxycholesterol is among the brain-specific lipids identified in the systemic blood circulation [5]. However, elevated serum levels of 24S-hydroxycholesterol are only observed following severe central nervous system trauma and not in response to brain tumors [7].
In general, GB xenograft tumor tissues have been observed to have significantly lower lipid levels compared with normal brain tissues. These results suggest that GB cells can oxidize FA as an additional energy source in a nutrient-free cancer environment. Normal brain tissues have extensive cellular insulation containing lipid-rich myelin. The replacement of normal neuronal cells by tumor cells is accompanied by a reduction in lipid-rich myelin, followed by a reduction in the overall lipid profile of the tumor. Ha et al. [12] investigated lipid biomarkers in ectopic and orthotopic human GB xenograft models. Proteins, metabolites, and lipids were isolated from the collected tumor tissues following the injection of primary patient cell lines, GBM10 and GBM43, into the lateral and right cerebral hemispheres of nonobese diabetic/severe combined immunodeficiency (NOD/SCID) mice. Lipid analysis was performed via reversed-phase high-performance liquid chromatography coupled with Fourier transform ion cyclotron resonance MS. More than 500 lipids were identified in each tumor model, and a comparison of ectopic and orthotopic tumor models revealed that the most prominent changes in lipid types predominantly occurred in four major lipid classes―glycosphingolipids, glycerophosphoethanolamines, triacylglycerols, and glycerophosphoserines [12].
CONCLUSIONIn our study, all lipid profiles of patients with GB and controls were compared using the untargeted lipidomics approach. Lipid types that differed significantly between patients with GB and controls were determined via screening using both positive and negative ion detection modes. The results obtained using the untargeted lipidomics approach predicted sxt-two m/z ratios which corresponding different lipid types with significantly increased/decreased levels (p<0.05) in patients with GB and controls as possible biomarkers for GB. With the application of the untargeted lipidomics approach, specific lipid classes can distinguished and the m/z ratios of the lipid types corresponding to more than one lipid class (Tables 2 and 3) can be determined, which can help predict more lipid types as biomarkers. In conclusion, lipid classes such as FA, glycerophospholipid, and glycerolipid displayed the most significant changes in patients with GB; however, the changes were also detected in a small number of lipid types among sphingolipid and sterol lipid classes. We propose that these lipid types can be used as possible biomarkers for GB diagnosis and also development different treatment stratecies.
NotesInformed consent Informed consent was obtained from all individual participants included in this study. Author contributions Conceptualization : BS, SŞB; Data curation : BS, ZB, SŞB; Formal analysis : SŞB; Funding acquisition : BS, ZB, SŞB; Methodology : BS, ZB, SŞB; Project administration : BS, ZB, SŞB; Visualization : BS, SŞB; Writing - original draft : BS, SŞB; Writing - review & editing : BS, ZB, SŞB Table 1.
Table 2.
Table 3.
References1. Astarita G, Piomelli D : Towards a whole-body systems [multi-organ] lipidomics in Alzheimer’s disease. Prostaglandins Leukot Essent Fatty Acids 85 : 197-203, 2011
3. Beloribi-Djefaflia S, Vasseur S, Guillaumond F : Lipid metabolic reprogramming in cancer cells. Oncogenesis 5 : e189, 2016
4. Bilgin E, Duman BB, Altintas S, Cil T, Gezercan Y, Okten AI : Predictors of survival in Turkish patients with primary glioblastoma. Turk Neurosurg 31 : 641-653, 2021
5. Björkhem I, Lütjohann D, Diczfalusy U, Ståhle L, Ahlborg G, Wahren J : Cholesterol homeostasis in human brain: turnover of 24S-hydroxycholesterol and evidence for a cerebral origin of most of this oxysterol in the circulation. J Lipid Res 39 : 1594-1600, 1998
6. Bligh EG, Dyer WJ : A rapid method of total lipid extraction and purification. Can J Biochem Physiol 37 : 911-917, 1959
7. Bretillon L, Sidén A, Wahlund LO, Lütjohann D, Minthon L, Crisby M, et al : Plasma levels of 24S-hydroxycholesterol in patients with neurological diseases. Neurosci Lett 293 : 87-90, 2000
8. Del Boccio P, Pieragostino D, Di Ioia M, Petrucci F, Lugaresi A, De Luca G, et al : Lipidomic investigations for the characterization of circulating serum lipids in multiple sclerosis. J Proteomics 74 : 2826-2836, 2011
9. Ejsing CS, Sampaio JL, Surendranath V, Duchoslav E, Ekroos K, Klemm RW, et al : Global analysis of the yeast lipidome by quantitative shotgun mass spectrometry. Proc Natl Acad Sci U S A 106 : 2136-2141, 2009
10. Guerrera IC, Astarita G, Jais JP, Sands D, Nowakowska A, Colas J, et al : A novel lipidomic strategy reveals plasma phospholipid signatures associated with respiratory disease severity in cystic fibrosis patients. PLoS One 4 : e7735, 2009
11. Guo D, Bell EH, Chakravarti A : Lipid metabolism emerges as a promising target for malignant glioma therapy. CNS Oncol 2 : 289-299, 2013
12. Ha SJ, Showalter G, Cai S, Wang H, Liu WM, Cohen-Gadol AA, et al : Lipidomic analysis of glioblastoma multiforme using mass spectrometry. Anal Chem 79 : 8423-8430, 2007
13. Han X : Multi-dimensional mass spectrometry-based shotgun lipidomics and the altered lipids at the mild cognitive impairment stage of Alzheimer’s disease. Biochim Biophys Acta 1801 : 774-783, 2010
14. Holdhoff M, Yovino SG, Boadu O, Grossman SA : Blood-based biomarkers for malignant gliomas. J Neurooncol 113 : 345-352, 2013
15. Hu X, Matsumoto K, Jung RS, Weston TA, Heizer PJ, He C, et al : GPIHBP1 expression in gliomas promotes utilization of lipoprotein-derived nutrients. Elife 8 : e47178, 2019
16. Jayaram S, Gupta MK, Polisetty RV, Cho WC, Sirdeshmukh R : Towards developing biomarkers for glioblastoma multiforme: a proteomics view. Expert Rev Proteomics 11 : 621-639, 2014
17. Jia L, Wang C, Zhao S, Lu X, Xu G : Metabolomic identification of potential phospholipid biomarkers for chronic glomerulonephritis by using high performance liquid chromatography-mass spectrometry. J Chromatogr B Analyt Technol Biomed Life Sci 860 : 134-140, 2007
18. Kinsey GR, Blum JL, Covington MD, Cummings BS, McHowat J, Schnellmann RG : Decreased iPLA2gamma expression induces lipid peroxidation and cell death and sensitizes cells to oxidant-induced apoptosis. J Lipid Res 49 : 1477-1487, 2008
19. Kuemmerle NB, Rysman E, Lombardo PS, Flanagan AJ, Lipe BC, Wells WA, et al : Lipoprotein lipase links dietary fat to solid tumor cell proliferation. Mol Cancer Ther 10 : 427-436, 2011
21. MetaboAnalyst : MetaboAnalyst - statistical, functional and integrative analysis of metabolomics data Available at : https://www.metaboanalyst.ca/
22. Min HK, Lim S, Chung BC, Moon MH : Shotgun lipidomics for candidate biomarkers of urinary phospholipids in prostate cancer. Anal Bioanal Chem 399 : 823-830, 2011
23. Muro E, Atilla-Gokcumen GE, Eggert US : Lipids in cell biology: how can we understand them better? Mol Biol Cell 25 : 1819-1823, 2014
24. Navas-Iglesias N, Carrasco-Pancorbo A, Cuadros-Rodríguez L : From lipids analysis towards lipidomics, a new challenge for the analytical chemistry of the 21st century. Part II: analytical lipidomics. Trends Anal Chem 28 : 393-403, 2009
25. Ollero M, Astarita G, Guerrera IC, Sermet-Gaudelus I, Trudel S, Piomelli D, et al : Plasma lipidomics reveals potential prognostic signatures within a cohort of cystic fibrosis patients. J Lipid Res 52 : 1011-1022, 2011
26. Peterson B, Stovall K, Monian P, Franklin JL, Cummings BS : Alterations in phospholipid and fatty acid lipid profiles in primary neocortical cells during oxidant-induced cell injury. Chem Biol Interact 174 : 163-176, 2008
27. Pinto RC, Trygg J, Gottfries J : Advantages of orthogonal inspection in chemometrics. J Chemom 26 : 231-235, 2012
28. Sabbagh MN, Sandhu S, Kolody H, Lahti T, Silverberg NB, Sparks DL : Studies on the effect of the apolipoprotein E genotype on the lipid profile in Alzheimer’s disease. Curr Alzheimer Res 3 : 157-160, 2006
30. Schwarz E, Prabakaran S, Whitfield P, Major H, Leweke FM, Koethe D, et al : High throughput lipidomic profiling of schizophrenia and bipolar disorder brain tissue reveals alterations of free fatty acids, phosphatidylcholines, and ceramides. J Proteome Res 7 : 4266-4277, 2008
31. Shukla G, Alexander GS, Bakas S, Nikam R, Talekar K, Palmer JD, et al : Advanced magnetic resonance imaging in glioblastoma: a review. Chin Clin Oncol 6 : 40, 2017
32. Taguchi R, Hayakawa J, Takeuchi Y, Ishida M : Two-dimensional analysis of phospholipids by capillary liquid chromatography/electrospray ionization mass spectrometry. J Mass Spectrom 35 : 953-966, 2000
33. Taïb B, Aboussalah AM, Moniruzzaman M, Chen S, Haughey NJ, Kim SF, et al : Lipid accumulation and oxidation in glioblastoma multiforme. Sci Rep 9 : 19593, 2019
35. Tugnoli V, Tosi MR, Tinti A, Trinchero A, Bottura G, Fini G : Characterization of lipids from human brain tissues by multinuclear magnetic resonance spectroscopy. Biopolymers 62 : 297-306, 2001
36. Vaz FM, Pras-Raves M, Bootsma AH, van Kampen AH : Principles and practice of lipidomics. J Inherit Metab Dis 38 : 41-52, 2015
37. Wood PL : Mass spectrometry strategies for clinical metabolomics and lipidomics in psychiatry, neurology, and neuro-oncology. Neuropsychopharmacology 39 : 24-33, 2014
38. Yang K, Rich JN : A delicate initiation: lipolysis of lipid droplets fuels glioblastoma. Mol Cell 81 : 2686-2687, 2021
39. Zhang L, Peterson BL, Cummings BS : The effect of inhibition of Ca2+- independent phospholipase A2 on chemotherapeutic-induced death and phospholipid profiles in renal cells. Biochem Pharmacol 70 : 1697-1706, 2005
40. Zhang RD, Price JE, Fujimaki T, Bucana CD, Fidler IJ : Differential permeability of the blood-brain barrier in experimental brain metastases produced by human neoplasms implanted into nude mice. Am J Pathol 141 : 1115-1124, 1992
41. Zhang Y, Wang Y, Guo S, Guo Y, Liu H, Li Z : Ammonia-treated N-(1-naphthyl) ethylenediamine dihydrochloride as a novel matrix for rapid quantitative and qualitative determination of serum free fatty acids by matrix-assisted laser desorption/ionization-Fourier transform ion cyclotron resonance mass spectrometry. Anal Chim Acta 794 : 82-89, 2013
42. Zhao YY, Cheng XL, Lin RC : Lipidomics applications for discovering biomarkers of diseases in clinical chemistry. Int Rev Cell Mol Biol 313 : 1-26, 2014
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