Lack of LCAT reduces the LPS-neutralizing capacity of HDL and enhances LPS-induced inflammation in mice

Πετροπούλου, Περιστέρα-Ιωάννα; Berbée, Jimmy F.P.; Theodoropoulos, Vassilios; Hatziri, Aikaterini; Stamou, Panagiota; Karavia, Eleni A.; Spyridonidis, Alexandros; Καραγιαννίδης, Ιορδάνης; Kypreos, Kyriakos E.

doi:10.1016/j.bbadis.2015.07.010

Cited by 34 publications

(40 citation statements)

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“…GO analysis of differentially expressed genes showed significantly enrichment in lipid metabolism terms involving 12 genes, 10 of which were downregulated only in dic (1;7) (Supplementary Tables 2-5). Among them, we found one group of lipid metabolism genes related to oxidative/ inflammatory response: the apolipoprotein APOM and the cholesterol esterifying enzyme LCAT that have been reported to decrease upon oxidative and/or inflammatory response [30,31]; the cytidine deaminase APOBEC2, found to be regulated by the inflammatory transforming growth factor-beta signaling [32] and the nuclear receptor NR1H2 that was involved in lipid homeostasis and inflammation [33]. A second group of genes is encoding for lipids related to cancer: LPL, lipoprotein lipase hypo-expression that was shown to predict evolution in chronic lymphocytic leukemia patients [34]; PLA2G7, a phospholipase which expression in the peripheral blood was predictive of survival in melanoma patients [35]; apolipoprotein APOC1 that was associated with poor prognosis in pancreas cancer patients; moreover, when inhibited, it induced apoptosis in pancreatic cancer cell lines [36].…”

Section: Dic(1;7) Has a Distinct Expression Signaturementioning

confidence: 99%

A distinct epigenetic program underlies the 1;7 translocation in myelodysplastic syndromes

et al. 2019

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The unbalanced translocation dic(1;7)(q10;p10) in myelodysplastic syndromes (MDS) is originated by centromeric juxtaposition resulting into 1q trisomy and 7q monosomy. More than half of cases arise after chemo/radio-therapy. To date, given the absence of genes within the centromeric regions, no specific molecular events have been identified in this cytogenetic subgroup. We performed the first comprehensive genetic and epigenetic analysis of MDS with dic(1;7)(q10;p10) compared to normal controls and therapy-related myeloid neoplasms (t-MNs). RNA-seq showed a unique downregulated signature in dic(1;7) cases, affecting more than 80% of differentially expressed genes. As revealed by pathway and gene ontology analyses, downregulation of ATP-binding cassette (ABC) transporters and lipid-related genes and upregulation of p53 signaling were the most relevant biological features of dic(1;7). Epigenetic supervised analysis revealed hypermethylation at intronic enhancers in the dicentric subgroup, in which low expression levels of enhancer putative target genes accounted for around 35% of the downregulated signature. Enrichment of Krüppel-like transcription factor binding sites emerged at enhancers. Furthermore, a specific hypermethylated pattern on 1q was found to underlie the hypoexpression of more than 50% of 1q-deregulated genes, despite trisomy. In summary, dic(1;7) in MDS establishes a specific transcriptional program driven by a unique epigenomic signature.

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Section: Dic(1;7) Has a Distinct Expression Signaturementioning

confidence: 99%

A distinct epigenetic program underlies the 1;7 translocation in myelodysplastic syndromes

et al. 2019

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“…In this second paradigm, we investigated the potential role of altered cell membrane fluidity on lipoprotein induced cellular changes studying RBC from LcatÀ/À and Apoa1À/À mice, which exhibit impaired high density lipoprotein (HDL) metabolic pathway and HDL cholesterol (HDL-C) homeostasis [42,43].…”

Section: Impact Of Lcat2/2 and Apoa12/2 On The Fluidity Of Mouse Rbcsmentioning

confidence: 99%

Fatty acid-related modulations of membrane fluidity in cells: detection and implications

Maulucci

Cohen

Daniel

et al. 2016

Free Radical Research

129

101

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Metabolic homeostasis of fatty acids is complex and well-regulated in all organisms. The biosynthesis of saturated fatty acids (SFA) in mammals provides substrates for b-oxidation and ATP production. Monounsaturated fatty acids (MUFA) are products of desaturases that introduce a methylene group in cis geometry in SFA. Polyunsaturated fatty acids (n-6 and n-3 PUFA) are products of elongation and desaturation of the essential linoleic acid and a-linolenic acid, respectively. The liver processes dietary fatty acids and exports them in lipoproteins for distribution and storage in peripheral tissues. The three types of fatty acids are integrated in membrane phospholipids and determine their biophysical properties and functions. This study was aimed at investigating effects of fatty acids on membrane biophysical properties under varying nutritional and pathological conditions, by integrating lipidomic analysis of membrane phospholipids with functional two-photon microscopy (fTPM) of cellular membranes. This approach was applied to two case studies: first, pancreatic beta-cells, to investigate hormetic and detrimental effects of lipids. Second, red blood cells extracted from a genetic mouse model defective in lipoproteins, to understand the role of lipids in hepatic diseases and metabolic syndrome and their effect on circulating cells.ARTICLE HISTORY

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“…Following plaque identification and isolation, adenoviruses were expanded in HEK293 cells (40) and then purified by double CsCl ultracentrifugation, followed by dialysis and titration of the recombinant adenoviruses, as described previously (39). of the anti-inflammatory capacity of HDL, where single fractions of endotoxin-free serum lipoproteins were fractionated by a different density gradient (1.063 g/ml over 1.019 g/ml over 1.0063 g/ml) and separation of 4 ml of pooled serum samples was performed under aseptic conditions, as described previously (41).…”

Section: Expansion and Purification Of Adgfp-apoc3mentioning

confidence: 99%

“…Mitochondria from BAT and WAT were isolated, as described previously (42). The protein concentration of each mitochondrial sample was determined using the DC TM protein assay kit (catalog number 500-0116; Bio-Rad) (41).…”

Section: Isolation Of Mitochondriamentioning

confidence: 99%

“…Esterified cholesterol was determined by subtracting free cholesterol from total cholesterol and multiplying the difference by 1.67 to correct for the fatty acid moiety, as proposed by Chapman et al (43). Triglyceride and phospholipid levels were also assessed spectrophotometrically in plasma samples and lipoprotein fractions by using the DiaSys Triglycerides FS kit (reference number 15710, Diagnostic Systems, GmbH) and the Lab Assay phospholipid determination kit (catalog number 296-63801, Wako Chemicals), respectively, according to manufacturers' instructions (41,44). Total protein in lipoprotein fractions was measured by the Lowry assay using the DC TM protein assay kit (catalog number 500-0116, Bio-Rad) (41).…”

Section: Determination Of Plasma and Lipoprotein Lipid Levelsmentioning

confidence: 99%

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Pleiotropic effects of apolipoprotein C3 on HDL functionality and adipose tissue metabolic activity

Zvintzou

Lhomme

Chasapi

et al. 2017

Journal of Lipid Research

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APOC3 is produced mainly by the liver and intestine and approximately half of plasma APOC3 associates with HDL. Though it was believed that APOC3 associates with HDL by simple binding to preexisting particles, recent data support that biogenesis of APOC3-containing HDL (APOC3-HDL) requires Abca1. Moreover, APOC3-HDL contributes to plasma triglyceride homeostasis by preventing APOC3 association with triglyceride-rich lipoproteins. Interestingly, APOC3-HDL also shows positive correlation with the morbidly obese phenotype. However, the roles of APOC3 in HDL functionality and adipose tissue metabolic activity remain unknown. Therefore, here we investigated the direct effects of APOC3 expression on HDL structure and function, as well as white adipose tissue (WAT) and brown adipose tissue (BAT) metabolic activity. C57BL/6 mice were infected with an adenovirus expressing human APOC3 or a recombinant attenuated control adenovirus expressing green fluorescent protein and blood and tissue samples were collected at 5 days postinfection. HDL was then analyzed for its apolipoprotein and lipid composition and particle functionality. Additionally, purified mitochondria from BAT and WAT were analyzed for uncoupling protein 1, cytochrome c (Cytc), and Cytc oxidase subunit 4 protein levels as an indirect measure of their metabolic activity. Serum metabolomic analysis was performed by NMR. Combined, our data show that APOC3 modulates HDL structure and function, while it selectively promotes BAT metabolic activation.

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Lack of LCAT reduces the LPS-neutralizing capacity of HDL and enhances LPS-induced inflammation in mice

Cited by 34 publications

References 40 publications

A distinct epigenetic program underlies the 1;7 translocation in myelodysplastic syndromes

A distinct epigenetic program underlies the 1;7 translocation in myelodysplastic syndromes

Fatty acid-related modulations of membrane fluidity in cells: detection and implications

Pleiotropic effects of apolipoprotein C3 on HDL functionality and adipose tissue metabolic activity

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