Free,esterified and glucosidic sterols in cocoa butter

Sterol lipids of cocoa butter (cocoa beansLome Tongo) were fractionated into free sterols, steryl esters (SE), steryl glucosides and acylated steryl glucosides (ASG). 4-Desmethyl, 4-methyl and 4,4′-dimethyl sterols or triterpene alcohols, which were isolated as free sterols or which resulted from hydrolysis, were determined by thin layer chromatography-flame ionization detection and identified by gas chromatography and combined gas chromatography-mass spectroscopy. Free sterols comprise the main sterol fraction in cocoa butter. Esterified sterols amount to 11.5% of total sterols and glucosidic sterols to 16.3%. Fatty acids and D-glucose from hydrolysis of esters and glucosides were analyzed. The fatty acids of SE and ASG are richer in unsaturated fatty acids than cocoa butter total fatty acids.     

Lipid changes during life cycle of marine copepod,Euchaeta japonica marukawa

All stages from egg to adult of the North Pacific copepod,Euchaeta japonica contained wax esters in their lipid stores, while triglycerides were important only in the eggs, early naupliar stages, and adults. The large lipid reserves of the eggs were wax esters and triglycerides (58% and 19% of the lipid, respectively), both of which were used rapidly during the early stages of development. Wax esters continued to decrease after triglycerides had been utilized completely for energy. The slow metabolism of lipid during starvation indicated that lipid stores in adult females may be conserved for egg production. The dominant alcohols of the wax esters of all stages were tetradecanol (24–42% of the total) and hexadecanol (25–65%). Only minor amounts of polyunsaturated alcohols were observed. There was, however, a high proportion of polyunsaturation in the wax ester fatty acids, even though octadecenoic was generally predominant (16–46% of the total wax ester fatty acids). The polyunsaturation of the wax esters fatty acids and the presence of 21∶6 hydrocarbon suggest phytoplankton in the diet of adults and in the younger stages. Cholesterol was the main sterol, but there were minor amounts of desmosterol (1–12% of the total sterols) present. The latter sterol has not been found previously in copepods, although reported from Cirripedia and Decapoda.     

Composition of total lipids in rapeseed

Total lipids in medium and low erucic acid cul-tivars of rapeseed(Brassica napus var. Sinus and Janpol, resp.) were fractionated into polar and non-polar constituents. Triglycerides, diglycerides, mono-glycerides, free fatty acids, sterol esters, sterols, phos-pholipids and glycolipids were quantitated and their fatty acid compositions determined. Triglycerides and phospholipids constituted 92 and 3.4%, resp., of the total lipid from each cultivar. Triglycerides were lower in saturated fatty acids but higher in monoun-saturated acids and linolenic acid than other lipid fractions. Phospholipids and glycolipids were higher in linoleic acid content than other lipid classes. Generally, the reduction in long chain, monoenoic, fatty acids was associated with a corresponding increase in oleic acid in most low erucic acid frac-tions.     

Lipid,sterol and fatty acid composition of antarctic krill (Euphausia superba Dana)

The lipid classes, fatty acids of total and individual lipids and sterols of Antarctic krill (Euphausia superba Dana) from two areas of the Antarctic Ocean were analyzed by thin layer chromatography (TLC), gas liquid chromatography (GLC) and gas liquid chromatography/mass spectrometry (GLC/MS). Basic differences in the lipid composition of krill from the Scotia Sea (caught in Dec. 1977) and krill from the Gerlache Strait (caught in Mar. 1981) were not observed. The main lipid classes found were: phosphatidylcholine (PC) (33–36%), phosphatidylethanolamine (PE) (5–6%), triacylglycerol (TG) (33–40%), free fatty acids (FFA) (8–16%) and sterols (1.4–1.7%). Wax esters and sterol esters were present only in traces. More than 50 fatty acids could be identified using GLC/MS, the major ones being 14∶0, 16∶0, 16∶1(n−7), 18∶1(n−9), 18∶1(n−7), 20∶5(n−3) and 22∶6(n−3). Phytanic acid was found in a concentration of 3% of total fatty acids. Short, medium-chain and hydroxy fatty acids (C≤10) were not detectable. The sterol fraction consisted of cholesterol, desmosterol and 22-dehydrocholesterol.     

The content and composition of sterols and sterol esters in low erucic acid rapeseed (Brassica napus)

The low temperature crystallization technique for the enrichment of “minor” components, such as sterols and sterol esters, from vegetable oils was applied to low erucic acid rapeseed oils. The recovery of free sterols and sterol esters was estimated by use of¹⁴C-cholesterol and¹⁴C-cholesterol oleate. 80% of the free sterols and 45% of the sterol esters were recovered in the liquid fraction, while in two studies total recoveries were 95% and 99%, respectively. This technique showed some selectivity toward the sterol bound fatty acids when compared to direct preparative thin layer chromatography (TLC) of the crude oil. Gas liquid chromatography (GLC) analysis of the free and esterified sterols as TMS-derivatives showed very little selectivity in the enrichment procedure. The fatty acid patterns of the sterol esters demonstrated, however, a preference in the liquid fraction for those sterol esters which have a high linoleic and linolenic acid content. The content of free sterols was 0.3–0.4% and that of sterol esters 0.7–1.2% of the rapeseed oils in both winter and summer types of low erucic acid rapeseed (Brassica napus) when the lipid classes were isolated by direct preparative TLC of the oils. The free sterols in the seven cultivars or breeding lines analyzed were composed of 44–55% sitosterol, 27–36% campesterol, 17–21% brassicasterol, and a trace of cholesterol. The esterified sterols were 47–57% sitosterol, 36–44% campesterol, 6–9% brassicasterol, and traces of cholesterol and Δ5-avenasterol. The fatty acid patterns of these esters were characterized by ca. 30% oleic acid and ca. 50% linoleic acid, whereas these acids constitute 60% and 20%, respectively, of the total fatty acids in the oil. Little or no variation in sterol and sterol ester patterns with locality within Sweden was observed for the one cultivar of summer rapeseed investigated by the low temperature crystallization technique.     

Free sterols,steryl esters,and lipid phosphorus in needles of scot's pine (Pinus sylvestris L.)

Free sterols, steryl esters, and lipid phosphorus were measured in new (current year) needles of Scot's pine during an annual cycle, and also in one-, two-, and three-year-old needles collected shortly after bud break. Sterols were identified and quantified by capillary gas chromatography and gas chromatography/mass spectrometry. Steryl esters were hydrolyzed enzymatically. Newly emerged needles contained highest amounts of free sterols and lipid phosphorus, probably reflecting increased membrane and organelle production, but low levels of steryl esters. Mature needles contained approximately equal amounts of free and esterified sterols. The molar phospholipid/free sterol ratio was 3∶1 at all the time periods studied. A dramatic increase of steryl esters was observed in the one-, two-, and three-year-old needles at times when new needles emerged. The individual free and esterified sterols were sitosterol, campesterol (presumably together with its C-24 epimer), and cholesterol, at approximately 88, 10, and 2%, respectively. Isofucosterol, an intermediate in sitosterol biosynthesis, was present almost exclusively in newly emerged needles. Esterified sterols contained only trace amounts of isofucosterol. Shifts in favor of cholesterol and 24ζ-methyl cholesterol occurred in the steryl esters during needle differentiation, and saturation grade of esterified fatty acids decreased. In mature needles, the composition of free sterols and steryl esters remained constant throughout the year.     

The effect of lyophilization on the solvent extraction of lipid classes,fatty acids and sterols from the oysterCrassostrea gigas

The lipid class compositions of adult Pacific oysters [Crassostrea gigas (Thunberg)] were examined using latroscan thin-layer chromatography/flame-ionization detection (TLC/FID), and fatty acid compositions determined by capillary gas chromatography and gas chromatography/mass spectrometry (GC/MS). The fatty acid methyl esters were separated using argentation TLC and also analyzed as their 4,4-dimethyloxazoline derivatives using GC/MS. Major esterified fatty acids inC. gigas were 16∶0, 20∶5n−3, and 22∶6n−3. C₂₀ and C₂₂ nonmethylene interrupted (NMI) fatty acids comprised 4.5 to 5.9% of the total fatty acids. The NMI trienoic fatty acid 22∶3(7,13,16) was also identified. Very little difference was found in the proportions of the various lipid classes, fatty acids or sterols between samples of adult oysters of two different sizes. However, significant differences in some of the lipid components were evident according to the method of sample preparation used prior to lipid extraction with solvents. Lyophilization (freeze drying) of samples led to a significant reduction in the amounts of triacylglycerols (TG) extracted by solvents in two separate experiments (7.0 and 52.5% extracted). Extracts from lyophilized samples had less 16∶0, C₁₈ unsaturated fatty acids, and 24-ethylcholest-5-en-3β-ol, while C₂₀ and C₂₂ unsaturated fatty acids comprised a higher proportion of the total fatty acids. There was no significant change in the amounts of polar lipids, total sterols, free fatty acids or hydrocarbons observed in extracts from lyophilized samples relative to extracts from nonlyophilized samples. Addition of water to the freezedried samples prior to lipid extraction greatly improved lipid yields and resulted in most of the TG being extracted.     

The fatty acids of degras

Degras contains a complex mixture of lipids comprised of branched and normal chain fatty acids, hydroxy acids, sterols, sterol esters and long chain wax esters. There are no glycerides in degras. This paper is a report on the composition of the branched and normal chain fatty acids. Preparative techniques of thin-layer chromatography were used to isolate the fatty acids from the other lipid classes. Gas chromatography was used on three different stationary phase separations of the fatty acid methyl esters. Identifications of the composition were based on a combination of techniques and known standards. Authorized for publication on April 20, 1965, as paper No. 3003 in the journal series of The Pennsylvania Agricultural Experiment Station.     

Skin surface lipids of the dog

The skin surface lipid of the dog has been reported to contain a high proportion of diol diesters having a lower mobility on thin layer chromatography than diesters from other species in spite of containing similar fatty acid and diol components. In the present study, dog skin surface lipid was separated by preparative thin layer chromatography into sterol esters (42%), wax diesters (32%), free sterols (9%), polar lipids (7%), and unidentified components (10%). The diesters contained 1,2-diols, each esterified with one long chain fatty acid and one isovaleric acid moiety. The diols were principally branched chain C₂₁ and C₂₂ compounds while the long chain fatty acids esterified with them were mainly C₂₀ and C₂₁ branched compounds. The fatty acids from the sterol esters were mostly saturated, branched chain C₁₉ to C₂₃, together with 7% of straight chain monoenoic acids, principally C₂₁ and C₂₂. There were only trace amounts of free sterols other than cholesterol, while the esterified sterols contained 96% cholesterol and 4% lathosterol.     

Freie und gebundene Sterine in rohen und raffinierten Palmölen,Teil II: Sterinhaltige Lipoproteine

Free and Bound Sterols in Raw and Refined Palm Oils, Part II: Sterol Containing Lipoproteins Twelve lipid fractions were isolated from raw palm oil which contain beside sterols, fatty acids and pigments also low amounts of phospholipids and proteins. The very stable complexes can only be decomposed by acid hydrolysis. The composition of sterols and fatty acids in the hydrolysate and the phosphor and nitrogen content in the purified lipid fractions were determined. According to composition and chemical behaviour of these lipid complexes they are sterol containing lipoproteins with strong lipophilic character. In some of these fractions the extremely high cholesterol content is striking which is partly more than 50% of the total sterols. The release of sterols from these complexes during refining might be the reason for the high cholesterol content in some refined palm oils.     

The content and composition of sterols and sterol esters in sunflower and poppy seed oils

The composition and proportion of free sterols and sterol esters in crude sunflower and poppy seed oils were determined, using preparative thin layer chromatography followed by gas chromatography with cholesterol as an internal standard. Free sterols and sterol esters were also isolated in a liquid fraction obtained by low temperature crystallization (−80 C) of the oils and enriched with minor lipid classes. This enrichment procedure provided a liquid fraction suitable for studies of minor components in the oils. However, selectivity towards sterol esters was observed since sterols esterified to very long chain fatty acids (C₂₀–C₂₄) were preferentially retained in the precipitate. The proportions of free and esterified sterols were found to be 0.34 and 0.28%, respectively, in the sunflower oil, whereas the corresponding figures for poppy seed oil were 0.33% and 0.05%. Sunflower oil was characterized by a relatively high percentage of Δ7-sterols, preferentially obtained in the esterified fraction, and by very long chain saturated fatty acids of sterol esters. The sterols in poppy seed oil were composed almost entirely of campesterol, stigmasterol, sitosterol and Δ5-avenasterol, although their percentage distributions were remarkably different in the free and esterified fraction.     

Thin layer chromatographic procedure for class separation of plant neutral lipids

A thin layer chromatographic method has been developed for the class separation of plant neutral lipids. Utilizing a two-step development in one dimension, lipid mixtures are separated into hydrocarbon waxes, steryl esters, methyl esters, triglycerides, fatty acids, diglycerides, sterols, and monoglycerides. The method may be employed for either qualitative or preparative purposes.     

Non-Polar Lipid Components of Human Cerumen

Human cerumen was separated by column chromatography into the following groups of compounds: hydrocarbons, squalene, wax esters and cholesterol esters, triacylglycerols, free fatty acids, free fatty alcohols, monoacylglycerols, free cholesterol, free sterols, and free hydroxy acids. The groups of compounds obtained were examined in detail by gas chromatography and gas chromatography–mass spectrometry. In total, about one thousand compounds have been identified.     

Lipids of the earthwormLumbricus terrestris

The lipid composition of the earthwormLumbricus terrestris has been reexamined under conditions intended to avoid enzymatic and chemical alterations during storage, extraction, and fractionation procedures. The simple lipids included aliphatic hydrocarbons, steryl esters, glycerides, and at least nine different sterols, all though to be derived from the diet. Free fatty acids, previously considered to be major components of worm lipids, comprised only 0.3% of the total lipid weight. Phospholipids included (in order of relative abundance) phosphatidylcholine, phosphatidylethanolamine, phosphatidylserine, and phosphatidylinositol, as well as sphingomyelin. Glycolipids included cerebrosides and sulfatides containing both glucose and galactose, and gangliosides containing glucosamine and sialic acid. The fatty acid compositions of these lipid classes appeared to be a mixture of what are considered typical plant, bacterial, and animal acids. Several fatty acids found in the worms, includingcis-vaccenic and eicosapentaenoic acids, were essentially absent from the dietary components, and it is concluded that these acids were synthesized in the worms. The earthworm derives much of its lipid adventitiously, but exerts at least some control over its tissue lipid composition.     

Phytosterol Ester Constituents Affect Micellar Cholesterol Solubility in Model Bile

Plant sterols and stanols (phytosterols) and their esters are nutraceuticals that lower LDL cholesterol, but the mechanisms of action are not fully understood. We hypothesized that intact esters and simulated hydrolysis products of esters (phytosterols and fatty acids in equal ratios) would differentially affect the solubility of cholesterol in model bile mixed micelles in vitro. Sodium salts of glycine- and taurine-conjugated bile acids were sonicated with phosphatidylcholine and either sterol esters or combinations of sterols and fatty acids to determine the amount of cholesterol solubilized into micelles. Intact sterol esters did not solubilize into micelles, nor did they alter cholesterol solubility. However, free sterols and fatty acids altered cholesterol solubility independently (no interaction effect). Equal contents of cholesterol and either campesterol, stigmasterol, sitosterol, or stigmastanol (sitostanol) decreased cholesterol solubility in micelles by approximately 50% compared to no phytosterol present, with stigmasterol performing slightly better than sitosterol. Phytosterols competed with cholesterol in a dose-dependent manner, demonstrating a 1:1 M substitution of phytosterol for cholesterol in micelle preparations. Unsaturated fatty acids increased the micelle solubility of sterols as compared with saturated or no fatty acids. No differences were detected in the size of the model micelles. Together, these data indicate that stigmasterol combined with saturated fatty acids may be more effective at lowering cholesterol micelle solubility in vivo.     

Variations in Fatty Acids,Phospholipids and Sterols During the Seed Development of a High Oleic Sunflower Variety

The changes in the content and composition of total fatty acids, phospholipids and sterol esters, and their fatty acids, and of free sterols and tocopherols in developing seeds of a selection of high oleic acid sunflower varieties grown in Bulgaria were examined over a period of 15th to 90th day after flowering by means of various chromatographic methods. Under the climatic and geographical conditions typical for the South-East Balkans phospholipid, sterol-, sterol ester- and tocopherol- species are formed practically completely in the first 15 days after flowering. Until the 90th day, only quantitative changes were detected to give a product with 65% oil content, 1% phospholipids, 0.3% total sterols and 0.09% tocopherols. Oleic acid is the main component in all acyl derivatives, reaching 85% of the total fatty acids while palmitic and stearic acid content is about 4% each. The product is a good quality HOSO with beneficial content of FA and good prospects as a salad and cooking oil.     

Chromatographic characterization of internal polar lipids from wool

Wool internal polar lipids were isolated and separated into different fractions based on polarity. Qualitative and quantitative analyses of the different fractions were performed by thin-layer chromatography and thin-layer chromatography coupled to flame-ionization detection, respectively. Cholesterol esters, free fatty acids, sterols, ceramides, glycosylceramides, and cholesterol sulfate were the main components, with ceramides being in the highest proportion. The fatty acid composition of ceramides and glycosylceramides was determined by gas chromatography/mass spectrometry. As for other keratinized tissues, long-chain fatty acids predominated in comparison to either free fatty acids or phospholipid-linked fatty acids; in both cases, stearic and lignoceric acids were the most abundant fatty acids, and a low amount of 18-methyleicosanoic acid was found. This work opens new avenues in the study of lipid rearrangement in more complex and realistic vesicle structures than conventional liposomes.     

Column types for the chromatographic analysis of oleochemicals

Chromatography has developed into one of the principle methods of analysis of oleochemicals. Gas chromatography has been used extensively for the analysis of long-chain fatty acids as well as for the analysis of triglycerides and plant sterols. In recent years, high pressure liquid chromatography (HPLC) has been used for the analysis of triglycerides as well as for other related materials. Specialized gas chromatography columns have been developed for the separation of long-chain fatty acids such as the methyl esters. These columns have generally used high polarity stationary phases which separate fatty acids by degree of unsaturation. A specialized use of these high polarity stationary phases is separation ofcis-trans isomers as well ascis-cis andtrans-trans isomers. In this paper, packed and capillary columns are compared for the separation of thecis-trans isomers of fatty acid methyl esters prepared from a hydrogenated vegetable oil. For HPLC separations, the presence of a double bond is approximately equivalent chromatographically to shortening the alkyl chain by two carbons. The long-chain polyenic acids or ethyl esters thus elute near but are resolved from the short-chain saturated fatty acids or esters. HPLC is the method of choice for relatively complex, high molecular weight, or labile esters, such as those of retinyl or cholesterol. Glyceryl esters are particularly well resolved by HPLC in terms of both total chain length and degree of unsaturation. This technique is also useful for lipid class separations and for the analysis of modified fatty acid products, such as prostaglandins and related materials. In general, these analyses are conducted with octadecyl bonded phase column packings.     

Fatty acid and sterol composition of ungerminated spores of the vesicular-arbuscular mycorrhizal fungus,Acaulospora laevis

The fatty acids and sterols of ungerminated chlamydospores of the vesicular-arbuscular (VA) endophyteAcaulospora laevis were examined by gas chromatography and mass spectrometry. The total lipid content of the spores was 45.5% of the spore dry weight. Predominant fatty acids were palmitoleic (52.5%), palmitic (25.5%) and oleic (7.4%). Minor fatty acids consisted of a range of (n−3) and (n−6) polyunsaturated acids. The occurrence of (n−3) polyunsaturated fatty acids is rare in fungi of the order Mucorales. Three sterols were identified as 24-ethylcholesterol (79.9%), cholesterol (11.0%) and 24-methylcholesterol (9.2%). No ergosterol was detected. Lipids of the chlamydospores ofA. laevis are compared with those ofGlomus caledonius.     

Study of free and bound lipids ofBrassica campestris,var yellow sarson

Mature seeds ofBrassica campestris var. yellow sarson were extracted with hexane to yield free lipid. The residue then was extracted with chloroform-methanol to release bound lipid. Free and bound lipids were separated into polar and nonpolar fractions chromatographically. The nonpolar fraction of both free and bound lipid consisted mainly of triglycerides with small amounts of steryl esters, free sterols, mono- and di-glycerides, and free fatty acids. The principal components of polar bound lipid were phosphatidyl choline, phosphatidyl ethanolamine, phosphatidyl inositol, and steryl glycoside. In the free polar lipid, there was more phosphatidyl inositol and less phosphatidyl choline and phosphatidyl ethanolamine. Erucic acid content was much greater in the nonpolar fractions and in the polar free lipid than in the polar bound lipid.