Raman spectroscopic analysis of thecis/trans isomer composition of edible vegetable oils

A new method is presented for determining thecis/trans isomer content of edible vegetable oils. The intensities of Raman lines near 1656 and 1670 cm⁻¹ are associated with thecis andtrans configuration, respectively. A precision of ca. 1% can be obtained in thecis/trans isomer analysis of binary mixtures of methyl esters and triglycerides of monoenes and dienes and of hydrogenated vegetable oils. The spectroscopic data also provide the iodine value of vegetable oils or isolated fractions with precision for a single determination of ca. 1%. Presented at the AOCS meeting, Houston, May 1971. W. Market. Nutr. Res. Div., ARS, USDA.     

Heat treatment of vegetable oils III. GC-MS characterization of cyclic fatty acid monomers in heated sunflower and linseed oils after total hydrogenation

Fractions of cyclic fatty acid monomers (CFAM) were isolated from linseed oil heated at 275°C for 12 hr under nitrogen, at 240°C for 10 hr under nitrogen and at 240°C for 10 hr under air. Cyclic fatty acid monomers fractions were also isolated from a sunflower oil heated at 275°C for 12 hr under nitrogen and at 200°C for 48 hr in a commercial fryer. The CFAM fractions were hydrogenated and their composition studied by gas liquid chromatography coupled with mass spectrometry (GC-MS). The CFAM in the fraction isolated from heated linseed oil samples were a mixture (1:1) ofcis andtrans cyclopentyl and cyclohexyl isomers, while the CFAM in the fractions isolated from heated sunflower oils were mostly cyclopentyl isomers. The major cyclopentyl isomers weretrans andcis methyl 7-(2′-hexylcyclopentyl) -heptanoate, methyl 9-(2′-butyl-cyclopentyl)-nonanoate and methyl 10-(2′-propylcyclo-pentyl)-decanoate. The major cyclohexyl isomers were thetrans andcis methyl 9-(2′-propylcyclohexyl)-nonanoate which represented about 50% of the CFAM isomers isolated from heated linseed oil samples. For part II in this series see Ref. 1.     

High performance liquid chromatography and glass capillary gas chromatography of geometric and positional isomers of long chain monounsaturated fatty acids

Positional and geometrical isomers of monounsaturated long chain fatty acids were analyzed by the combination of high performance liquid chromatography (HPLC) and glass capillary gas chromatography (GC). A preparative group separation ofcis andtrans isomers of the monounsaturated fatty acid methyl esters was achieved according to chain length by reversed-phase HPLC, and using a highly sensitive interference refractive index detector. After collection of the different fractions containingcis andtrans forms of the monounsaturated fatty acid methyl esters, the fractions were analyzed for their content of positional isomers using glass capillary GC with Silar-5 CP as stationary phase. The preparative step in the HPLC was also used analytically for the determination of the ratio between thecis andtrans monounsaturated fatty acids. A comparison was made between the results obtained with the HPLC technique and the results of a GLC technique with a packed OV-275 column. There was a good correlation between the 2 techniques with a tendency to highertrans values with the HPLC technique (4%). It was shown with reference substances that 18∶1ω6-cis to ω11-cis and 18∶1ω5-trans to ω12-trans, the most common monounsaturated fatty acid isomers in partially hydrogenated vegetable oils, could be almost quantitatively recovered in the HPLC step. Most of the individual positional isomers of monounsaturated fatty acids of varying chain length could be separated and determined in the glass capillary GC step with the exception of those isomers containing the double bond in a relatively high ω-position. The relative standard deviation of the technique as determined with reference substances was better than 4%. The described technique was applied to the analysis of the isomeric monounsaturated fatty acid content in partially hydrogenated vegetable and marine oils, and about 5 samples a day could be executed. Part of this work has been presented at the ISF/AOCS World Congress, New York (1980)JAOCS 58, (4), 1981, abstr. no. 184.     

Linolenic acid artifacts from the deodorization of oils

Gas liquid chromatography on polar open tubular columns of the methyl esters of fatty acids from vegetable oils shows that the linolenic acid in deodorized oils is accompanied by two major artifacts identified as cis-9,cis-12,trans-15 and trans-9,cis-12,cis-15 isomers. Physicochemical studies, isolation, and partial degradation steps showed two additional isomers with trans-9,cis-12,trans-15 and cis-9,trans-12,cis-15 structures. Gas liquid chromatography also showed that linoleic acid was accompanied by the trans-9,cis-12 isomer. These artifacts were not present in unrefined oils or bleached oils but could be induced by deodorization in the laboratory. Proportions of the two major artifacts in total 18:3ω3 are given for some vegetable oils from the retail market. Presented in part at the AOCS Spring Meeting, New Orleans.     

Determination ofcis andtrans-Octadecenoic acids in margarines by gas liquid chromatography-infrared spectrophotometry

A combined capillary gas liquid chromatography (GLC) and infrared spectrophotometry (IR) method is described for the determination ofcis andtrans-octadecenoic acids in margarines made from partially hydrogenated vegetable oils. The totaltrans-unsaturation of margarine fatty acid methyl esters determined by IR, with methyl elaidate as the external standard, was correlated to the capillary GLC weight percentages of the componenttrans fatty acid methyl esters by the mathematical formula: IRtrans=%18∶1t+0.84×%18.2t+1.74×%18∶2tt+ 0.84×%18∶3t where 0.84, 1.74 and 0.84 are the correction factors which relate the GLC weight percentages to the IRtrans-equivalents for mono-trans-octadecadienoic (18∶2t),trans, trans-octadecadienoic (18∶2tt) and mono-trans-octadecatrienoic (18∶3t) acids, respectively. This formula forms the basis for the determination of totaltrans-andcis-octadecenoic acids in partially hydrogenated vegetable oils. From the weight percentages of 18∶2t, 18∶2tt and 18∶3t determined by capillary GLC on a cyanosilicone liquid phase and the totaltrans-unsaturation by IR, the percentage of the totaltrans-octadecenoic acids (18∶1t) is calculated using the formula. The difference between the total octadecenoic acids (18∶1), determined by capillary GLC, and the 18∶1t gives the totalcis-octadecenoic acids. Presented in part at the 81st Annual Meeting of the American Oil Chemists' Society, Baltimore, Maryland, April 22–25, 1990.     

Occurrence of octadecenoic fatty acid isomers from hydrogenated fats in human tissue lipid classes

The level oftrans-18∶1 isomers in several isolated lipid classes of human liver, heart, red blood cells and plasma was determined. Phospholipids contained substantially fewertrans-18∶1 isomers than triglycerides. The double bond distribution of thecis andtrans octadecenoate fraction of triglycerides and phosphatidylcholines from human liver and heart was determined. Whereas the double bond distribution of the triglycerides correlated closely with the pattern found in dietary hydrogenated vegetable oils, the phosphatidylcholine fraction showed evidence of selective incorporation or metabolism of specifictrans positional isomers. In general, isomers with double bonds near the methyl terminus were present at levels higher than expected from their relative abundance in the diet. Refinements in methodology needed to analyze octadecenoate double bond configuration and location in human tissues are presented.     

Participation of thecis-12 ethylenic bond tocis-trans isomerization of thecis-9 andcis-15 ethylenic bonds in heated α-linolenic acid

To understand thecis-trans isomerization reaction of ethylenic bonds in heated octadecatrienoic acids (occurring during industrial deodorization of oils), we have prepared a mixture ofcis-9,cis-12,cis-15, andcis-9,cis-15 18:2 acids by partial hydrazine reduction ofcis-9,cis-12,cis-15 18:3 acid present in linseed oil. This mixture (as fatty acid methyl esters) was heated under vacuum at 270°C for 2.25 h. The two methylene-interrupted acids isomerize at a similar rate under such conditions, but the nonmethylene-interruptedcis-9,cis-15 18:2 acid remains unchanged. This means that the mechanism of isomerization does not involve a direct interaction between the two external ethylenic bonds as previously hypothesized. The centralcis-12 ethylenic bond is apparently necessary for the isomerization of the two externalcis-9 andcis-15 ethylenic bonds. However, this bond is itself rather protected against isomerization in the originalcis-9,cis-12,cis-15 18:3 acid which is mainly isomerized totrans-9,cis-12,trans-15,cis-9,cis-12,trans-15, andtrans-9,cis-12,cis-15 18:3 acids. Thecis-9,trans-12,cis-15 18:3 isomer is less than 10% of totaltrans isomers of α-linolenic acid. As a general rule, only one of the two double bonds in a methylene-interrupted diethylenic system can undergocis-trans isomerization when submitted to heat treatment, at least for temperatures equal to or less than 270°C.     

Characterization of γ-linolenic acid geometrical isomers in borage oil subjected to heat treatments (deodorization)

Heating of borage oil, either under vacuum as a model or during steam-vacuum deodorization, produces artifacts that are geometrical isomers of γ-linolenic acid (cis-6,cis-9,cis-12 18∶3 acid). In a first approach, we have studied the behavior of these fatty acids in the form of either methyl or isopropyl esters on two capillary columns (CP-Sil 88 and DB-Wax). From this study, it appears that the DB-Wax capillary column is the best suited analytical tool to study in some detail γ-linolenic acid geometrical isomers. In a second approach, the structure of these isomers was formally established by combining several analytical techniques: Argentation thin-layer chromatography, comparison of the equivalent chainlengths with those of isomers present in NO₂-isomerized borage oil on two different capillary columns, partial hydrazine reduction, oxidative ozonolysis, gas chromatography coupled with mass spectrometry and gas chromatography coupled with Fourier transform infrared spectroscopy. The two main isomers that accumulate upon heat treatments are thetrans-6,cis-9,cis-12 andcis-6,cis-9,trans-12 18∶3 acids with minor amounts ofcis-6,trans-9,cis-12 18∶3 acid. One di-trans isomer, supposed to be thetrans-6,cis-9,trans-12 18∶3 acid, is present in low although noticeable amounts in some of the heated oils. The content of these artificial fatty acids increases with increasing temperatures and duration of heating. The degree of isomerization (DI) of γ-linolenic acid is less than 1% when the oil is deodorized at 200°C for 2 h. Heating at 260°C for 5 h increases the DI up to 74%. Isomerization of γ-linolenic acid resembles that of α-linolenic (cis-9,cis-12,cis-15 18∶3) acid in several aspects: The same kinds and numbers of isomers are formed, and similar degrees of isomerization are reached when the octadecatrienoic acids are heated under identical conditions. It seems that the reactivity of a double-bondvis-à-vis cis-trans isomerization is linked to its relative position, central or external, and not to its absolute position (Δ6, 9, 12 or 15).     

Determination of trans fatty acids in hydrogenated vegetable oils by attenuated total reflection infrared spectroscopy: Two limited collaborative studies

An attenuated total reflection infrared spectroscopy procedure was collaboratively studied among two sets of five laboratories for quantitating the total trans fatty acid levels in neat (without solvent) hydrogenated vegetable oils, measured as triacylglycerols in one study, and as fatty acid methyl ester derivatives in the other. Unlike the fatty acid methyl esters, the triacylglycerols required no derivatization but had to be melted prior to measurement. To obtain a symmetric absorption band at 966 cm⁻¹ on a horizontal background, the single-beam spectrum of the trans-containing fat was "ratioed" against that of a refined oil or a reference material that contained only cis double bonds. A single-bounce horizontal attenuated total reflection cell that requires 50 μL of undiluted test samples was used for oils, melted fats, or their methyl esters. For fatty acid methyl esters, the reproducibility relative standard deviations were in the range of 0.9 to 18.46% for 39.08 to 3.41% trans, determined as methyl elaidate per total fatty acid methyl esters. For five pairs of triacylglycerol blind duplicates, the reproducibility and repeatability relative standard deviations were in the ranges of 1.62 to 18.97%, and 1.52 to 13.26%, respectively, for 39.12 to 1.95% trans, determined as trielaidin per total triacylglycerols. Six pairs of spiked triacylglycerol blind duplicates (quality assurance standards) exhibited high accuracy in the range of 0.53 to 40.69% trans and averaged a low bias of 1.3%. These statistical analysis results were compared to those collaboratively obtained by the recently adopted AOCS Cd14-95 and AOAC 994.34 Infrared Official Methods.     

Identification of noveltrans isomers of 20∶5n−3 in liver lipids of rats fed a heated oil

Trans polyunsaturated n−3 fatty acids are formed as a result of the heat treatment of vegetable oils. It was demonstrated previously that the 18∶3 Δ9cis, 12cis, 15trans containing acis Δ9 ethylenic bond was converted to a geometrical isomer of 20∶5n−3, the 20∶5 Δ5cis, 8cis, 11cis, 14cis, 17trans. In the present study, we have identified two new isomers of eicosapentaenoic acid, the Δ11 monotrans and the Δ11, 17 ditrans isomers in liver of rats fed a heated oil. These are formed as a result of the conversion of two of the main isomers of linolenic acid which are present in refined and frying oils, the 18∶3 Δ9trans, 12cis, 15cis and the 18∶3 Δ9trans, 12cis, 15trans.     

Chromatographic separation ofcis andtrans fatty esters by argentation with a macroreticular exchange resin

Methyl oleate and methyl elaidate, as well as other monoenecis andtrans isomers of fatty esters, can be separated quickly and conveniently by a preparative chromatographic procedure in which a silver-saturated ion-exchange resin is used. Separations are based on differences in stabilites of the silver-olefin complexes. Recoveries of better than 95% were made, and puretrans andcis monoene fractions were collected. This method can be used to separate saturates fromcis andtrans monoenes. Thecis,trans,cis,cis, andtrans,trans-9-12-octadecadienoates were separated. Whilecis,trans andtrans,trans dienes were cluted separately, thecis,cis diene isomer remained on the column. Presented at AOCS Meeting, in Minneapolis, 1963. A laboratory of the No. Utiliz. Res. and Dev. Div., ARS, USDA.     

Evidence for [1,5] sigmatropic rearrangements of CLA in heated oils

Linoleic acid was heated at 200°C under helium. Analysis of degradation products by GC on a long polar open tubular capillary column showed the presence of CLA isomers. The identified mono trans CLA isomers were cis-9, trans-11, trans-9, cis-11, trans-10, cis-12, cis-10, trans-12, trans-8, cis-10, and cis-11, trans-13 18:2 acids. Oils containing different levels of linoleic acid (peanut, sesame seed, and safflower seed oils) were also heat treated, resulting in similar CLA distributions. Elution order was confirmed using cis-9, trans-11 and trans-10, cis-12 acid methyl esters standards and their respective configuration isomers (trans-9, cis-11, cis-10, trans-12), obtained after mild selenium-catalyzed isomerization. These results indicated that two conjugated mono trans isomers of 18:2 acid, cis-8, trans-10 and trans-11, cis-13 18:2 were absent from the series, thus strongly suggesting that some constraints were preventing their formation. By heating pure methyl rumenate (cis-9, trans-11 18:2) under similar conditions, isomerization resulted principally in a nearly equimolar mixture of methyl rumenate and trans-8, cis-10 18:2. Similarly, the methyl ester of trans-10, cis-12 18:2 acid was partially transformed into cis-11, trans-13 18:2 acid. Respective geometrical isomers were also formed in trace amounts. A concerted pericyclic isomerization mechanism, a [1,5] sigmatropic rearrangement, is proposed that limits the conjugated system to isomerization from a cis-trans acid to a trans-cis acid, and vice versa. This mechanism is consistent with undetected cis-8, trans-10 and trans-11, cis-13 18:2 isomers in heated oils containing linoleic acid.     

The composition of hydrogenated fats by high-resolution13C nuclear magnetic resonance spectroscopy

The high-resolution¹³C nuclear magnetic resonance spectra of twelve hydrogenated fats have been examined. Each spectrum contains 50–100 signals and reveals much about the nature of the acyl chains of both double-bond position and configuration. The signals for the ω1, ω2 and ω3 carbon atoms give information on thecis andtrans isomers of the Δ15, Δ14, Δ13 and Δ12 18:1 esters, respectively. Allylic signals distinguish betweencis andtrans esters, and the proportion of totalcis to totaltrans isomers can be obtained from these. Olefinic signals are the most informative, and most of these have been assigned. This leads to a semi-quantitative estimate of the various 18:1 isomers present. Assignments are based mainly on information already in the literature, but some were confirmed after urea fractionation of the acids from a hydrogenated oil in whichcis andtrans monoene acids were separately concentrated.     

Analysis of the monoenoic fatty acid distribution in hydrogenated vegetable oils by silver-ion high-performance liquid chromatography

A silver-ion high-performance liquid chromatography column (hexane/acetonitrile as solvent, ultraviolet detection) was used to analyze the fatty acid distribution (as fatty acid methyl esters) of a representative sample of hydrogenated oil. Fractions containingcis- andtrans-18:1 isomers were readily separated. The positional fatty acid isomers were separated by rechromatographing these fractions. The elution order and percent compositions were compared with results obtained by gas chromatography. Of the Δ8 to Δ14trans-18:1 isomers, only the Δ8 and Δ9 pair could not be separated. The Δ8 and Δ9cis-18:1 pair also could not be separated, and the Δ10 isomer was poorly separated from this pair. Area percents were comparable to results obtained by gas chromatography.     

Rapid determination of the totaltrans content of neat hydrogenated oils by attenuated total reflection spectroscopy

A Fourier transform infrared spectroscopy procedure is described for quantitating the levels of totalrans triglycerides or their fatty acid methyl ester derivatives in neat fats and oils. It requires either warming or no preparation of the laboratory sample, and about 5 min for spectroscopic measurement, band area integration, and calculation of thetrans content from a linear regression equation. To eliminate the strongly sloping background of the 966-cm⁻¹ trans band, the single-beam spectrum of thetrans-containing fat is “ratioed” against that of an unhydrogenated oil or a reference material that contains onlycis double bonds. Thus, a symmetric absorption band on a horizontal background is obtained. The area under thetrans band can then be accurately integrated between the same limits, 990 and 945 cm⁻¹, for alltrans levels investigated. To speed up the analysis, an attenuated total reflection liquid cell was used, into which oils, melted fats or their methyl esters were poured without weighing or quantitative dilution with the toxic and volatile carbon disulfide solvent. Thetrans levels determined by attenuated total reflection were closer to those found by capillary gas chromatography when the hydrogenated fat was measured against the corresponding unhydrogenated oil than when it was measured against acis reference material. Small differences were found betweentrans levels in hydrogenated fat test samples and the corresponding methyl ester derivatives (9.3 and 2.2% at about 2 and 41%trans, respectively). The lower limits of identification and quantitation were 0.2 and 1%, respectively.     

The 9-hexadecenoic and 11-octadecenoic acid content of natural fats and oils

The monoenoic methyl esters from numerous fats and oils which contained appreciablecis-9-hexadecenoic acid (cis-9-16∶1) were isolated by liquid-solid chromatography on silver nitrate-silica gel. Analysis of the monoenes by packed and capillary column gas-liquid chromatography showed that significant amounts ofcis-11-octadecenoic acid (cis-11-18∶1) were present in all samples. The amount ofcis-11-18∶1 found in the monoenoic methyl esters increased proportionally to logarithmic increases in thecis-9-16∶1 level. Most analyses reported in the literature also show this proportionality. This mathematical relationship suggests that chain elongation ofcis-9-16∶1 tocis-11-18∶1 is a biosynthetic pathway operative in a wide variety of species.     

Chemical synthesis and spectroscopic characteristics of C18 1,2-disubstituted cyclopentyl fatty acid methyl esters

The chemical synthesis of methyl 9-(2′-n-butylcyclopentyl)nonanoate and methyl 10-(2′-n-propylcyclopentyl)-decanoate was performed using a Wittig reaction between 2-alkylcyclopentanones and the corresponding ω-carbomethoxyalkyl triphenylphosphonium bromides. The intermediate alkylcyclopentylidene alkanoate esters were isolated from the reaction mixture, characterized by spectrometric methods, and then catalytically hydrogenated to the desired cyclopentyl esters. Gas chromatographymass spectrometry (GC-MS) showed that the final products contained a mixture oftrans- andcis-ring isomers with small amounts of other cyclic by-products. The GC-retention features, the mass fragmentation pattern, and the spectroscopic characteristics of both the final and the unsaturated intermediate products are discussed.     

trans Fatty acid content of commercial margarine samples determined by gas liquid chromatography on OV- 275

Gas liquid chromatography (GLC) of margarine methyl esters on a 20 ft × 1/8 in. column containing 15% OV-275 on 100/120 mesh Chromosorb P AW-DMCS at 220 C provided practical separations oftrans octadecamonoenoates from the correspondingcis-isomers and oftrans, trans- andcis,trans- octa-decadienoates from the correspondingcis.cis-isomers.Trans content by GLC was in reasonable agreement (±1–2%) with totaltrans content by infrared analysis in six of seven commercial margarine samples.     

Preparation of malvalic and sterculic acid methyl esters from Bombax munguba and Sterculia foetida seed oils

A method has been developed for the preparation of highly pure malvalic (cis-8,9-methyleneheptadec-8-enoic) and sterculic (cis-9,10-methyleneoctadec-9-enoic) acid methyl esters starting from Bombax munguba and Sterculia foetida seed oils. The methyl esters of these oils were prepared by sodium methylate-catalyzed transmethylation followed by cooling (6°C) the hexane solution of crude methyl esters and separation of insoluble fatty acid methyl esters by centrifugation in the case of B. munguba and by column chromatography in the case of S. foetida. Subsequently, the saturated straight-chain fatty acid methyl esters were almost quantitatively removed by urea adduct formation. Finally, methyl malvalate and methyl sterculate were separated from the remaining unsaturated fatty acid methyl esters, in particular methyl oleate and methyl linoleate, by preparative high-performance liquid chromatography on C₁₈ reversed-phase using acetonitrile isocratically. Methyl malvalate and methyl sterculate were obtained with purities of 95–97 and 95–98%, respectively.     

Studies on the nuclear magnetic resonance spectra of olefinic protons of conjugated fatty acid methyl esters

The NMR spectra of olefinic protons in the four representative conjugated fatty acid methyl esters, methylcis-9,trans-11-octadecadienoate, methyltrans-9,trans-11-octadecadienoate, methyl α eleostearate, and methyl β eleostearate, were studied. The chemical shift of each olefinic proton in these compounds was determined by considering their intramolecular environment. Coupling constants were also obtained as the results of spectral analysis.