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Page 1: International Journal of Food and Nutritional Science...For microwave drying, mango kernel powder was kept in petri plates arranged at equal distances in the microwave tray (Model

International Journal of Food and Nutritional Science

Int J Food Nutr Sci | Volume 3: Issue 1

Copyrights: © 2016 Arora, A. This is an Open access article distributed under the terms of Creative Commons At-tribution 4.0 International License.

Research Article

Jhumur Banerjee1, Antonio F. Patti2, Douglas MacFarlane2, R. Vijayaraghavan2, Ramkrishna Singh1, Amit Arora1,3*

Abstract Inthisstudy,effectofdryingmethodandtimetemperatureregimeofextractiononqualityofmangokernellipidwasevaluated.Hotairdryingrequireddryingofseedsforlongintervalsandexposuretohighertemperature,whereasmicrowavedryingwasfoundtobequickduetoheatinginducedatthemolecularlevel.Thedryingtimeunderoptimizedconditionsformicrowavewasreducedby34foldswhencomparedwithhotairdrying.Parametersincludingdryingtemperature,extractiontime,lipidyieldandfat-tyacidprofilewereevaluated.Thestudyshowsthatmodificationofextractionmethodfor lower temperatureand lesser timedoesnotalter thequalityandquantityof lipidsfrommangokernel(10.8%).Structuralchangesinducedduetodryingwerestudiedusingscanningelectronmicroscopy.Statisticalanalysisshowedthatdryingconditionsandex-tractionconditionsaffectedthelipidyield.Thefurthercomparisonbetweentwomethodswasdoneintermsoffattyacidprofilesandoxidativestability.Thestabilityoflipidwasestimatedbymeasuringtheratiooflinoleicacidtopalmiticacidforallextractioncon-ditions.TheratioofC18:2/C16wassimilarformicrowaveirradiationwhencomparedtohotairdriedsamples(1.0-1.2).Itwasconcludedthatmildmicrowavepowerlevel(180W)helpsinquickdryingofkernels.Thestructurewasfoundtobeintactwithmini-maldamagetostarchgranules.Lowermicrowavepowerlevelhelpedinretentionofthelipidyieldandqualitywhilehighermicrowavepower levels significantlyaffected theunsaturated fatty acids.

*Corresponding author: AmitArora, Indian Institute ofTechnology, Powai,Maharashtra, India,Tel: +91(22)-2576-7293;E-mail:[email protected]

Received Date: February 13, 2016Accepted Date: May 11, 2016Published Date: May 16, 2016

Keywords:Mangokernel;Microwave;Fattyacids;Scanningelectronmicroscopy

Introduction

Worldwideproductionofmangopulphasreachedmorethan1.5milliontonneswithanannualproductionoffruitcrossing43milliontonnes.Asiaaccountsfornearly84%oftotalpulpproductioninwhichIndiaisthelargestproducer[1].Nearly18.4milliontonnesofMangofruitsproductionwasrecordedin2014[2].Industriesprocessthemangofruitsforpulpproductionandgenerateahugequantityofwastewhichvariesfrom25-40%.Compostingandbiogasformationismainlyfollowedinlargeindustries,whileinsmallscaleindustries;thewasteisdisposedatafarsite.Thecurrentdisposalmechanismlacksvalueadditionofwasteandmanyimportantnutrientssuchasbioactivecompoundsarelost.Thewastealsobeingrichinmoistureleadstoenvironmentalpollution.Limitedlandfillingareaespeciallyindevelopingcountriesposedisposalchallenges. AsshowninFigure1,themangoprocessingwastemainlyconsistsofpeelsandseeds.Mangopeelsproximatecomposition

Effect of Drying Methods and Extraction Time-Temperature Regime on Mango Kernel Lipids

1IITB-MonashResearchAcademy,IITBombay,Mumbai,Maharashtra,India,4000762SchoolofChemistry,FacultyofScience,MonashUniversity,Claytoncampus,VIC,Australia3IndianInstituteofTechnology,Powai,Maharashtra,India

DOI: 10.15436/2377-0619.16.048

Citation: Arora, A., et al. Effectof Drying Methods and ExtractionTime-Temperature Regime on MangoKernelLipids. (2016) IntJFoodNutrSci3(1):229-338.

Arora, A., et al. 229

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showsthepresenceofasignificantamountofpectin,phenolicsandcarotenoidslikebioactive[3,4]. They play an important role as health-promotingadditivesinfoodindustry.Thespentpeelfrompectinextractionmayalsobeusedforutilisationofcellulosewhichisaround35%.Mangokernelsarefoundtoberichinstarch(50-60%),lipids(8-14%)andprotein(6-10%).Afewreportsonchar-acterizationofproteinshowedthatitcanbeagoodsourceforessentialaminoacids[5].Researchershavealsoshowngreatinterestinmangokernellipidsduetopeculiarfattyacidprofile(Saturatedfattyacid48-55%;unsaturatedfattyacid45-52%).Mangokernellipids have been used as a valuable substitute for cocoa butter in food items[6].Thecocoabutterconsistsofsaturated(60-65%)andunsaturatedfattyacids(35-40%).Thefattyacidsfrommangokernelswerealsousedasalipidbaseincosmeticse.g.lipsticksandemollients,inpreparationofbiosurfactantsetc.Thetendencyofkernellipidstostaypartlysolidatroomtemperaturemakesitusefultobeusedinfoodandcosmeticproductsespeciallyfordevelopingcountries.Thelipidcanalsobeblendedwithotheroilswhichrequiresuchapplicationsandtheratiocanbetunedaspertheproductdesirability.

Figure 1:Massbalanceformangoprocessing.

Extractionof lipidsfrommangokernel iscarriedoutbyusingvariousphysical,chemicaland/orcombinationof theseprocesses.Coldpressormechanicalexpellerisacommonlyusedindustrialmethodwherelossoflipidsissignificant[7,8]. Another methodforoilextractionisSoxhletextractionorhotsolventpercolationmethod.Theyieldobtainedinthismethodishighbutitsuffersdisadvantageoflargeamountofsolventusage.Hexaneismainlyusedassolventwhichistoxicinnatureandreportedtobeenvironmentallyhazardous.Thelargesolventusagealsoincurshighprocesscost.Alsowithnonpolarsolvents,dryingofmaterialbecomesanecessarystepbeforelipidsextraction.Theyieldofmangokernellipidsusinghotairdryingfollowedbyconventionalextractionvariesfrom7-9%forIndianvarieties[7-9].Otherrecentlydevelopedmethodsincludesupercriticalfluidextractionusingcarbondioxideinwhichyieldwasfoundtovaryfrom6.5to13.5%[10]. Dryingisoneofthemostimportantunitoperationinvolvedbeforeoilextractionastheyieldoftheextractedoilisdepen-dent on the moisture content of the material[11].Dryingisthemostenergyintensiveoperation.Commonlyusedmethodsfordryingaresundrying,solardrying,hotairdrying,vacuumdrying,freezedryingorcombinationofthesemethods(Sonwai,Kaphueakngam&Flood2014).Hotairdryingandfreezedryingareenergyintensiveprocesses[12].The product attributes in case of freeze dried sam-plesaresuperiorascomparedtoanyotherdryingmethod.Sundryingrequireslongintervalsofsunlightexposure.Thelimitationsassociatedwithsundryingareinconsistentavailabilityofsunlight,longhours,weatherconditionsanddamagetosamplesduetoenvironmentalfluctuations.Freezedryingisanenergyintensivenon-disruptivetechniquebutisnotwidelyapplicableduetohighercost.Hotairdryingiscommonlyfollowedinfoodprocessingindustriesowingtoitssimplicity,developmentoveryearsandprecisecontrolofparametersascomparedtoabovetwotechniques.Thetemperaturecanbevariedoveralargerangeandthus,qualitativeparameterscanbewellstudiedundercontrolledconditions. Microwavedryingisanoveltechniquewhichacceleratestheremovalofmoistureduetovibrationofwatermoleculesandvolumetricheating.Thetechniquewasreviewedforitsenergyefficiencyandquickerdryingascomparedtoothermethods[13-15].Microwaveshavebeenusedfordryingoffruitsandvegetableslikecarrot,spinachleavesandmushroom.Thequalityattributeswerefoundtobeacceptabletothatofcommercialproducts[16,17].Previousstudiesconcerningextractionofmangokerneloilhavefocussedonapplicationofhotairdryingonyieldofoil,phenolicandantioxidantcapacity[18].However,effectofdryingmethodsonstructuralmorphologyinrelationtooilextractionhasnotbeenreported.Also,itwouldbeimportanttounderstandhowvariousex-tractiontime-temperaturescombinationsforagivendryingconditionbringchangesintheoilextractabilityandoilquality.Aquickandeffectivedryingmethodpriortomangokernellipidextractionisthus,neededtodesignasustainableextractionprocess.Theextractionmethodmodificationmayaddfreshinsightintomangokernellipidextractionwhichmayfurtherbeusedasanessentialoil for various applications. Thepresentstudyaimsto(i)evaluateandcomparetheeffectofhotairdryingandmicrowavedryingonstructuralmor-phologyofmangokernelpowderand(ii)assesstheeffectofdifferentextractiontemperature-timecombinationsonlipidyields

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Materials and Methods

Raw material Themangoes(Totapurivariety)wereobtainedfromlocalmarket.Pulpwasremovedmanuallyandseedcoatswerewashedwithdistilledwatertoremoveresidualsugarsanddried.Seedcoatswereseparatedfromkernelusingacutterdesignedspecificallyforthispurpose.Thekernelsweregroundanddriedat105±2°Cforproximateanalysis[19].Driedpowderwassieved(≤500µ),packedinairtightcontainersandstoredat4°C.AllreagentswereofanalyticalgradeandprocuredfromMerck,India. Proximate analysis of kernels Themoisture,ash,lipid,proteinandcarbohydrateweredeterminedasperstandardAOACmethods[19].Sugarsweredeter-minedusingphenolic-sulphuricacidmethod.StarchwasquantifiedusingstarchassaykitfromMegazyme[20].

Hot air drying of kernel powder Theinitialmoisturecontentofthegroundkernelwasmeasured.Fordrying,aknownweightofgroundkernelswerekeptinpetriplatesinathinlayeranddriedatdifferenttemperatures.Eachreadingwasmeasuredintriplicate.Hotairdryingat1.0m/sairvelocitywasdoneforatemperaturerangeof40°C,60°C,80°Cand105°Cfordifferenttimeintervals.Themoisturecontentwasdeterminedusingmoistureanalyser(CitizenMB200,India). Formicrowavedrying,mangokernelpowderwaskeptinpetriplatesarrangedatequaldistancesinthemicrowavetray(ModelLGMG607APR,output900W).Kernelswereexposedtofourpowerlevels,i.e.20%(180W),40%(360W),60%(540W)and80%(720W)tillconstantweightwasachieved.MicrowavewassetuptostayONforaminuteandturnOFFfor30secandcyclecontinuedinthisfashionuntilexperimentswerecompleted.ThirtysecondsOFFtimewasmaintainedaftereveryminutetoavoidsampleburningduetooverheating.

Structural and morphological study Scanningelectronmicroscopywasconductedoncontrolandtreatedsamples(FEIQuanta200,Oregon,USA).Topreparethesample,driedpowderswereadheredtoadoublesidedadhesivetape.Platinumcoatingat20kVwasdonefor300spriortovi-sualisationofimages.Themicrographswerestudiedforpresenceofgranulesandstructuraldisruptionduringdrying.

Lipid extraction LipidextractionwascarriedoutusingSoxhletextractionmethod(Dhara,Bhattacharya&Ghosh2010).Tengramsofdriedkernelpowderwasplacedinathimbleandhexanewasusedasanextractionsolvent.Topreventthelipidfromdegradation,40°Cand60°Cwasusedasextractiontemperatureforatimeintervalof2hrsand4hrs.Nosignificantdifferenceinyieldwasfoundforlongerextractionperiods(8-24hrs)duringinitialexperiments,thus,temperatureandtimedurationwaskeptlowtoavoiddegrada-tionoffattyacids.Aftersolventremoval,thelipidwaskeptat40°Cfor24hourstoremovetracesofhexane.Theobtainedlipidwasthenstoredat4°Cinambercolouredcontaineruntilfurtherusage.Theyieldwascalculatedondrybasis.

Fatty acid profile and qualitative tests Thefattyacidprofilewasdeterminedtocompareanychangesinfattyacidcompositionduetodifferentdryingmethods.Thefattyacidcompositionwasdeterminedusinggaschromatographyequippedwithaflameionizationdetector(PerkinElmer,AutosystemXL).Forflameionizationdetector,columnusedwasPE-FFAP,carriergasnitrogen,Injectiontemperatureanddetectortemperaturewaskeptat250°C.Thequalitativeparameterssuchasperoxidevalue(PV),iodinevalue(IV),saponificationvalue(SV)andacidvalue(AV)weredeterminedasperthestandardprotocolsofFSSAI(FSSAI2012).

Statistical analysis ThedifferencebetweenvarioussetofresultswastestedusingonewayANOVAwithDunnett’spost-test(Minitab;version16).Theresultswereexpressedasmean±standarderror.Thesignificanceofdatawasrepresentedintermsofpvalue(p<0.05wasconsideredassignificant).Alltestswereperformedintriplicates.

Results and Discussion

Proximate analysis TheproximateanalysisTable1showedthatmangokernelisrichlyconstitutedofcarbohydrates(58±2%starches)withaninitialmoisturecontentof54.5±3.0%.Theproteincontentwasfoundtobe7.5%.Theaveragelipidcontentwasfoundtobe12.4%.

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Table 1:ProximateanalysisofTotapurimangokernelsCONSTITUENTS QUANTITYEnergy 411.3K.calMoisture 7.8±1%Fat 11.5±1.4%Protein 7±0.3%TotalSugars 15.6±2.0%Starch 54±0.6%Ash 2.1±0.2%

Drying curves Themoisturecontent(w.b)asafunctionoftimeforconventionaldryingandmicrowavedryingareshowninFigure2andFigure3.Conventionalmethodofdryingtooksignificantlylongertimethanmicrowave.Microwavesreducedthedryingtimeto14minuteswhenusedatpowerlevelof180Wwhileat540W,anexposureof11minutesreducedthemoisturecontentto7.5%.Char-ringofsampleswasobservedbeyond540W.Forhotairdrying,itwasnotedthatdryingiscontinuouswithtimeandlagtimewasnotobservedwhencomparedwithmicrowavedryingcurves.Thismaybeduetovibrationofwatermoleculesincaseofmicrowaveexposureandsurfacemoistureremovalafterdiffusionofmoisturefromcoreofthestructuretoouterlayersduetohydrogenbondbreaking.However,lagtimeinmicrowavedryingprocesswassmallandmaynothaveapracticalsignificance.

Figure 2:Conventionalhotairdryingofmangokernels(Ddenotesdryingtemperaturein°C)

Figure 3:Microwavedryingofkernelsfordrying(20%power:180W,40%power:360W,60%power:540W)

Scanning electron microscopy OverallstructureofmangokernelpowderasshowninFigure4.Indicatedpresenceofovalandcircularstarchgranules.Thegranuleswerefoundtobepresentinsidelayeredcomplexeswhichmaybeconsistingofprotein,lipidsandstructuralcarbo-hydrates.Similarfindingswerereportedearlierforwheatstarch[21]. Increase indryingtemperaturewasfoundtoaffect theovalgranuleswhichmaybedue todisruptionofstarchgranulesabove theirgelatinization temperature,whichwas found tostartat

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73.4°Casreportedpreviously(Kittiphoom2012).Inboththedryingmethodsthelayersstartedtodisappearfromthesurfaceofstarchgranulesasdryingtemperatureandmicrowavepowerlevelwasincreased.Structuraldisruptionwasclearlyvisibleunderhotairdryingconditionat105°C.Mildmicrowavedryingconditionswerefoundtoaffectthegranulestoalesserextentascomparedtohighestmicrowavepowerlevelinwhicharubberymassmaybeseenalongwithnointactgranules.Thestructuralchangemaybeduetoswellingofstarchgranulesinthepresenceofsignificantmoisture.Similarresultswereobtainedinstudiesperformedoncookedpastainpreviousreportswhereitwasconcludedthatpostcookingtheproteinandstarchlayersarenotdistinguishableandamyloseleachesoutfromthestarchgranulesforminglayers[21].Thus,theimageswerefoundtobeagoodevidenceofstructuralchangesduetodrying.

Figure 4 (a):Airdriedsamplesofmangokernelpowder Figure 4 (b):Mangokernelshotairdriedat40°C

Figure 4 (c):Mangokernelshotairdriedat60°C Figure 4 (d): Mangokernelshotairdriedat80°C

Figure 4 (e): Mangokernelshotairdriedat105°CFigure 4 (f):Microwavedriedkernels(at180Wpowerlevel)

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Figure 4 (g):Microwavedriedkernels(at360Wpowerlevel) Figure 4 (h):Microwavedriedkernels(at540Wpowerlevel)

Figure 4 (i):Microwavedriedkernels(at720Wpowerlevel)

Lipid yield Theyieldoflipidsfromconventionaldryingatdifferenttemperatureswasrangingfrom8.6-11.5%,whileformicrowaveitwasfoundtobe9.9-11.7%(Figure5).Thebestextractionconditionsoutofeachset(foragivendryingmethodunderdifferentextractionconditions)werecomparedamongrowsandcolumns(Table2).Foragivenextractioncondition,thedifferenceamongyieldswerecomparedatdifferentdryingcondition(Hotair(40°C,60°C,80°C,105°C),andmicrowave(180Wand360W)Thehighestyieldwasgreaterthan11%whichwasobtainedinmostofthedryingandextractionconditions.Itcanbeconcludedthatdryingathighertemperaturesdidnotaffectthelipidyield.Sincethetimerequiredformicrowavedryingissignificantlylessthanhotairdrying,thesamecanbeusedforthedryingmangokernels.Extractionyield(40°C,2h)fromthemangokernelflour,whichwasdriedat40°C,wassignificantlylowerthanotherextractionconditions(p<0.05).Itshowsthatrelativelylowtemperatureandshortertimeposesmasstransferlimitationproblemsduringoilextraction.Athighertemperatures,onewouldexpecthighdiffusioncoefficientoftheoil.Micellaviscositywouldalsoimproveathighertemperatureswhenexposedforlongertimewhichisapparent(Table2).Ingeneral,solventextractioniscarriedoutattemperaturesascloseaspossibletotheboilingpointofsolventwhichinturnimprovesthemiscibilityofoil-solventsystem.Forexample,solventextractionprocesswithn-hexanesolvent(boilingpointis68°C)istypicallykeptat60-70°C.Itisnoteworthythatbyincreasingthetimeofinteractionofsolvent(from2hto4h)withthemicellahelpedinextractingoilevenatlowtemperature(40°C)(Figure5)

Table 2:ComparisonofdryingandextractionconditionsonlipidyieldExtraction D1 D2 D3 D4 D5 D6 D72hr/40°C 8.6±0.5b,2 10.9±0.2a,1 9.2±0.4c,2 10.6±0.3a,1 10.3±0.7a,1 11.0±0.2a,1 10.9±0.2b,1

4hr/40°C 11.3±1.2a,1 11.5±0.2a,1 11.1±0.2b,1 10.5±0.4a,1 10.9±0.3a,1 10.7±0.3ab,1 9.9±0.2c,1

2hr/60°C 11.5±0.6a,1 10.7±0.5a,12 11.3±0.4a,1 9.8±0.4a,2 10.8±0.07a,12 9.8±0.3b,2 10.6±0.2b,12

4hr/60°C 11.2±0.5a,12 11.7±1.1a,123 11.2±0.3a,12 10.4±1.0a,3 10.5±0.2a,123 10.0±0.3b,3 11.7±0.2a,1

(D1:40°C, D2:60°C, D3:80°C, D4:105°C, D5:180W, D6:360W, D7:540W; The final moisture contents of dried kernels were 8%, 4.7%, 4.3%, 2.4%, 8.6%, 5.2%, 5.5% respectively. Comparisons were made using one way ANOVA across columns and rows separately. Means that do not share a common letter are significantly different e.g. letters containing “a” in one column are similar, “b” and “c” denotes dissimilarity with values with “a”; the first alphabet shows comparison across the columns (vertical comparison) i.e drying vs different extraction conditions and second numeric post coma denotes comparison across rows (horizontal comparison) i.efor a given extraction condition comparison of lipids yields were donefordifferentdryingmethods).

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Figure 5: Lipidyieldundervariousdryingandextractionconditions

Fatty acid profile and other qualitative parameters ThefattyacidprofileoflipidsextractedfromconventionallydriedseedsandmicrowavedriedkernelswerecomparedandshowninTable3.Oleicacidandstearicacidweretwomajorfattyacidspresentinthemangokerneloil.Thefattyacidprofileinallcasesmatcheswellwithreference.Thequantityofdifferentfattyacidsunderallhotairdryingconditionswasfoundtobeconsistent,irrespectiveofextractionconditions.However,anunusualobservationwasnoticedincaseofhighestmicrowavepowerlevel.Thecontentofoleicacidfoundtodecreasewhenbothdryingandextractionconditionsweretowardshigherrange.Forexample,oleicacidcontentofsamplesdriedat540Wandextractedat60°Cfor4hwerefoundtodecreasefrom44%to41%forhighestmicrowavepowerlevel.Thesimilarobservationswerefoundforlinoleicacid.Toevaluatetheeffectoftheobservationmentionedabove,oilswereextractedpostsdryingatoptimumhotairandmicrowavedryingconditionsselectedfromtheTable3.Oleicacidandlinoleicacidasreportedinoneofthefindings[23]wereshowntoundergothermalandoxidationreactiontoformaldehydes,ketonesandalco-holswhichfurtherundergooxidationintocarboxylicacidswhenfryingofmethyloleateandmethyllinoleateasmodelcompoundswasdoneat180°C.Theresultsobtainedinourstudysuggeststhatrapidandlocalizedheatingconditionsundermicrowavemayhavecauseddegradationofoleicacidwhilemildmicrowavepowerlevelmaybesuitablefordrying.Also,hotairdryingconditiondidnotinitiatethedeteriorationoflipidsbutprominenteffectsmaybeseenonthestarchgranulesathightemperatures.Thedetailedstudyonundergoingchemicalchangesaftermicrowavemayfurtherrequireanunderstandingofgaschromatography-massspectraanalysisforderivatizationandidentificationoftheintermediatecompounds.

Table 3:Fattyacidprofileforhotairandmicrowavedriedsamples

Fatty acid (%)Extraction temperature = 40°C, time = 2 hours

D1 D2 D3 D4 D5 D6 D7Palmitic (C16) 6.8 7.8 6.7 8.3 7.9 7.1 8.4Stearic (C18:0) 36.6 38.02 36.9 35.8 37.5 38.4 36.8Oleic (C18:1) 46.9 43.7 45.1 44.7 43.1 43.5 44.0Linoleic (C18: 2) 7.3 7.8 7.9 8.5 8.9 8.8 8.5Linolenic (C18:3) 0.3 0.4 0.4 0.4 0.3 0 0Unknown 1.9 2.1 2.6 2.0 1.9 2 2.0C18:2/C16 1.07 1.0 1.1 1.0 1.1 1.2 1.0

Fatty acid Extraction temperature = 40°C, time = 4 hours

D1 D2 D3 D4 D5 D6 D7Palmitic (C16) 7.4 7.6 7.3 8.4 7.8 7.8 8.1Stearic (C18:0) 39.3 38.1 38.3 35.3 38.5 37.4 35.9Oleic (C18:1) 44.1 45.1 44.6 44.7 44.8 43.1 45.9Linoleic (C18: 2) 7.0 6.4 7.5 8.6 7.1 8.9 8.2Linolenic (C18:3) 0 0.4 0 0.4 0.4 0.4 0Unknown 2.0 2.1 2.0 2.3 2.1 1.9 1.7C18:2/C16 0.9 0.8 1.0 1.0 0.9 1.1 1.0

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Fatty acid Extraction temperature = 60°C, time = 2hours

D1 D2 D3 D4 D5 D6 D7Palmitic (C16) 8.1 8.3 7.0 8.6 8.8 7.9 8.0Stearic (C18:0) 36.0 36.8 36.9 36.0 33.8 39.2 37.4Oleic (C18:1) 44.6 44.1 45.6 44.8 44.6 43.1 42.5Linoleic (C18: 2) 8.5 8.1 7.8 8.4 10.8 9.8 8.7Linolenic (C18:3) 0.4 0.4 0.4 0 0 0 0Unknown 2.0 2.0 2.0 1.9 1.8 2.01 3.1C18:2/C16 1.04 0.9 1.1 0.9 1.2 1.2 1.0

Fatty acid Extraction temperature = 60°C, time = 4hours

D1 D2 D3 D4 D5 D6 D7Palmitic (C16) 7.6 8.1 7.8 8.3 8.5 7.8 7.5Stearic (C18:0) 37.8 36.5 36.6 35.5 33.1 39.1 40.6Oleic (C18:1) 44 43.8 44.8 45 44.6 42.8 41.1Linoleic (C18: 2) 7.9 8.3 7.9 8.5 10.7 8.1 8.6Linolenic (C18:3) 0.3 0.5 0.4 0.4 0.4 0 0Unknown 2.0 2.5 2.3 2.0 2.5 2.0 1.9C18:2/C16 1.0 1.0 1.0 1.0 1.2 1.0 1.1

(D denotes drying temperature: D1:40°C, D2:60°C, D3:80°C, D4:105°C, D5:180W, D6:360W, D7:540W)

Thevaluesforqualitativeparameterssuchasperoxidevalue,iodinevalue,saponificationvalueandacidvalueareshowninTable4.Peroxidevalue(PV)indicatestheformationofhydroperoxidesinthesystemwhicharetheprimaryoxidationproductofoilsandunstableinnature.Theeffectonoilwhereseedsweredriedat540Wissignificantlydifferentthantherestofthecondi-tions.Thereasonmaybeformationoffreeradicalsathighermicrowavepowerlevels.Thisalsoconcludesthatmildpowerlevelssuchas180WhaslesschangeinPVvaluewhencomparedwithhotairdrying.Similarobservationswerenotedinacidvaluewherethesampledriedat540Wwasfoundtoshowhighestacidvalueamongall,indicatingthepresenceoffreercarboxylicacidgroupsinlipid.TheobservationmaybecorrelatedwithobservedhigherPVandsimilarfindingshavebeenreportedforvegetableoilsasdiscussedbelow.Thevaluesofiodinevalueandsaponificationvaluewerefoundtobesimilarforalltheconditions.

Table 4:ComparisonbetweendryingmethodsfortheireffectonoilqualityDrying conditions Peroxide value

(mequiv/kg of oil)Iodine value (mg/100gm of oil)

Saponification value (mg KOH/g)

Acid value (mg KOH/g)

D2 0.1±0.02 53.0±1.00 189.3±1.0 4.8±0.25D4 0.3±0.02 57.5±0.50 238.1±2.0 5.2±0.47D5 0.3±0.01 57.0±0.75 231.0±0.9 5.4±0.36D7 1.6±0.20 64.3±1.05 181.3±1.2 6.6±0.25

(D denotes drying temperature: D2:60°C, D4:105°C, D5:180W, D7:540W)

TheratioofC18:2(linoleicacid)toC16(palmiticacid)denotesastandardforfatdeterioration,linoleicacidbeingsus-ceptibleandpalmiticacidbeingresistanttooxidation[16].Inthisstudyitwasfoundthattheratioobservedmatcheswellwiththereferencevalue.Itdidnotdiffersignificantlyforconventionallydriedkernelsandmicrowavedriedkernels.Linoleicacidthough,wasfoundtobelessorabsentinmicrowavedriedkernelswhichissimilartothereportedfindings.Unsaturatedbondsarepronetooxidativecleavageathighertemperatureoracceleratedreactionsinthepresenceofmicrowaveheating. Previouslymicrowaveswerestudiedforpretreatmentofoilseeds.Astudyoneffectofmicrowaveirradiation(lowerpowerlevels)onrapeseedsexplainstheincreasedyieldofoilthroughcoldpresspostmicrowavetreatment.Thequalitativeparametersoftheextractedoilwerefoundtobesimilartothecontrolsampleswherenopretreatmentwasdone[24].Anotherstudyoneffectofqualitativeparameterspostroastingofsunflowerseedsshowedsignificantdecreaseinoilcontent,increaseinperoxidevalue,anincreaseinfreefattyacidcontentanddecreaseinunsaturatedfattyacidcontent(linoleicacid)whenseedswereexposedto500Wofpowerandroastingwasdonefor10minutes[25].Exposuresofvegetableoilstomicrowaveheatingwerefoundtodeterioratethequalityoflipidssignificantlyascomparedtohotairheating.AnincreaseintheTransisomericformofunsaturatedfattyacidwasalso reported[26-29].Thus,thefindingsofourstudymatchwellwiththephenomenadiscussedabove.

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Int J Food Nutr Sci | Volume 3: Issue 1Arora, A., et al.

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Conclusion

Thetwodryingtechniques;hotairdryingandmicrowavedryingwerecompared.Thedryingtimeusingmicrowave(180W)wasfoundtoreducesignificantly(by34folds)ascomparedtohotairdrying(60°C).Themorphologicalstudiessuggestedthathigh-ertemperatureofdryingandhighermicrowavepowerlevelschangesthestructureofthekernel.Theeffectofheatingwasfoundtobeprominentonstarchgranulesandoverlappinglayerswhichmayindicateproteindenaturationduetoheating.Athighertempera-ture(105°Chotairdrying/540Wmicrowavepower)theglobulesweredisrupted.Thestatisticalanalysisoflipidyieldssuggestedthatmicrowavedryingandhotairdryingbothwascomparableintermsoflipidyield.Theextractionconditionsunder40°C/4hor60°C/2hwerefoundtoshowlessvariationandthus60°C/2hwaschosenasoptimumsinceitwasclosetoboilingpointofn-hexaneandtimedurationrequiredwasminimum.Thequalityoflipidwasfoundtobeconsistentunderallhotairdryingtemperatureswhilethedegradationofoleicacidandlinoleicacidwereobservedforsamplesdriedat540Wunderthemicrowave.Thoughtheratioofunsaturatedtosaturatedfatremainssimilarinbothtypesofdrying,thesignificantdecreaseinoleicacidcontentforhighestmicro-wavepowerlevelalongwithincreasedperoxidevalueandacidvalueindicateddeteriorationoflipidquality.Thus,fromtheabovestudyitcanbeconcludedthatmangokernelscanbedriedbestat180Wmicrowavepowerlevel.Overall,onthebasisofstructuralchanges,lipidyieldandlipidqualitytheoptimizedconditionswereconcludedasdryingat180Wmicrowavepower,extractionat60°Cfor2h.Modifyingtheconventionalextractionmethodintermsoftime-temperatureregimeworkswellformangokernelsandloweringtheextractiontimeto2hathighertemperaturesdidnotaffecttheyieldoflipidwhendriedwithanymethod.Furtherstudiescanbedoneoneffectofstorageconditionsonlipidquality.Theresidueleftafterlipidremovalunderoptimizedconditionsmayfurtherbeprocessedtorecoverstarchandphenolics,thus,thecompleteprocessmaybedesignedasabiorefinery.

Acknowledgement Wearegrateful to theMinistryofFoodProcessing Industries (MOFPI)underDepartmentofScienceandTechnology(DST)forprovidingfundingthroughtheexternalcompetitivegrantsprogram(ProjectID:SERB/MOFPI/0036/2013).

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