Vaccine26(2008)5700–5711 ContentslistsavailableatScienceDirect Vaccine journal homepage: www.elsevier.com/locate/vaccine Th1-stimulatory polyproteins of soluble Leishmania donovani promastigotes ranging from 89.9 to 97.1kDa offers long-lasting protection against experimental visceral leishmaniasis ShraddhaKumaria,MukeshSamanta,PragyaMisraa,PrashantKharea,BrijeshSisodiab, AjitK.Shasanyb,AnuradhaDubea,∗ aDivisionofParasitology,CentralDrugResearchInstitute,Lucknow,India bProteomicsLaboratory,GeneticResourcesandBiotechnologyDivision,CentralInstituteofMedicinalandAromaticPlants,India a r t i c l e i n f o a b s t r a c t Articlehistory: Ourearlierstudiesidentifiedafraction(F2)ofLeishmaniadonovanisolublepromastigoteantigenbelonging Received4July2008 to97.4–68kDaforitsabilitytostimulateTh1-typecellularresponsesincuredvisceralleishmaniasis Receivedinrevisedform5August2008 (VL)patientsaswellasincuredhamsters.AfurtherfractionationofF2-fractionintosevensubfractions Accepted11August2008 (F2.1–F2.7)andre-assessmentfortheirimmunostimulatoryresponsesrevealedthatoutofthese,only Availableonline30August2008 four(F2.4–F2.7)belongingto89.9–97.1kDa,stimulatedremarkableTh1-typecellularresponseseither individuallyorinapooledform(P4-7). Keywords: Inthisstudythesepotentialsubfractionswerefurtherassessedfortheirprophylacticpotentialincom- SolubleLeishmaniadonovanipromastigotes binationwithBCGagainstL.donovanichallengeinhamsters.Optimumparasiteinhibition(∼99%)was (SLD) Th1-stimulatoryproteins obtainedinhamstersvaccinatedwithpooledsubfractionsandtheysurvivedfor1year.Theprotection Immunoprophylaxis wasfurthersupportedbyremarkablelymphoproliferative,IFN-(cid:2)andIL-12responsesalongwithprofound Hamsters delayedtypehypersensitivityandincreasedlevelsofLeishmania-specificIgG2antibodyasobservedon MALDI-TOF/MS days45,90and120post-challengesuggestingthatasuccessfulsubunitvaccineagainstVLmayrequire multiple Th1-immunostimulatory proteins. MALDI-TOF–MS/MS analysis of these subfractions further revealed that of the 19 identified immunostimulatory proteins, Elongation factor-2, p45, Heat shock protein-70/83,Aldolase,Enolase,Triosephosphateisomerase,DisulfideisomeraseandCalreticulinwere themajoronesinthesesubfractions. ©2008ElsevierLtd.Allrightsreserved. 1. Introduction chemotherapyforVLisfarfromsatisfactorybecauseantileishma- nial drugs are costly with unpleasant side effects. The situation Visceral leishmaniasis (VL), caused by the intracellular para- hasfurtherworsenedwithemergenceofdrugresistanceinvari- siteLeishmaniadonovani,L.chagasiandL.infantumischaracterized ousregionsofendemicity[1].Vaccinationwould,therefore,bea bydefectivecell-mediatedimmunity(CMI)andisusuallyfatalif betteroptionforaneffectivecontrolstrategyforVL. not treated properly [1]. An estimated 350 million people are at To control Leishmania infections in experimental and human risk of acquiring infection with Leishmania parasites worldwide VL, the development of an effective CMI, capable of mounting with approximately 500,000 cases of VL has been reported each Th1-typeofimmuneresponses,playanimportantrole[3–7].This year.RecentepidemicsofVLinSudanandIndiahaveresultedin is derived from the fact that a large number of people living in over 100,000 deaths [2]. With the advent of the HIV epidemics, endemic areas have self-resolving subclinical infection and the thediseasehasemergedasanimportantopportunisticinfection infectedindividualsoncerecoveredafterthetreatmentareimmune in AIDS patients [1]. In India, high incidence has been reported toreinfection.Thisprovidesarationalefordesigningimmunopro- from the states of Bihar, Assam, West Bengal and eastern Uttar phylacticstrategiesagainstVL[8].Sofar,successfulimmunization Pradeshwhereresistanceandrelapseareontheincrease.Available with fractionated and purified antigens reported against murine VLandCLhasledtoveryfewproteinsthathavebeentakenupfor preclinical/clinicalevaluation[9–12].Successfulsecondgeneration vaccineswithexcretedfactors(LiESAp)[13]orpurifiedglycopro- ∗ Correspondingauthor.Tel.:+91522212411/212418x4398; teins(FML)[14,15]areusedintrialswithefficacyandevenlicensed. fax:+91522223405/223938. There are only few reports in literature deal with vaccines, viz., E-mailaddresses:[email protected], [email protected](A.Dube). FML,FML-QuilASaponin,etc.againstcaninevisceralleishmaniasis 0264-410X/$–seefrontmatter©2008ElsevierLtd.Allrightsreserved. doi:10.1016/j.vaccine.2008.08.021 S.Kumarietal./Vaccine26(2008)5700–5711 5701 [14,16–20].Amongtherecombinantandnativeantigenstestedin andfedwithstandardrodentfoodpellet(LiptonIndiaLtd.,Bom- murinemodels,theLACKprotein[21],theLPGAPpeptides[22],the bay) and water ad libitum. The usage of hamsters was approved LeIFprotein[6]andthedp72glycoproteinofL.donovani[23]were by the Institute’s Animal Ethical Committee (protocol number protectiveimmunogensformice.Protectionresultsobtainedwith 24/05/Para/IAECdated15September2005). thethirdgenerationvaccinescomposedofcDNAencodingleishma- nialantigensclonedintoaneukaryoticexpressionvectorarestill 2.2. Parasites inpreliminarystage[24]. Although a great number of antigens have been tested for The L. donovani strain (2001) was procured from a patient protection against the cutaneous disease with in vitro cell or admitted to the Kala-azar Medical Research Centre of the Insti- mouse models, no effective vaccine against human kala-azar is tuteofMedicalSciences,BHU,Varanasiandwasculturedinvitro yet available. The reason perhaps being that the cell epitopes as described elsewhere [28]. Promastigotes were grown in L-15 that were protective in the murine model did not elicit an ade- mediumat26◦C(Sigma,USA)in75cm2cultureflasks(Nunc)[34]. quate effective immune response in human [25–27]. Hence, the The strain has also been maintained in hamsters through serial evaluation of potential leishmanial antigenic proteins for their passage,i.e.fromamastigotetoamastigote[34]. ability to elicit cellular immune responses in humans as well as in experimental model was considered important [28,29] before 2.3. PreparationofsolubleL.donovanipromastigote(SLD) theyarefurtherevaluatedfortheirprophylacticpotentialagainst antigen experimental VL. The golden hamster (Mesocricetus auratus) has been proven to be the most appropriate experimental model as SLD was prepared as per method described by Gupta et al. it largely reflects the clinic-pathological features of progressive [33,34].Briefly,latelogphasepromastigotes(109)wereharvested human VL, including a relentless increase in visceral parasitic from3to4daysofcultureandwashedfourtimesincoldphosphate- burden,cachexia,hepatosplenomegaly,pancytopenia,hypergam- bufferedsaline(PBS)andresuspendedinPBScontainingprotease maglobulinemiaandultimatelydeath.Oflate,ithasalsobeenused inhibitors cocktail (Sigma, USA) and subjected to ultrasonication extensively for vaccination studies [28,30]. Interestingly, while andcentrifugationat40,000×gfor30min.Theproteincontentof infectionofthehamsterwithL.donovanireproducedthefeatures thesupernatantwasestimated[35]andstoredat−70◦C. ofhumanVL,themechanismsofdiseaseinthehamsterdifferstrik- inglyfromthoseobtainedinmice,asuitableexperimentalmodel 2.4. SubfractionationofF2-fractionbycontinuouselutiongel forearlyinfectionofVLastheinfectiontendstoself-cureinthis electrophoresis rodentmodel[31]. Themainfocusinvaccinedevelopmenthasbeentheidentifi- SubfractionationofF2-fractionwasdonebycontinuouselution cationandcharacterizationofdefinedleishmanialantigensaswell SDS-PAGE using Laemmli’s buffer system in a ‘Prep-Cell’ (Model astheelucidationoftherangeandspecificityofantileishmanial 491;BioRad,Hercules,CA)containingfractioncollector[36].Prior immune responses. Advances made in clinical proteomic tech- tothis,aresolvinggelconcentrationsuitableforthewholerange nologieshavefurtherenhancedourmechanisticunderstandingof of proteins was determined by running a series of SDS-PAGE on leishmanial pathobiology thereby defining novel vaccine targets mini slab gel. Accordingly, 8% resolving gel and 4% stacking gel [28,32,33].Theevaluationofsuchvaccinetargetsfortheirprophy- werecastintube.Lyophilizedprotein(10mg)wasloadedunder lacticpotentialwillprovidefurtherleadtowardsthedevelopment standard condition [37] and electrophoresis was carried out as ofacandidatevaccine(s). perprotocolmentionedinmanufacturer’smanual,Total120frac- We have further fractionated the Th1-stimulatory fraction of tionswerecollectedandeachwasanalyzedconsequentlyonmini 68–97.4kDa (F2) of soluble protein of L. donovani promastigotes gel slabs and silver stained [38] to visualize the eluted proteins. bycontinuouselutiongelelectrophoresis(Prep-Cell)onthebasis Wide range molecular weight marker (Bangalore Genei, India) of molecular weight and there of obtained seven subfractions was used to identify and assess the exact molecular weights of (F2.1–F2.7)belongingto69.0,74.9,78.4,89.9,94.9,96.9,97.1kDa, protein bands and their number and density were assessed by respectively[86].Outofsevensubfractionsonlyfoursubfractionsof softwareAlphaImagerTM2200.Fractionnumber40–100displayed 89.9,94.9,96.9,97.1kDastimulatedremarkablecellularresponses, theproteinbandsrangingbetweenthedesiredmolecularweight i.e.lymphoproliferative,IFN-(cid:2)andIL-12responsesandsuppressed of 68–97.4kDa. The bands with identical molecular weight were IL-10 cytokine levels in cured/exposed VL patients as well as in pooledinsuchawaysoastoprovidesevendiscretesubfractions cured Leishmania infected hamsters. Interestingly, all of these as F2.1,F2.2,F2.3,F2.4,F2.5,F2.6andF2.7[86].Thesubfractionswere pooledsubfractionsyieldedoptimumefficacyascomparedtothe furtherprocessedforSDSremovalbythemethodofWesseland individualones. Flügge[39].TheremovalofSDSwascheckedbycolorimetricesti- In this study, these potential antigenic subfractions were mationusingthemethodofArandetal.[40].Proteinquantification assessed for their prophylactic efficacy alongwith Bacillus Cal- wasdonebyLowry’smethod[35]. metteGuerin(BCG)—anadjuvant,againstL.donovaniinfectionin Themostpotentsubfractions(F2.4–F2.7)weretakenbothindi- hamsters.Thosesubfractionswhichexhibitedsignificantcellular viduallyaswellasinpooledform(referredasP4-7subfraction)for responsesaswellasprophylacticpotentialwerefurthercharacter- vaccination studies. In addition, the subfractions F2.1–F2.7 were izedbyMALDI-TOF/TOF-MSsoastoensuretheproteincontentsas alsopooledintooneandusedasreferenceantigen(F2). prospectivevaccinetargets. 2.5. Vaccination 2. Materialsandmethods Ninegroupscontaining12–15hamstersineachwereemployed 2.1. Animalandparasites fortheimmunizationwithdifferentpreparationsofantigenicfrac- tions.ThehamstersofGroups1–7wereimmunizedintradermally Laboratory bred male golden hamsters (M. auratus, 45–50g) onthebackwitheachsubfractionsF2.4,F2.5,F2.6,F2.7,P4-7,F2- from the Institute’s Animal House Facility were used as experi- fractionandSLD(50(cid:3)g/(0.05mlanimal))alongwithequalvolume mental host. They were housed in climatically controlled room of BCG (0.1mg/(0.05mlanimal)) in emulsified form. The eighth 5702 S.Kumarietal./Vaccine26(2008)5700–5711 groupwasgivenBCGonlyandthelastninthgroupwhichreceived (BARC,India)wasaddedtoeachwellandthentheywereharvested onlyPBSservedascontrol.Fifteendayslateraboosterdoseofhalf onglassfibremats(Whatman)andcountedinaliquidscintillation oftheamountofantigensalongwithBCGorPBSwasgivenintra- counter. Results were expressed as stimulation index (SI) which dermallytoallthehamstersofrespectiveexperimentalgroups(i.e. wascalculatedasmeancountsperminute(cpm)ofstimulatedcul- Groups1–8)asmentionedabove. ture/meancpmofunstimulatedcontrol.SIvaluesofmorethan2.5 wereconsideredaspositiveresponse. 2.6. Infection 2.7.3. QuantificationofNOinmacrophagesofhamstersandcell Twenty-onedaysaftertheboosterdose,allthevaccinatedand lines unvaccinated control groups were challenged intracardially with Thepresenceofnitrite(NO −)contentwasassessedusingGriess 2 108 latelogphasepromastigotesofL.donovani.Theprophylactic reagent in the culture supernatants of naïve hamster peritoneal efficacyoftheimmunogenwasassessedinspleen,liverandbone macrophages after the exposure with supernatant of stimulated marrowofthreevaccinatedhamstersonnecropsyatdifferenttime lymphocyte’s cultures. Briefly, isolated peritoneal macrophages intervals,i.e.ondays0,45,90,120post-challenge(p.c.).Peritoneal [42]weresuspendedinculturemediumandplatedat106cells/well exudatescells,inguinallymphnodesandbloodwerealsocollected andexposedtothesupernatantsofabovedescribed5-day-oldanti- atthesetimepointstoobtaincellsandseraforevaluationofcellular gen stimulated lymphocyte’s cultures from all the study groups. andantibodyresponses[41]. The supernatants (100(cid:3)l) collected from macrophage cultures Thecriterionofprophylacticefficacywastheassessmentofpar- 24h after incubation was mixed with an equal volume of Griess asiteloadasthenumberofamastigotes/1000cellnucleiineach reagent(Sigma,USA)andleftfor10minatroomtemperature.The organincomparisontotheunvaccinatedcontrolsandthepercent- absorbance of the reaction was measured at 540nm in an ELISA ageinhibition(PI),wasassessedincomparisontotheunvaccinated reader[43]. controlbyfollowingformula[28]: 2.7.4. RT-PCRofmRNAcytokinesandinducibleNOsynthase No.ofparasitecountfrominfectedcontrol (iNOS) −No.ofparasitefromvaccinatedgroup PI= ×100 RT-PCRwasperformedtoassesstheexpressionofvariousmRNA No.ofparasitecountfrominfectedcontrol cytokinesandiNOSinsplenocytesofmainexperimentalgroupsas For post-challenge survival animals from both the experimental wellasunvaccinatedcontrolanimals.Threerepresentativeham- andcontrolgroupsweregivenpropercareandwereobservedfor sters from each experimental group were randomly selected to theirsurvivalperiodwhichlastedformorethan12monthsp.c.Sur- analyzethespleniccytokineprofile.RNAfromsplenocytesofdif- vivalofindividualhamsterwasrecordedandmeansurvivalperiod ferentgroupsofhamsterswasisolatedusingTri-reagent(Sigma, wascalculated. USA) on days 45, 90 and 120 p.c. and quantified by using Gene- quant(Biorad,USA).TheprimersequencesofcytokineandiNOS 2.7. Immunologicalassays primersasdescribedbyMelbyetal.[44]asmentionedinTable1 wereusedtoamplifytheirrespectivecDNA.HGPRTwasusedasa 2.7.1. Delayedtypehypersensitivity(DTH) housekeepingcontrol. DTHwasperformedbyinjectingintradermally50(cid:3)g/50(cid:3)lof OnemicrogramoftotalRNAwasusedforthesynthesisofcDNA SLD in PBS into one footpad and PBS alone into the other foot- usingfirststrandcDNAsynthesiskit(Fermentas).0.5(cid:3)gofcDNA pad of each vaccinated hamsters and unvaccinated controls. The wasamplifiedbyPCRunderthefollowingcondition:initialdenat- responsewasevaluated24hlaterbymeasuringthedifferencein urationat95◦Cfor2min,40cyclesofdenaturationstepeachat footpadswellingbetweeneachofthevaccinatedandcontrolgroups 95◦Cfor30s,annealingat55◦Cfor40s,followedbyextensionstep ofhamsters[4]. at72◦Cfor40s.Thefinalextensionstepwascarriedoutat72◦C for10min.Further,thedensitometricanalysisofPCRproductwas 2.7.2. Lymphocyteproliferationassay(LTT) carriedoutusingsoftwareAlphaImagerTM2200(Alfainnotech).The Lymphocytessuspension(1×106ml−1)ofvaccinatedhamsters samebandareawastakenforbandintensityandwasnormalizedto was cultured in 96-well flat bottom tissue culture plates (Nunc, HGPRT.Themeanpercentageexpressionvalueswererepresented Denmark).Thisassaywascarriedoutasperprotocoldescribedby relativetotheircorrespondingHGPRTvalues. Gargetal.[28].About100(cid:3)lofpredeterminedconcentrationof mitogen-ConA(10(cid:3)g/ml,Sigma,USA)andantigen-SLD(10(cid:3)g/ml 2.7.5. Antileishmanialantibodyresponses each)wereaddedtothewellsintriplicate.Wellswithoutstimu- Thelevelofantileishmanialantibodyinserasamplesfromham- lantsservedasblankcontrols. stersofboththesetofexperimentalgroupswasmeasuredasper Cultureswereincubatedat37◦CinaCO incubator(5%CO )for protocolofVolleretal.[41].Briefly,ELISAplates(Nunc,Denmark) 2 2 3daysinthecaseofConAandfor5daysinthecaseofSLD.Eigh- were coated overnight at 4◦C with 1(cid:3)g/ml SLD antigen diluted teenhourspriortoterminationofculture,0.5(cid:3)Ciof[3H]thymidine in0.02Mphosphatebuffer(pH7.5)andwerethenblockedwith Table1 Sequenceofreverseandforwardprimers S.no. Primer Primersequence Productsize(bp) 1 HGPRT:forward;reverse 5(cid:5)ATCACATTATGGCCCTCTGTG3(cid:5);5(cid:5)CTGATAAAATCTACAGTYATGG3(cid:5) 125 2 iNOS:forward;reverse 5(cid:5)GCAGAATGTGACCATCATGG3(cid:5);5(cid:5)CTCGAYCTGGTAGTAGTAGAA3(cid:5) 198 3 IFN(cid:2):forward;reverse 5(cid:5)GGATATCTGGAGGAACTGGC3(cid:5);5(cid:5)CGACTCCTTTTCCGCTTCCT3(cid:5) 309 4 IL-12:forward;reverse 5(cid:5)GTACACCTGYCACAAAGGAG3(cid:5);5(cid:5)GATGTCCCTGATGAAGAAGC3(cid:5) 430 5 TGF(cid:4):forward;reverse 5(cid:5)CCCTGGAYACCAACTATTGC3(cid:5);5(cid:5)ATGTTGGACARCTGCTCCAC3(cid:5) 310 6 IL-4:forward;reverse 5(cid:5)CATTGCATYGTTAGCRTCTC3(cid:5);5(cid:5)TTCCAGGAAGTCTTTCAGTG3(cid:5) 463 7 IL-10:forward;reverse 5(cid:5)ACAATAACTGCACCCACTTC3(cid:5);5(cid:5)AGGCTTCTATGCAGTTGATG3(cid:5) 432 DegeneratebasesareindicatedbytheappropriateInternationalUnionofPureandAppliedChemistrydesignation(Y=CorT,R=AorG). S.Kumarietal./Vaccine26(2008)5700–5711 5703 1% BSA in PBS, after washing with PBS containing 0.05% Tween pendentexperiments)wereanalyzedbyone-wayANOVAtestand 20. The optimum dilution of sera for determination of IgG was comparisonswithcontroldataweremadewithDunnett’spost-test foundtobe1:200andforIgG1andIgG21:100in1%BSA–PBSat usingGraphPadPrismsoftwareprogram.Comparisonsweremade 4◦Cfor1.5h.AfterwashingwithPBSTweentheplateswereincu- betweeninfectedcontrolgroupsandalltheexperimentalgroups. batedfor3hwithHRP-conjugatedGoatanti-HamsterIgG(H+L) TheupperlevelofsignificancewaschosenasP<0.001. (1:1000)(Serotec,USA).Parallely,plateswereincubatedovernight withBiotin-conjugatedmouseanti-HamsterIgG1andmouseanti- 3. Results Armenianandanti-SyrianhamsterIgG2(BD,Pharmingen)2(cid:3)g/ml in PBS (100(cid:3)l/well) and incubated for 3h according to manu- 3.1. Vaccinationwithpotentialsubfractionsinpooledform factures instruction. The plates were developed using the OPD inducedoptimumprotectionagainstL.donovanichallenge substrate(o-phenylenediaminedihydrochloride,Sigma)andread at492nmusinganELISAreader(BioTek,USA). Thepotentialsubfractionsvaccinatedhamsterswereprotected from the challenge infection of L. donovani, as observed by their 2.8. MALDIanalysisofpotentTh1-stimulatorysubfractions weight gains (Fig. 1A) similar to normal hamsters kept simulta- neouslyforthesametimeperiod,i.e.ondays45,90and120p.c. The potential subfractions F2.4–F2.7 were run on one- Hepatosplenomegaly,associatedwithchallengeinfection,wasvir- dimensional PAGE (12% resolving gel, 1.0mm thick). Bands were tuallyabsentinthepotentialsubfractionsvaccinatedgroup(Fig.1B separatedoutandweredigestedin-gelasperprotocoldescribed andC).Parasiteloadwasdirectlycorrelatedwithweightandsize earlier [33,45]. Briefly, the coomassie blue stained bands were of liver and spleens among different groups: significant parasite washed, in-gel reduced, S-alkylated and digested with trypsin (Promega, Madison, WI, USA) at 37◦C overnight. Peptides were inhibitionwasobservedinhamstersvaccinatedwithF2.5,F2.6and F2.7 subfractions, P4-7 subfractions and F2-fraction wherein the extracted, dried in a Speed-Vac and resolubilized in 0.1% tri- parasiteloadwasobservedtobe≤2×102.Interestingly,thepro- fluoroacetic acid. Zip Tips (Millipore) were used to desalt and phylactic efficacy was more marked in the hamsters immunized concentratethepeptidemixture.Peptidemassfingerprintingwas withP4-7subfractions.Therewasprogressivedecreaseinparasite performedbyspotting0.3(cid:3)loftheextractedproteindigestmixed loadinspleen,liverandbonemarrowfrom<1×102,amorethan with(cid:5)-cyano-4-hydroxycinnamicacid(CHCA,Sigma)onaMALDI 96%inhibitionofparasitemultiplicationonday45p.c.toanegli- targetplate.MSandMS/MSspectrumwereacquiredinthepositive giblelevelonday120p.c.,renderingthemdifficulttodiscern,i.e. ionmodeonMALDI-TOF/TOFMassSpectrometer,AppliedBiosys- ∼99%parasiteinhibitionwasobserved(Fig.2A–C).F2andSLDvac- tems4700ProteomicsAnalyzer(Framingham,MA,USA). cinatedhamstersharboredmorethan2×102parasitesonday45 Theinstrumentwasoperatedinthedelayedextractionmode p.c.TheremainingparasiteintheP4-7pooledsubfractionvacci- with delay time of 200ns. Spectra were obtained by accumula- natedgroup,whencheckedfortheirvirulenceonday120p.c.by tionof1000and4000consecutivelasershotsrespectivelyinMS puttingthesplenic/livertissueandlymphnodesininvitroculture, and MS/MS mode and laser intensity used were in the range of didnotconvertintopromastigotesevenafter10daysofculture. 5000–6000.CloseexternalcalibrationforMSwasperformedwith Allthevaccinatedhamstersimmunizedwiththeindividualsub- 4700CalMix(AppliedBiosystems,USA)astandardmixture.Peak fractionsF2.5–F2.7andpooledP4-7subfractionssurvivedlonger harvestingwascarriedoutusing4000SeriesExplorerTMSoftware afterthelethalchallengeofL.donovaniandremainedhealthyuntil (AppliedBiosystems,USA).Onlybaselinecorrectionswereapplied the termination of the experiment at 12 months post-infection. totherawdata. WhilehamstersimmunizedwithF2.4subfraction,F2-fractionand Database searching for protein identifications was performed SLDsurvivedonlytill6months,allthehamsterswhichwereimmu- with mass spectrometry data (MS or MS/MS) using Global Pro- nizedwithBCGaloneaswellasunimmunizedonessuccumbedto teome Server v3.5 software (Applied Biosystems, USA) equipped virulentL.donovanichallengewithin2–2.5months. withMASCOT(MatrixScience)searchengine.Onlymonoisotopic masseswereusedforsearchingagainsttheSwiss-ProtandNCBInr databases with a minimum number of matched masses set at 3.2. PotentialsubfractionsstimulatesubstantialDTHand 4. The maximum peptide precursor tolerance was set at 40ppm mitogenicandLeishmania-specificcellularresponsesin and MS/MS fragment tolerance was defined as 0.2Da. At most immunizedhamsters one missed cleavage for tryptic peptides was allowed, and the modificationsacceptedwerecarbamidomethylcysteinesasfixed Tocharacterizethefateofcell-mediatedimmuneresponsefol- modification and methionine oxidation as variable modification. lowingimmunizationwehaveinvestigatedthepotentsubfractions Tandem MS was performed only in the cases where identifica- (F2.4–F2.7)inducedDTHresponsesinhamsterschallengedwithL. tionappearedambiguouswithMALDI-TOF–MSdata.Thecriteria donovaniandthecapacityoftheircellstoproliferateinresponseto usedtoacceptidentificationsforpeptidemassfingerprintincluded mitogenandleishmaniaantigen-SLDondays0,45,90and120p.c. the probabilistic protein score-based confidence interval %, the Fig.3Ashowsthatthehamstersreceivingpotentsubfractionseither extentofsequencecoverage,thenumberofpeptidesmatchedand individuallyorinpooledformdisplayedsignificantlystrongerDTH whetherLeishmaniaspp.orTrypanosomaproteinappearedastop responseascomparedwiththeothergroups,viz.,infectedcontrol candidatesduringthefirstsearch,whennorestrictionwasapplied and BCG vaccinated hamsters at these time points. Immuniza- to the species of origin. Identification criteria with MS/MS data tionwithP4-7inducedsignificantly(P<0.001)higherlevelofDTH werethatpeptidescountshouldbenotlessthantwoormoreand response,i.e.eightfoldincreaseascomparedtoinfectedcontrolon confidenceinterval%forthebestionscoreshouldbeabove95[33]. day45p.c.thatremainedincreasedsignificantlythroughday90till day120p.c. 2.9. Statisticalanalysis Invitrostimulationofthelymphocyteswiththemitogen-Con A, showed proliferative responses with no differences between Resultswereexpressedasmean±S.D.Threesetsofexperiments control and antigen immunized groups at pre-challenge time were performed for vaccination studies and in each experiment point(Fig.3BandC).Followingchallenge,thevaccinatedgroups 10–15animalswereused.Theresults(pooleddataofthreeinde- showed intact responses to Con A but, on the other hand, it 5704 S.Kumarietal./Vaccine26(2008)5700–5711 Fig.1. Bodyweight(A),weightofspleen(B)andliver(C)ingondays45,90and120p.c.ofvaccinatedhamsterswithpotentsubfractions(F2.4–F2.7),pooledsubfraction P4-7,F2-fractionandSLD.Eachbarrepresentsthepooleddata(mean±S.D.value)ofthreereplicates. was lowered in the infected control groups. In antigen-specific 3.3. ImmunizationwithP4-7subfractionelicitsprominent re-stimulation assays, performed after immunization, there was Th1-typecytokineresponseinprotectedgroupofhamstersby significant(P<0.001)stimulatoryresponseinthecellsofhamsters RT-PCR vaccinatedwithpotentsubfractionsF2.4–F2.7incombinationwith BCGonday45p.c.,whichwas∼10–20foldshigherascompared Impairment of CMI response during active VL is reflected by totheinfectedcontrolgroup(Fig.3C).Moreover,maximumlym- marked T-cell anergy specific to Leishmania antigens [30]. Since phoproliferativeresponsewasnoticedonday45p.c.inthecells optimumprotectiveefficacywasobservedinP4-7vaccinatedham- ofanimalsimmunizedwithP4-7subfractionwhichwas∼27folds sters, the expression of Th1 and Th2 cytokines was evaluated in higherandtheresponsesincreasedprogressivelyondays90and this group only and compared with infected and normal control 120p.c.Ontheotherhand,therewasnoproliferativeresponsein groupofanimals.AcomparativeRNAcytokineprofileofspleno- animalsvaccinatedwithBCGaloneaswellasunvaccinatedinfected cytes,analyzedondays45,90,and120p.c.,showedthatamongthe control(Fig.3C). threegroupsofhamstersexpressionofIFN-(cid:2)andIL-12transcripts Similarly, we have observed that macrophages isolated from wassuppressedininfectedgroup,butwassignificantlyhigherby naïvehamsters,whenincubatedwithstimulatedsupernatantsof two and three folds, respectively (P<0.001) in vaccinated group lymphocytesfromP4-7subfractionvaccinatedhamsters,produced (Fig. 4A). Higher expression of two to three folds of iNOS tran- significantamountofNOwhichwas∼7foldsmorethantheinfected scriptwasobservedinP4-7vaccinatedhamstersascomparedto controlsonday45p.c.TheNOlevelwasfurtherincreasedincredibly theinfectedcontrolson45daysp.c.(Fig.4B).Levelofexpressionof bydays90and120p.c.Incontrast,littleamountofNOwaspro- Th1suppressivecytokines,TGF-(cid:4),IL-10andIL-4whichwereup- ducedbythecellsofhamstersbelongingtounvaccinatedcontrol regulatedininfectedgroup,weresignificantlydown-regulatedin groupandBCGonly(Fig.3D). P4-7vaccinatedhamstersbydays45through120p.c.(Fig.4B). S.Kumarietal./Vaccine26(2008)5700–5711 5705 Fig.2. Parasiteburden(no.ofamastigotesper1000cellnuclei)ondays45,90and120p.c.in(A)spleen,(B)liverand(C)bonemarrowofvaccinatedhamsterswithpotent subfractions(F2.4–F2.7),pooledsubfractionP4-7,F2-fractionandSLD.Eachbarrepresentsthepooleddata(mean±S.D.value)ofthreereplicates. 3.4. PotentsubfractionscausedecreaseinLeishmania-specific 3.5. Characterizationofthefourpotentsubfractionsby1-DGE IgGandIgG1isotypeandincreaseinIgG2isotypeantibody andMALDI-TOF–MS responsesinvaccinatedhamsters Inordertoassessthecomponentsofthefourpotentsubfractions Wehaveassessedtheleishmanialantigen-specificIgGandits theircharacterizationbyMALDI-TOF–MSwascarriedout.Major- isotype(IgG1andIgG2)levelsintheseraofallthegroupsofvac- ity of the proteins was detected around 4–8 pI acidic to neutral cinated hamsters through ELISA. As shown in Fig. 5C the groups pHrange.MassesandpIwerecalculatedbysoftware;measuresof ofhamstersvaccinatedwithpotentialsubfractionsdevelopedan theconfidenceoftheidentificationonthebasisofnumberofpep- effectiveimmuneresponsebyshowingsubstantiallyhigherlevels tidesmatchedandsequencecoveragewhichwasdeterminedusing ofIgG2antibody,whichisameasureofCMI(Fig.5C).Ahighlysig- MASCOT.Theidentifiedspotsmatchedto168databaseentries.Of nificantdifference(twofolds)wasfoundinIgG2levelbetweenP4-7 spotsanalyzedbyMALDI-TOFandMS/MS,41%wereclearlyiden- vaccinatedandinfectedcontrolgroupsofhamsters(P<0.001).In tifiedbytheirhomologywiththoseofL.major.Theproteinsthus contrast,therewasdecreasedlevelsofIgGandIgG1(P<0.5)inP4-7 identifiedarelistedinTable2.Theanalysisrevealedthesimilar- vaccinatedhamstersascomparedtotheinfectedcontrols(Fig.5A ityofproteinpatternasobservedwith2DgelmapofF2-fraction andB). [33]. In all, a total of 19 proteins were identified by 1-DGE and 5706 S.Kumarietal./Vaccine26(2008)5700–5711 Fig.3. Cellularresponsesondays45,90and120p.c.inhamstersvaccinatedwithpotentfractionhamsterswithpotentsubfractions(F2.4–F2.7),pooledsubfractionP4-7, F2-fractionandSLDalongwithBCG.Datafornormalandunvaccinatedinfectedgroupshavebeenrepresentedascontrolgroups,respectively.(A)DTHresponse(mm)to SLDinhamsterswasmeasuredasfootpadswellingat24h,(BandC)LTTresponse(SIvalue)againstConAandSLD.SIvaluesofmorethan2.5wereconsideredaspositive response,and(D)NOproduction((cid:3)g/ml).Eachbarrepresentsthepooleddata(mean±S.D.value)ofthreereplicates. Fig.4. AnalysisofTh1andTh2mRNAcytokineprofileinnormal,infectedandP4-7vaccinatedhamstersondays45,90and120p.c.byRT-PCR.(A)SpleniciNOSandcytokine expression.Eachbandrepresentsoneoutofthreerepresentativehamstersfromeachexperimentalgroup.(B)Densitometryanalysisshowingtherelativemean%changein iNOSandcytokinemRNAexpression±S.D.incomparisontocontrol(HGPRT).Significancevaluesindicatethedifferencebetweenvariousanimalgroupsandnormalgroup (*P<0.05and***P<0.001). S.Kumarietal./Vaccine26(2008)5700–5711 5707 Fig.5. Antileishmanialantibodylevels(ODvalue)inhamstersvaccinatedwithpotentsubfractions(F2.4–F2.7),pooledsubfractionP4-7,F2-fractionandSLDofLeishmania donovanialongwithBCGondays45,90and120p.c.DataforBCGvaccinated,unvaccinatedcontrolandnormalhamstersrepresentedaspositiveandnegativecontrolgroups, respectively(A)IgGanditsisotype(B)IgG1or(C)IgG2.Eachbarrepresentsthepooleddata(mean±S.D.value)ofthreereplicates. MALDI-TOF–MSinsubfractionsF2.4–F2.7,includingfivehypothet- of lymphocytes in vitro and the release of very high amount of icalproteins/unknowns.Amongthese,mostoftheseproteinswere Th1-typecytokines,viz.,IFN-(cid:2)andIL-12p40,wereobserved.Again, ofknownimmunostimulatoryorimmunogenictypeorhavebeen theexcellentcellularresponseswereobtainedwhenallthefour evaluatedasvaccinecandidatessuchasElongationfactor-2,p45, subfractions were pooled together, i.e. P4-7. On the other hand, HSP-70, HSP-83, Fructose-1,6-Bisphosphate Aldolase (Aldolase), theTh2-typecytokineIL-10wasfoundtobesuppressedincured Enolase, Triosephosphate isomerase (TPI), Protein Disulfideiso- patientsaswellasinendemiccontactsagainstallthesubfractions merase and Calreticulin. Some of the other proteins including [86]. someenzymesfromenergymetabolism,phosphorylationpathway, Basedontheirimmunostimulatoryproperties,thefourpotent aminoacidmetabolismpathwaysandfromdiversemetabolicroute individualsubfractionsaswellaspooledonewerefurtherevalu- havealsobeenreportedaspotentialdrugtargets,viz.,Adenosyl- atedfortheirimmunoprophylacticpotentialwithBCGinhamsters. homocysteinase,Cofactor-independentphosphoglyceratemutase, BCGhadbeenusedasanadjuvantduetoitspropertyofactivating Trypanothione reductase, and NAD-dependent deacetylase SIR2 macrophagesforinducingNO[46,47]andelicitinglong-lastingcel- homolog. lularandhumoralimmuneresponses[48,49].Althoughsignificant parasiteinhibitionwasnoticedinhamstersimmunizedwitheither 4. Discussion ofF2.5–F2.7subfractionsorF2-fraction,theefficacywasremark- ableinhamstersreceivingP4-7subfractions.Theparasiteloadinall Previous studies from this laboratory have hinted toward the visceralorgansdecreasedprogressivelyreachinganegligiblelevel prophylacticpotentialofF2-fractionofsolublepromastigoteanti- byday120p.c.,renderingthemdifficulttodiscerndemonstrating genbelongingto68–97.4kDainexperimentalVLmodel[28].Using its strong vaccine potential. Moreover, post-challenge mean sur- theconventionalscreeningapproachfoursubfractionsbelongingto vivalofhamstersinP4-7subfractionvaccinatedgroupalongwith molecularweightof89.9,94.9,96.9,97.1kDawereidentifiedwhich F2.5–F2.7vaccinatedhamstersbeingmorethan12monthsfurther gaveconsiderablygoodcellularresponse,viz.,lymphoproliferative strengthen the evidence that combination of all the four potent aswellasNOreleaseagainstallthecuredhamsters.However,the subfractionsarerequiredtoinduceoptimumprophylacticefficacy. optimumcellularresponseswereobservedwhenallthefoursub- Mostoftheassaysinthisstudyweredonebetween45and120 fractions were pooled together, i.e. P4-7. The responses of these dayspost-challengeasthediseaseprogressionreachesitspeakby identifiedsubfractionsinhamsterswerefurthervalidatedincured thistime.Successfulvaccinationofhumansandanimalsisoften patients/endemiccontactsandanalogousresults,i.e.proliferation relatedtoantigeninducedDTHresponsesinvivoandT-cellstim- 5708 S.Kumarietal./Vaccine26(2008)5700–5711 Table2 ImmunostimulatoryproteinsidentifiedinpotentsubfractionF2.4,F2.5,F2.6andF2.7ofF2MALDI-TOF–MS/MS SFsa Identifiedproteinsb Sp.c Acc.no.d kDa/pIe Pm/Ms/Sc%f FCg Remarksh Cofactor-independentphosphoglyceratemutase Lmx 28400787 61/5.4 10/151/20 5 DT[72] Trypanothionereductase Lmj 7677022 53/5.8 12/117/32 5 DT[73] HypotheticalproteinL5769.02 Lmj 12311865 29/6.8 10/100/25 ??i ?j NAD-dependentdeacetylaseSIR2homolog Lmj *SIR2LEIMA 43/5.64 16/75/14 4 DT[74] Adenosylhomocysteinase Ld 1710837 48/5.7 17/98/21 5 DT[75] F2.4 Proteinofunknownfunction Tc 32401138 38/5.22 15/114/31 ??i ?j Fructose-1,6-BisphosphateAldolase Lmx 5834626 47/7.9 18/152/14 1–3 VC,DT[58,59,76] Elongationfactor-2 Lmj 11244578 75/7.2 24/124/32 4 Th1[68] Enolase Lmj 8388689 46/5.6 21/124/38 1–4 IGP[59,63,76] Heatshock70-relatedprotein1precursor Lmj 50299857 69/5.5 19/115/32 1 Th1[65–67] NAD-dependentdeacetylaseSIR2homolog Lmj *SIR2LEIMA 43/5.7 12/63/28 4 DT[74] Adenosylhomocysteinase Ld 1710837 48/5.7 10/102/23 5 DT[75] Proteinofunknownfunction Tc 32401138 38/5.22 15/121/36 ??i ?j Enolase Lmj 8388689 46/6.6 16/167/27 1–4 IGP[59,63,76] F2.5 Fructose-1,6-BisphosphateAldolase Lmx 5834626 47/7.5 16/155/38 1–3 VC,DT[58,59,76] dnaK-typemolecularchaperonehsp70.4 Lmj 7441842 70/5.5 13/89/39 1 Th1[65–67] DisulfideisomerasePDI Lmj 25990151 52/5.2 9/100/25 1 VF,DT,VC[70] Elongationfactor-2 Lmj 11244578 73/7.2 15/114/29 4 Th1[68] Hypotheticalprotein5769.02 Lmj 12311865 29/6.8 11/86/34 ??i ?j Elongationfactor-2 Lmj 11244578 73/7.2 15/114/29 4 Th1[68] Enolase Lmj 8388689 46/6.6 16/104/27 1–4 IGP[59,63,76] Fructose-1,6-BisphosphateAldolase Lmx 5834626 41/7.0 16/156/32 1–3 VC,DT[58,59,76] Proteinofunknownfunction Tc 32401138 38/5.22 15/121/36 ??i ?j Heatshock70-relatedprotein1precursor Lmj 50299857 69/5.5 9/128/29 1 Th1[65–67] F2.6 DisulfideisomerasePDI Lmj 25990151 55/5.2 9/100/25 1 VF,DT,VC[70] Hypotheticalprotein,unlikely Tb 25992853 53/5.5 17/86/33 ??i ?j p45 Lmj 6274526 44/6.6 15/156/37 5 T-cellst[68] Calreticulin Lmj 5263289 33/4.7 16/87/25 1 VF,IGP[20,69] Triosephosphateisomeraseglycosomal Tc *TPISTRYCR 76/6.6 15/142/38 1–3 Th1,VC[61,62] Heatshockprotein-90 Ld 323030 53/5.6 24/128/34 1 Th1[65–67] Calreticulin Lmj 5263289 33/4.7 8/74/21 1 VF,IGP[20,69] Triosephosphateisomerase,glycosomal Tc *TPISTRYCR 76/6.6 21/212/31 1–3 Th1,VC[61,62] Hypotheticalprotein Lmx 2131001 47/7.1 12/125/31 ??i ?j HypotheticalproteinL2385.08 Lmj 12311835 84/5.4 14/121/37 ??i ?j Heatshock70-related Lmj 50299857 69/5.5 21/137/32 1 Th1[65–67] F2.7 Elongationfactor-2 Lmj 11244578 73/7.2 15/114/29 4 Th1[68] DisulfideisomerasePDI Lmj 25990151 52/5.2 15/110/25 1 VF,DT,VC[70] Enolase Lmj 8388689 46/6.6 19/127/39 1–4 IGP[59,63,76] Fructose-1,6-BisphosphateAldolase Lmx 5834626 45/7.9 16/102/27 1–3 VC,DT[58,59,76] p45 Lmj 6274526 41/6.6 12/126/46 5 T-cellst[68] Hsp83protein Ldi 362545 81/5.1 21/141/25 1 Th1[65–67] Theproteinspotsindicatedinthistablewereidentifiedusingpeptidemassfingerprinting. a Subfractionno. b Nameoftheprotein. c Species:Lmx,Leishmaniamexicana;Lmj,Leishmaniamajor;Li,Leishmaniainfantum;Ld,Leishmaniadonovani;Ldf,Leishmaniadonovaniinfantum;Ldc,Leishmaniadonovani chagasi;Tb,Trypanosomabrucei;Tbr,Trypanosomabruceirhodesiense;Tc,Trypanosomacruzi. d AccessionnumbersaccordingtoNCBIand*Swiss-Protaccessionnumber. e PredictedMrandpI. f No.ofpeptidesmatched/MOWSEscore/sequencecovered%. g Identifiedproteinsfellintothefollowingmajorsixfunctionalcategories;withsomeofthemfallingintotwoormoregroups:1.stressresponse;2.cytoskeletonandcell membrane;3.energymetabolismandphosphorylation;4.cellcycleandproliferation;5.aminoacidmetabolism. h Remarks:VC,vaccinecandidate;Th1,Th1stimulatory;T-cellst,T-cellstimulatoryproteins;VF,virulencefactor;DT,drugtargetmolecule;IGP,immunogenicprotein; IDP,immunodiagnosticprotein. i ?Notpreviouslydescribed. j ??Unknowns/hypotheticalfunctionoftheproteinarenotknown. ulation with antigen in vitro [4,50]. It has been further reported regardingtheup-regulationofinducibleNOsynthase(iNOS,NOS2) that a major factor that is believed to contribute to healing in byTh1cellassociatedcytokinesandconfirmsthatNOmediated leishmaniasis is the development of strong CMI responses like macrophageeffectormechanismiscriticalinthecontrolofparasite DTH responses, T-cell responses and NO production [28,51–53]. replicationintheanimalmodel[28]. Notably, the hamsters vaccinated with P4-7 subfraction elicited ThepresenceofacomparableexistenceofTh1andTh2clones strongestDTHreaction,LTTresponsesandNOproduction,among producingIL-12andIFN-(cid:2)aswellasIL-10obtainedfrompatients alltheexperimentalgroupssuggestingagoodcorrelationbetween cured of VL encouraged us to assess whether the protective CMIandresistancetoinfectioninthismodel.Inaddition,allthe responsewhichwasutmostelicitedbyP4-7vaccinationinham- hamstersvaccinatedwithpotentsubfractionschallengedwithL. sterscanreflectthisfeatureofclinicalfindings[54–56].Following donovani have a specific active T-cell response that was severely vaccination with P4-7 subfractions in the hamster transcripts of impededininfectedunvaccinatedandBCGvaccinatedhamsters. iNOS, IL-12 and IFN-(cid:2) showed manifold increase and the syner- The generation of NO in these cultures also support the view gismofIL-12withIFN-(cid:2)mighthaveanadditionalparamounteffect S.Kumarietal./Vaccine26(2008)5700–5711 5709 onleishmanicidalactivitiesofL.donovani[30].Wefoundthatsig- Theoretically,linkingtheabovestatedantigenicproteinsmight nificant iNOS transcript production in P4-7 vaccinated hamsters increase the number of epitopes available for inducing Th1-type correlatedproportionallywithNOgenerationthatwasconsider- immune responses and protective immunity in a heterogeneous ably higher with SLD stimulation. Possibly the cumulative effect human population with diverse major histocompatibility com- of IFN-(cid:2) and IL-12 alongwith iNOS mediated the parasite killing plextypes.Thus,thisclearlyindicatethatwhileidentificationof [30,51,57,58]. The levels of Th-2 cytokines IL-4, IL-10 and TGF-(cid:4) antigens recognized by T cell is an important step in defining a mRNA, on the other hand, were observed to be down-regulated protective immunogens, empirical immunization studies in vac- inthevaccinatedhamsters.ThestrongpresenceofIL-4,IL-10and cinemodelsarecrucialindefiningaleishmanialvaccine,therefore, TGF-(cid:4)ininfectedhamstersarereportedtobethemajorimmuno- emphasizingthatasuccessfulsubunitvaccinemayrequiremultiple suppressivecytokinesinexperimentalandhumanVL[44,58–62]. immunogenic/Th1immunostimulatoryproteinsthatarealsopro- Apartfromdiminishedcellularresponses,VLisassociatedwith tectiveagainstVL.Extendedstudiessuchascloningandexpression theproductionofhighlevelofantibody,observedpriortodetection ofthebestantigenictargets,asdeterminedbytheirimmunoprotec- ofparasite-specificT-cellresponse[4].Unlikeinmice,whereinIL-4 tivepotential,togetherwiththeirspecificassociationanddefinite andIL-12,IFN-(cid:2),thetwocytokinesthatdirectIgGclassswitching allocationarerequiredtocharacterizethesenewproteinsfurther. ofIgG1andIgG2a,respectively,therearenosuchdistinctclassi- ficationsofIgGinhamsters[30].ItisbelievedthathamsterIgG2 Acknowledgements correspondstomouseIgG2a/IgG2bandhamsterIgG1corresponds tomurineIgG1[30].Ithasbeenwell-establishedthattheincrease We express our sincere gratitude to the Directors CDRI and ofIgGandIgG1antibodiestitreisindicativeoftheL.donovaniload CIMAP for their keen interest and for providing facilities for the [30]. These antibodies were quiet low in P4-7 vaccinated group experiments. Our grateful acknowledgement is due to Dr. Nikhil which reflected the decreased parasite burden. In contrast, the Kumar,forcriticallyreviewingthemanuscriptandforhisencour- levelofIgG2significantlyincreasedonlyinP4-7vaccinatedanimals agingsuggestions.WearealsothankfultoDrRajeevSingh,Scientist furthersupporttheviewsthatprotectionagainstleishmaniasisis and Mr. Malaya Sahoo, research fellow for their kind support. inducedbyastrongT-cellresponseandthispatternwasalsoseen Financial support to this work from DBT, New Delhi and for inclinicalaswellasexperimentalVL[4,28,30,49,63–65]. SeniorResearchFellowshiptoMsSKandMr.MSfromCSIR,New To examine the molecular basis of the immune responses Delhi is gratefully acknowledged. This has CDRI communication elicited during Leishmania infection, recent efforts have been no7555. focused on evaluating responses to defined parasite T-cell epi- topesasvaccinetargetsusingproteomicsapproaches[33].Since MALDI-TOF/MS-MSisaverypowerfulanalyzingtoolwhichmay References pinpointallthespecificproteinscontainedinafraction[32],we [1] HandmanE.Leishmaniasis:currentstatusofvaccinedevelopment.ClinMicro- havedonethecharacterizationoffourpotentsubfractionsbyusing biolRev2001;14(2):229–43. this tool. Interestingly, all that proteins that we have identified [2] Desjeux P. Leishmaniasis: current situation and new perspectives. Comp through2DandMALDIanalysisearlier(ref)werefoundtobesim- ImmunolMicrobiolInfectDis2004;27(5):305–18. [3] MurrayHW,HariprashadJ,CoffmanRL.BehaviorofvisceralLeishmaniadono- ilartothoseidentifiedthroughoneDanalysisofF2subfractions vaniinanexperimentallyinducedThelpercell2(Th2)-associatedresponse [33]. Out of total 19 identified proteins, major immunostimula- model.JExpMed1997;185(5):867–74. torywereElongationfactor-2,Aldolase,EnolaseandHSP-70that [4] BhowmickS,RavindranR,AliN.Leishmanialantigensinliposomespromote protectiveimmunityandprovideimmunotherapyagainstvisceralleishmani- were present in all the four subfractions (Table 2) and detailed asisviapolarizedTh1response.Vaccine2007;25:6544–56. immunogenicinformationwasdescribedbyGuptaetal.[33].Pro- [5] ReedSG,ScottP.T-cellandcytokineresponsesinleishmaniasis.CurrOpin tein Disulfideisomerase, p45, HSP-83, TPI and Calreticulin were Immunol1993;5(4):524–31. absentinF2.4subfraction.Perhapsduetothismoderateprotective [6] SkeikyYA,KennedyM,KaufmanD,BorgesMM,GuderianJA,SchollerJK,etal. LeIF:arecombinantLeishmaniaproteinthatinducesanIL-12-mediatedTh1 responsewithanindividualF2.4subfractionwasnoticed.Further cytokineprofile.JImmunol1998;161(11):6171–9. explanationforlowsuccessrateofsubunitvaccineisperhapsdue [7] ColerRN,SkeikyYA,BernardsK,GreesonK,CarterD,CornellisonCD,etal. tothefactthatsomepolypeptidesmaybeslightlyimmunogenic ImmunizationwithapolyproteinvaccineconsistingoftheT-Cellantigens thiol-specificantioxidant,Leishmaniamajorstress-inducibleprotein1,and andmayprovideonlypartialprotectionindividuallybuttheymay Leishmaniaelongationinitiationfactorprotectsagainstleishmaniasis.Infect be excellent in a cocktail vaccine [66–70] as has been observed Immun2002;70(8):4215–25. with P4-7 subfraction. Some of the proteins such as Aldolase, [8] MullerI,FruthU,LouisJA.Immunobiologyofexperimentalleishmaniasis.Med MicrobiolImmunol1992;181(1):1–12. Enolase, and TPI the glycolytic enzymes, may be considered as [9] ModabberF.Developmentofvaccinesagainstleishmaniasis.ScandJInfectDis potentialvaccinecandidates,sincetheyhavebeenreportedtobe Suppl1990;76:72–8. immunogenicinotherorganisms[71–76].Amongtheothermajor [10] ColerRN,GotoY,BogatzkiL,RamanV,ReedSG.Leish-111f,arecombinant polyproteinvaccinethatprotectsagainstvisceralleishmaniasisbytheelici- identifiedimmunostimulatoryproteinsHSPs70and83/90arethe tationofCD4+Tcells.InfectImmun2007. outcomeofthestressresponse,participatinginalargenumberof [11] KamilAA,KhalilEA,MusaAM,ModabberF,MukhtarMM,IbrahimME,etal. immunologicalpathways[33,77–81].Elongationfactors-2andp45 Alum-precipitatedautoclavedLeishmaniamajorplusbacilleCalmette-Guerrin, acandidatevaccineforvisceralleishmaniasis:safety,skin-delayedtypehyper- arereportedtoinduceproliferativeresponseincuredCLpatients sensitivityresponseanddosefindinginhealthyvolunteers.TransRSocTrop PBMCsaswellasleishmanialparasite-specificT-celllinesderived MedHyg2003;97(3):365–8. fromanimmunedonor[33,82].Calreticulin,astressshockprotein [12] KhalilEA,AyedNB,MusaAM,IbrahimME,MukhtarMM,ZijlstraEE,etal. and identified as Th1-stimulatory, is an important multifunc- Dichotomyofprotectivecellularimmuneresponsestohumanvisceralleish- maniasis.ClinExpImmunol2005;140(2):349–53. tional immunodominant calcium (Ca+2)-binding protein [33,83]. [13] LemesreJL,HolzmullerP,GoncalvesRB,BourdoiseauG,HugnetC,Cavaleyra Anotherprotein—ProteinDisulfideIsomerase(LmPDI),responsible M,etal.Long-lastingprotectionagainstcaninevisceralleishmaniasisusing forvirulencefactor[84],isbelievedtorepresentsanewpotential theLiESAp-MDPvaccineinendemicareasofFrance:double-blindrandomised efficacyfieldtrial.Vaccine2007;25(21):4223–34. componentofnovelimmunogenicorvaccinepreparationsaimedat [14] Borja-CabreraGP,CorreiaPontesNN,daSilvaVO,ParaguaideSouzaE,Santos conferringimmunityinhumansoranimalsagainstLeishmania[85]. WR,GomesEM,etal.Longlastingprotectionagainstcaninekala-azarusing Remarkably, the study also documents completely unknown or theFML-QuilAsaponinvaccineinanendemicareaofBrazil(SãoGonc¸alodo Amarante,RN).Vaccine2002;20(27–28):3277–84. hypotheticalproteinsoftheparasite,whichmayrepresentpoten- [15] Palatnik-de-SousaCB.Vaccinesforleishmaniasisintheforecoming25years. tialtargetsforputativevaccinecandidates. Vaccine2008;26(14):1709–24.