Patent Application: US-201314376234-A

Abstract:
the present invention is based upon the identification of a number of antigens derived from species of the genus teladorsagia , which can be used to raise immune responses in animals — particularly those animals susceptible or predisposed to infection by one or more teladorsagia species . the antigens may be exploited to provide compositions and vaccines for raising protective immune responses in animals — the protective immune responses serving to reduce , prevent , treat or eliminate teladorsagia infections / infestations .

Description:
the present invention will now be described in detail with reference to the following figures which show : fig1 : effects of immunization of sheep with recombinant antigens derived from teladorsagia circumcincta on faecal worm egg counts ( fwec ) after challenge infection . panels a and c : fwecs of sheep challenged with 2000 t . circumcincta three times per week for 4 weeks following immunization with an 8 - protein cocktail in the context of quil a ( dashed line ) or with quil a only ( solid line ). each data point represents the arithmetic mean fwec ± sem . panel a represents data from trial 1 ; panel c represents data from trial 2 . panels b and d show cumulative fwecs , for each animal in each group in trial 1 ( panel b ) and trial 2 ( panel d ). “ imm ” represents sheep immunized with the 8 - protein cocktail ; “ con ” represents those administered with quil a adjuvant only . note that , in panel d , for groups 1 and 2 in trial 2 , cumulative fwec is calculated over 84 days , whereas for groups 3 and 4 cumulative fwec is calculated over 112 days . one “ outlier ” animal in group 1 of trial 2 , sheep number 675j , is indicated . fig2 . trial 1 : lumenal t . circumcincta burdens of sheep in group 1 and group 2 . each data point represents the mean number (± sem ) of t . circumcincta enumerated in lumenal contents of seven sheep in each group . panel a depicts counts categorised into developmental stage and the gender of the adult worms harvested . panel b depicts the counts as overall burdens ( all stages and genders ). “*” denotes a significant difference between the means ( p & lt ; 0 . 05 ), “**” denotes a highly significant difference between mean ( p & lt ; 0 . 01 ). fig3 . trial 1 : mucosal t . circumcincta burdens of sheep in group 1 and group 2 . each data point represents the mean number (± sem ) of nematodes harvested from the mucosal contents of seven sheep in each group . “*” denotes a significant difference between the means ( p & lt ; 0 . 05 ). fig4 : effects of immunization of sheep with recombinant antigens derived from teladorsagia circumcincta on abomasal nematode burden after challenge infection ( trial 1 ). panels a - c represent the number of t . circumcincta enumerated in the abomasum . panel a depicts the total nematode burden , panel b the adult nematode burden and panel c the juvenile nematode burden of each of seven sheep in group 1 ( immunized ) or group 2 ( control , adjuvant only ). horizontal bars represent the mean value . fig5 : weight gain of sheep in group 1 and group 2 from day 0 to day 84 of the experiment ( trial 1 ). fig6 : effects of immunization of sheep with recombinant antigens derived from teladorsagia circumcincta on juvenile nematode burden distribution after challenge infection ( trial 2 ; group 1 and group 2 ). numbers of juvenile t . circumcincta enumerated in the abomasal lumen and the abomasal mucosa of each of these sheep are shown . “ imm ” represents sheep immunized with the 8 - protein cocktail ; “ con ” represents those immunized with quil a adjuvant only . fig7 : effects of immunization of sheep with recombinant antigens derived from teladorsagia circumcincta on abomasal nematode burden after challenge infection ( trial 2 ; group 3 and group 4 ). data shown represent the total numbers of t . circumcincta enumerated in the abomasum of each of seven sheep in group 3 ( immunized ) or group 4 ( control , adjuvant only ). fig8 : serum antibody responses of sheep to the recombinant proteins used to immunize group 1 in trial 1 . each data point represents the mean value derived from 7 sheep . standard errors in panels a and b have been omitted to aid interpretation . panels a and b show serum antibody responses for vaccinated sheep ( group 1 ). panel a shows data for igg , panel b shows data for iga . “ imm ” represents dates on which sheep were immunized ; “ trick ” represents the trickle infection ; “ pm ” is the post mortem date . fig9 : serum antibody responses of sheep to the recombinant proteins used to immunize groups 1 and 3 in trial 2 . each data point represents the mean value derived from 14 sheep until day 84 , after which each data point represents the mean of 7 sheep necropsied later in the trial . standard errors have been omitted to aid interpretation . panel a shows data for igg , panel b shows data for iga . “ imm ” represents dates on which sheep were immunized ; “ trick ” represents the trickle infection ; “ pm ” is the post - mortem date . fig1 : serum antibody responses of sheep to l4 excretory / secretory products of teladorsagia circumcincta . ‘ imm ’ represents the days on which animals were immunized with recombinant antigen cocktail ( immunized group ) or adjuvant only ( control group ). fig1 : immunoblots to investigate serum igg ( panel a ) and iga ( panel b ) binding to components of somatic extracts and excretory / secretory products of teladorsagia circumcincta . lanes 1 and 5 contain l3 somatic extract , lanes 2 and 6 contain l4 somatic extract , lanes 3 and 7 contain l4 es material and lanes 4 and 8 contain adult somatic extract . blots were incubated with sera pooled from 7 immunized sheep ( lanes 1 - 4 , sheep from group 3 , trial 2 ) or non - immunized sheep ( lanes 5 - 8 , sheep from group 4 , trial 2 ). sera had been collected from the animals on the date of the third immunization immediately prior to the initiation of trickle infection . * represents molecular mass ( kda ). fig1 : serum igg responses of control , adjuvant only recipients to recombinant tci - mep - 1 and tci - apy - 1 . each data point represents the mean value (± sem ) derived from 7 ( trial 1 , panel a ) or 14 ( trial 2 , panel b ) sheep until day 84 , after which each data point represents the mean of 7 sheep in trial 2 . fig1 : mucosal antibody titres to the recombinant proteins used to immunize sheep in trial 1 . each bar represents the mean value derived from 7 sheep (± sem ). panel a shows data for igg , panel b shows data for iga . asterisks indicate mean values which are statistically significantly higher than those for the remaining antigens within the same treatment group . fig1 : mucosal antibody titres to the recombinant proteins used to immunize sheep in trial 2 . each bar represents the mean value derived from 7 sheep (± sem ). panel a shows data for igg , panel b shows data for iga . asterisks indicate mean values which are statistically significantly higher than those for the remaining antigens within that group . fig1 : mucosal antibody levels to the recombinant proteins used to immunize sheep in trials 1 and 2 . panels a and b show data for igg , panels c and d show data for iga . all graphs show correlation biplots jointly representing sheep ( points ) and their antigen - specific antibody responses ( axes ). the arrows indicate directions of higher antigen - specific antibody response . the orthogonal projection of points onto each axis approximates the relative responses by sheep . the correlations between responses to specific antigens are represented by the angle between the corresponding vectors for each antigen . open circles represent immunized sheep , closed circles represent control , non - immunized sheep . in trial 2 ( panels b and d ), blue circles and pink circles represent groups 1 and 3 ( immunized ) respectively . green and orange circles represent control group 2 and 4 respectively . eight recombinant proteins were used in combination to immunise 6 month - old lambs . details of these proteins are given in table 1 . three proteins , macrophage migration inhibitory factor - 1 ( tci - mif - 1 ), calcium - dependent apyrase - 1 ( tci - apy - 1 ) and a tgf6 homologue ( tci - tgh - 2 ) were selected because of their putative immunoregulatory function ( mcsorley et al ., 2009 ; nisbet et al ., 2010a ; nisbet et al ., 2011 ). the remaining five proteins were selected using a combined immunoscreening / proteomics approach : cathepsin f - 1 ( tci - cf - 1 ), astacin - like metalloproteinase - 1 ( tci - mep - 1 ), a 20 kda protein of unknown function ( tci - es20 ) and activation - associated secretory protein - 1 ( tci - asp - 1 ) ( redmond et al ., 2006 ; smith et al ., 2009 ; nisbet et al ., 2010b ). a final protein was chosen because of its homology to known vaccine candidate antigens of other parasitic nematodes . this protein is known as surface - associated antigen ( tci - saa - 1 , nisbet et al ., 2009 ). cloning and sequencing of the cdna encoding tci - saa - 1 , tci - mif - 1 and tci - apy - 1 and production of recombinant versions of each of these proteins in a bacterial expression system have been described previously ( nisbet et al ., 2009 ; nisbet et al ., 2010a ; nisbet et al ., 2011 ). identical production and purification parameters were employed in the current study . for tci - mep - 1 , oligonucleotide primers for use in the rapid amplification of cdna ends ( race ) were designed from the est sequence cb036707 and race performed using the smart ™ race kit ( clontech ) according to the manufacturer &# 39 ; s instructions , using total rna extracted from l4 stage t . circumcincta ( prepared as described in nisbet et al ., 2008 ) as a template . amplification of the full coding sequence ( cds ) of tci - mep - 1 was performed using oligonucleotide primers incorporating the initiation and termination codons from the contigs generated by 5 ′ and 3 ′ race , cdna generated from l4 as template ( prepared as described in redmond et al ., 2006 ) and the advantage ® 2 pcr kit ( clontech ) according to the manufacturer &# 39 ; s instructions . following confirmatory sequencing , oligonucleotide primers were designed to amplify the cds of tci - mep - 1 , omitting the sequence encoding the signal peptide ( bases 1 - 48 of the cds ) and the termination codon . using these primers , plasmid containing the full - length cds as a template and the advantage ® 2 pcr kit ( clontech ), tci - mep - 1 was amplified and sub - cloned into the expression vector pet sumo ( invitrogen ). the resulting plasmid was used to transform escherichia coli bl21 - codonplus ® ( de3 )- ril competent cells ( stratagene ). recombinant protein expression was induced in the presence of 1 mm isopropyl β - d - 1 - thiogalactopyranoside ( iptg ). insoluble recombinant tci - mep - 1 was purified from inclusion bodies solubilised in 8m urea , followed by nickel column affinity chromatography using histrap ™ hp columns ( ge healthcare ) and a step - wise imidazole gradient in the presence of 8m urea in 20 mm phosphate buffer , ph 7 . 6 . purified tci - mep - 1 was then dialysed against 2m urea in 20 mm phosphate buffer , ph 7 . 6 . the full cds of the cdna encoding tci - tgh - 2 ( accession number fj410914 ) was amplified by pcr using oligonucleotide primers incorporating the initiation codon , but omitting the termination codon . plasmid containing the full cds in a cloning vector was used as a template ( kindly supplied by prof rick maizels , university of edinburgh ) and the advantage ® 2 pcr kit ( clontech ) was employed according to the manufacturer &# 39 ; s instructions . tci - tgh - 2 was sub - cloned into the expression vector pet sumo ( invitrogen ) and recombinant protein expression performed as described above . soluble recombinant tci - tgh - 2 was purified from cell lysates by nickel column affinity chromatography using histrap ™ hp columns ( ge healthcare ). next , rtci - tgh - 2 was eluted in 500 mm imidazole , 20 mm phosphate buffer , ph 7 . 6 and then dialysed against 20 mm phosphate buffer , ph 7 . 6 at rt for 3 hrs . sub - cloning of the cds of tci - asp - 1 ( after removal of the bases encoding the signal peptide ) from a pet22b (+) vector ( described in nisbet et al ., 2010b ) into pet sumo , using the conditions outlined above for tci - tgh - 2 , permitted the expression of soluble recombinant tci - asp - 1 which was expressed and then purified by nickel column affinity chromatography as described , above , for tci - tgh - 2 . for the expression of tci - cf - 1 protein , oligonucleotide primers were designed to amplify the cds of tci - cf - 1 , omitting the sequence encoding the signal peptide ( bases 1 - 42 of the cds ) and the termination codon . using these primers , cdna generated from l4 as template ( prepared as described in redmond et al ., 2006 ) and the advantage ® 2 pcr kit ( clontech ), tci - cf - 1 was sub - cloned into the vector ppiczac ( invitrogen ) and used to transform the yeast pichia pastoris [ x - 33 mut + strain ( invitrogen )] following linearisation with pmei ( new england biolabs ). recombinant protein expression was induced in the presence of 0 . 5 % methanol , as described in nisbet et al . ( 2007 ) and soluble recombinant tci - cf - 1 was purified from culture supernatant by nickel column affinity chromatography as described above for tci - tgh - 2 . tci - es20 , a homologue of a 20 kda excretory / secretory ( es ) protein of ostertagia ostertagi , was identified during an immunoscreening / proteomic analysis of immunogenic t . circumcincta es molecules ( smith et al ., 2009 ). the complete coding sequence was determined by obtaining the putative full - length cdna via polymerase chain reaction ( pcr ) amplification from a cdna library . this smart ™ cdna library was constructed [ using t . circumcincta l4 ( 8 days post infection , dpi ) rna ] in xtriplex2 by long - distance pcr following manufacturer &# 39 ; s instructions ( clontech ). it was packaged using gigapack gold iii packaging extract ( stratagene ) and amplified in e . coli xl1 - blue cells ( stratagene ). a gene - specific oligonucleotide primer ( incorporating the putative termination codon identified from est cb043664 ) was used in conjunction with a vector - specific primer to amplify the tci - es20 cds directly from a heat - denatured phage lysate preparation of the library . the resultant amplicon was column - purified ( qiaquick ® pcr purification kit , qiagen ) and ligated into pgem ®- t ( promega ). constructs were transformed into e . coli jm109 ( promega ), colonies with tci - es20 - containing plasmids were isolated and propagated and the plasmids subjected to automated sequencing ( eurofins mwg operon ). the cdna encoding tci - es20 was then subcloned into the vector ppiczac ( invitrogen ) and used to transform p . pastoris [ x - 33 ( mut +) strain ( invitrogen )] following linearisation with pmei ( new england biolabs ). recombinant protein expression and purification were as described , above , for tci - cf - 1 . protein concentrations were determined using the pierce bca ™ ( bicinchoninic acid ) assay ( thermo scientific ) with bovine serum albumin ( bsa ) standards and stability and integrity of each recombinant protein were monitored using sds - page . tci - mif - 1 ; tci - apy - 1 ; tci - saa - 1 ; tci - cf - 1 ; tci - es20 and tci - mep - 1 were stored in solution at + 4 ° c . and tci - asp - 1 and tci - tgh - 2 were stored at − 20 ° c . ** tci - cf - 1 is highly polymorphic , the clone used for vaccine production had following amino acid substitutions compared to published sequence . in each case the amino acid in the published sequence is in italics , that in the vaccine isoform sequence is in normal font and the amino acid position in the published sequence is in subscript : i 44 t 44 , n 101 d 101 , t 129 a 129 , r 137 q 137 , r 305 k 305 , l 306 p 306 , s 307 y 307 *** full length sequences not yet deposited . these molecules have been derived from est data in the public domain : tci - es20 based on cb043664 , tci - mep - 1 based on cb036707 fourteen , texel crossbred male / female sheep which had been raised in conditions to minimise helminth infection risk , were housed in two groups of 7 animals in separate pens within the same building . the sheep were 204 - 206 days old at the initiation of the experiment . faecal egg counts ( fec , christie and jackson 1982 ), performed prior to initiation of the experiment , confirmed that all animals had negative fecs . sheep in group 1 were immunised by subcutaneous injection using a 400 μg recombinant protein mix ( incorporating 50 μg each tci - asp - 1 ; tci - mif - 1 ; tci - tgh - 2 ; tci - apy - 1 ; tci - saa - 1 ; tci - cf - 1 ; tci - es20 ; tci - mep - 1 in pbs ) plus 5 mg total quil a ( brenntag biosector ). seven of the 8 recombinant proteins were pbs - soluble and were administered as a mixture in a single injection with 2 . 5 mg quil a . tci - mep - 1 was insoluble in pbs and was therefore formulated with 100 mm urea in pbs plus 2 . 5 mg quil a . the two preparations were injected subcutaneously , one immediately following the other , at two sites on the neck of each sheep . each sheep received three immunisations of the recombinant protein mix with an interval of 3 weeks between each immunisation . sheep in the control group ( group 2 ) each received three immunisations with urea / pbs / quil a only , at the same time as the sheep in group 1 . on the day of the third immunisation , an oral trickle challenge was initiated whereby each sheep in both groups was administered with 2000 t . circumcincta l3 . this was continued three times per week ( monday , wednesday and friday ) for 4 weeks . blood samples were taken prior to each immunisation and weekly samples taken from the day of the third immunisation onwards to determine antigen - specific serum iga and igg responses and serum pepsinogen levels ( lawton et al ., 1996 ). fecs were performed ( christie and jackson 1982 ) three times per week ( monday , wednesday and friday ) from 14 days after the start of the trickle challenge until the end of the experiment 5 weeks later . all sheep were weighed weekly . for both groups , abomasal swab samples were collected at post - mortem ( smith et al ., 2009 ) to determine levels of antigen - specific iga and igg antibody at the abomasal mucosal surface . at necropsy , lumenal and mucosal nematode burdens ( adult and larval parasites ) were enumerated following standard techniques . the percentage of stunted or “ inhibited ” larvae was determined , based on size , as described previously ( halliday et al ., 2010 ). the experiment was performed under the regulations of a uk home office project licence . twenty - eight , texel crossbred male / female sheep were raised as described for trial 1 and were housed in four groups of 7 animals . the sheep were 172 - 178 days old and were not excreting helminth eggs at the start of the experiment . groups 1 and 3 were immunized by subcutaneous injection using the recombinant protein mix exactly as described for trial 1 , with each sheep receiving three immunizations with an interval of 3 weeks between each . sheep in groups 2 and 4 each received three immunizations with urea / pbs / quil a , at the same time as groups 1 and 3 . at the final immunization , the oral trickle challenge commenced in all groups and all biological samples were obtained as described above , for trial 1 . sheep in groups 1 and 2 were euthanized 7 weeks after the start of the infection period ( as for trial 1 ) and those in groups 3 and 4 were euthanized 4 weeks later . for all groups , lumenal and mucosal nematode burdens were enumerated as described for trial 1 . trial 1 and trial 2 were performed under the strict regulations of a uk home office project licence and the experimental design was ratified by the moredun research institute experiments and ethics committee . following initial antibody : antigen titrations to ensure optimisation of the technique , antigen - specific antibody levels in serum and abomasal mucus samples were assessed by elisa . high binding microtitre plates ( greiner bio - one ) were coated overnight at 4 ° c . with 50 μl antigen ( 5 μg ml − 1 in 50 mm carbonate buffer , ph 9 . 6 ). plates were washed six times with wash buffer [ phosphate buffered saline ( pbs ), 0 . 05 % v / v tween - 20 ], then blocked with 5 % soya milk powder in 0 . 5 % ( v / v ) tween 20 in tris buffered saline ( ttbs ), ph 7 . 4 , for 1 h at room temperature . after washing , 50 μl abomasal mucus ( diluted 1 : 4 in ttbs ) from individual animals or 50 μl serum [ diluted at 1 : 10 ( iga ) or 1 : 1000 ( igg ) in ttbs ], were added and incubated for 1 h at room temperature . wells were re - washed and 50 μl horseradish peroxidase - conjugated polyclonal mouse anti sheep / goat igg ( a9452 , sigma ) at 1 : 1000 or 50 μl mouse anti - bovine / ovine iga monoclonal antibody ( serotec , mca628 ) at 1 : 250 in ttbs , were added for 1 h at room temperature . after a further wash , the igg elisa was developed by the addition of 50 μl o - phenylenediamine dihydrochloride substrate ( opd , sigma ) to each well . after 15 min in darkness , the reaction was stopped by addition of 25 μl 2 . 5m h 2 so 4 and od values read at 490 nm . for the iga elisa , 50 μl horseradish peroxidase - conjugated polyclonal rabbit anti - mouse igg ( p0260 , dakocytomation ), at 1 : 1 , 000 were added for 1 h at room temperature prior to a final wash and development with opd as described above . each sample was assayed in triplicate . od values were corrected against a reagent blank and all test plates had a positive and negative serum control to account for plate to plate variation . antigen - specific igg levels in the sera of sheep which had been immunized with the recombinant antigen cocktail , or the non - immunized control sheep , were assessed by elisa . the native antigens used to coat elisa plates were somatic extracts of t . circumcincta l3 , prepared as described previously ( nisbet et al ., 2009 ), along with l4 es products , prepared as described in smith et al ., ( 2009 ). antigen - specific igg levels were assessed in all sera from animals in trial 1 and from four , randomly selected , animals from groups 1 and 2 of trial 2 . all experimental conditions were as described , above , for the determination of recombinant antigen - specific igg levels in serum by elisa . somatic extracts of t . circumcincta l3 , l4 and adult worms , prepared as described previously ( nisbet et al ., 2009 ), along with l4 es products , prepared as described in smith et al ., ( 2009 ), were subjected to immunoblotting using serum , collected on the date of the third ( final ) immunization immediately prior to the initiation of trickle infection , from immunized or non - immunized sheep . immunoblotting , to determine serum igg and iga binding to components of each extract , was performed as described previously ( nisbet et al ., 2009 ) using pools of serum from 7 immunized ( group 3 ) and 7 non - immunized sheep ( group 4 ). a generalised additive mixed modelling ( gamm ) approach was adopted for the analysis of longitudinal fec data . a gamm model on log ( fec + 1 ) was specified with gaussian error structure and identity link function , with group as a fixed effect and animal effects introduced as random . the model included separate smoothing curves to model the nonlinear relationship of the response with time by group and non - homogenous within - group variances were allowed . a first order autoregressive residual correlation structure was incorporated . serum and mucosal antibody responses to individual antigens were modelled using linear mixed models ( lmms ) with group as a fixed effect and animal as a random effect . for serum antibody data , repeated measures over time were modelled by random intercept and slope lmms also including time and its interaction with group as a fixed effect . heterogeneous within - group variances were allowed in all cases . linear contrasts were set up to compare subsets of antigen - specific responses in abomasal mucus at post mortem . in trial 2 , the 28 animals were housed in 4 separate groups ( pens ) of 7 animals for logistical reasons . two groups ( 14 animals ) were immunized ( group 1 and group 3 ), and the other two ( 14 animals ) were used as adjuvant - only controls ( group 2 and group 4 ). pen effects between the two immunized groups ( 1 and 3 ) and between the two adjuvant - only groups ( 2 and 4 ) were tested . no statistically significant pen effects were found for any of the above response types , so groups 1 and 3 were combined and groups 2 and 4 were combined for data modelling . for analysis of worm burden data , generalised linear models ( glms ) were used . data overdispersion was detected and it was generally accounted for by specifying a negative binomial error distribution . where necessary , overdispersion was incorporated using poisson glms correcting the standard errors by specifying the mean and variance relationship . nematode burdens were assessed at post mortem in groups 1 and 2 four weeks before those of groups 3 and 4 , so data were analysed separately . model selection was based on the akaike &# 39 ; s information criterion ( aic ) and likelihood ratio tests ( lrt ) ( akaike , 1974 ). the mixed models were fitted by residual maximum likelihood ( reml ; smouse and kojina , 1972 ). throughout the data analysis some animal measurements were identified as outliers . their influence on parameter estimates was considered in each case . the cook &# 39 ; s distance with a 4 / n cut - off value was used to support decisions in relation to outlying values ( cook , 1977 ). statistically significant terms were determined at the level of 0 . 05 . all statistical analyses were conducted using r version 2 . 13 . trial 1 : fec data is shown in fig1 a and b . sheep in both immunised and control groups began to excrete trichostrongyle type eggs in their faeces from 16 - 19 days after the start of the trickle challenge . in both groups , fecs rose until 23 days after the start of challenge . thereafter , sheep in group 1 excreted substantially fewer eggs than those in group 2 . by the end of the experiment , at day 42 of the trickle challenge , group 1 sheep were producing a mean of 8 . 7 (± 5 . 5 ) eggs per gramme ( epg ) of faeces , whereas sheep in group 2 were producing 107 . 6 (± 50 . 8 ) epg , representing a reduction of 92 % in mean fec at that time - point . reml ( gamm ) analysis identified an overall effect of treatment ( immunization ) ( p = 0 . 003 ) and time ( p & lt ; 0 . 001 ), and a significant treatment × time interaction ( p = 0 . 20 ). the mean cumulative fecs for the duration of the experiment , estimated by taking the sum of all egg counts on each sampling date , were 252 (± 132 ) epg in group 1 and 890 (± 231 ) epg in group 2 , representing an overall mean fec reduction of 72 % in the immunised versus the control group . fec mean cumulative fecs for the duration of the challenge period , calculated using the area under the curve ( auc , taylor et al ., 1997 ) technique were 595 (± 316 ) epg in group 1 and 1975 (± 532 ) epg in group 2 , representing an overall reduction of 70 % in the immunized versus the control ( adjuvant only ) group ( fig1 b ). in trial 2 , sheep began to excrete nematode eggs from 14 - 16 days after challenge ( fig1 c ). at peak egg shedding , on day 86 , mean fecs in the extant immunized group ( group 3 ) were 251 ± 75 epg , whereas in the control group ( group 4 ) they were 908 ± 158 epg , representing a 73 % reduction in mean fec . mean cumulative fecs , calculated using the area under the curve ( auc , taylor et al ., 1997 ) technique , in trial 2 were 4998 (±) 2233 epg in group 1 ( immunized ) and 4127 (±) 803 epg in group 2 ( adjuvant only , fig1 d ). the high mean fecs , and associated sem , in group 1 were attributable to the influence of data from a single outlier animal ( sheep 675j , fig1 d ). influence was assessed using cook &# 39 ; s distance criterion ( cook , 1977 ): 675j was regarded as a “ highly influential ” case ( cook &# 39 ; s distance = 0 . 3129 based on a lmm model ). for groups 3 and 4 , which were necropsied 4 weeks after groups 1 and 2 , mean cumulative fecs were 7005 (±) 681 epg in group 3 ( immunized ) and 16727 (±) 2 , 699 epg in group 4 ( control , adjuvant only ), representing an overall mean fec reduction of 58 % in the immunized versus the control group ( fig1 d ). gamm analysis indicated a statistically - significant effect of immunization ( data from groups 1 and 3 combined vs . groups 2 and 4 combined as detailed in materials and methods ) on fec over the course of the experiment ( p = 0 . 0237 ). abomasal t . circumcincta enumerations were subdivided into lumenal and mucosal burdens . within the lumen , group 1 sheep had significantly fewer adult male ( p = 0 . 004 ) and female t . circumcincta ( p = 0 . 011 , fig2 a ) than was observed in the group 2 sheep . there was no significant difference in parasite gender ratio between the two groups . taking all developmental stages and genders into account ( fig2 b ) group 1 harboured significantly fewer luminal parasites than the sheep in group 2 ( p = 0 . 0037 )— sheep in group 1 had 72 % less nematodes in the abomasal lumen than those in group 2 . within the mucosa , the numbers of adult female worms in group 1 were significantly less than those observed in group 2 ( p = 0 . 016 ) ( fig3 ). there was no significant difference between the numbers of male worms or larval stages enumerated in the mucosa in the two groups , although fewer male worms were enumerated in group 1 sheep and fewer larval stages in group 2 sheep ( fig3 ). trial 1 : supplementary analysis of total worms numbers ( lumenal plus mucosal ) immunized sheep ( group 1 ) harboured 55 % fewer t . circumcincta ( total of adults and larvae ) at necropsy than control , adjuvant only ( group 2 ) sheep ( p = 0 . 011 , fig4 a ). group 1 sheep had statistically - significantly lower mean adult nematode burdens than sheep in group 2 ( 75 % reduction , p = 0 . 0066 , fig4 b ). comparison of juvenile nematode burdens in the abomasum indicated no significant differences between the two groups ( fig4 c ). no significant differences were observed in the length of worms recovered from the different groups ( data not shown ). the average increase in weight from day 0 - day 84 of sheep in group 1 was 2 . 1 kg more than that observed in sheep in group 2 ( p = 0 . 10 ) ( fig5 ). the total abomasal nematode burdens ( adults and larvae ) in immunized sheep were not statistically significantly different to the control , adjuvant only group ( mean total nematode burdens : group 1 ; 6843 ± 1144 , group 2 ; 6250 ± 966 ). when adult nematode burdens and juvenile nematode burdens were analysed separately , the adult nematode burdens in immunized sheep were not statistically significantly different to the control , adjuvant only group . comparison of the juvenile nematode burdens indicated that immunized sheep had fewer juvenile nematodes than control , adjuvant only sheep in the abomasal lumen ( group 1 : 50 ± 42 ; group 2 : 218 ± 81 ), ( fig6 ). because of the preponderance of “ zero ” values in the counts from the immunized sheep , statistical analysis using models was unreliable in this case . conversely , there were more juvenile stages in the abomasal mucosa of group 1 than group 2 ( group 1 : 643 ± 198 ; group 2 : 114 ± 70 ; p = 0 . 0367 , fig6 ). immunised sheep ( group 3 ) harboured 57 % fewer t . circumcincta total nematodes at necropsy than did the control , adjuvant only ( group 4 ) recipients ( p = 0 . 0199 , fig7 ). in both groups 3 and 4 , adult worms comprised 99 % of the total nematode burden and no significant difference in the numbers of juvenile stages was observed between the two groups . in both trials , following tertiary immunization , serum igg levels against all recombinant proteins reached peak levels , which declined slowly thereafter ( fig8 a and 9a ). serum iga levels peaked after secondary immunization and , for all recombinants , with the exception of tci - mif - 1 , levels remained relatively constant until the end of the experiment ( fig8 b and 9b ). following immunization with the recombinant antigens , sheep produced serum igg , prior to parasite challenge , which bound native l4 es components ( fig1 ). the nature of the immunoreactive antigens in this es material , and other t . circumcincta extracts , was investigated further by immunoblotting : igg bound to parasite components , in somatic extracts of l4 and adult t . circumcincta as well as l4 es , of the expected size range for the following vaccine components , tci - cf - 1 ( 23 . 9 kda ), tci - apy - 1 ( 38 . 6 kda ) and tci - mep - 1 ( 55 . 6 kda ) ( fig1 a ). iga also bound parasite components , in somatic extracts of l4 and adult t . circumcincta and l4 es , of the expected size range for the vaccine components , tci - cf - 1 , tci - apy - 1 ( adult only ) and tci - mep - 1 ( fig1 b ). in addition iga bound an unknown parasite component of ca . 43 kda in l3 somatic extract . in both trials 1 and 2 , from 14 days after initiation of challenge , control , adjuvant only recipients generated serum igg that bound recombinant tci - mep - 1 and tci - apy - 1 ( fig1 ). antigen - specific serum iga which bound to the recombinant proteins was not observed in the control , adjuvant only recipients ( data not shown ). in trial 1 and 2 , mean recombinant antigen - specific mucosal igg levels in abomasal mucus of the immunized sheep were significantly higher than in the control , adjuvant only recipients for each protein ( fig1 a and 14a ). in trial 1 , mean tci - apy - 1 -, tci - mep - 1 -, and tci - cf - 1 - specific igg levels were significantly higher than those measured against the other five recombinants ( p & lt ; 0 . 0001 ), whereas in trial 2 , mean tci - mep - 1 - specific igg levels were significantly higher than responses to the remaining antigens ( day 84 necropsy ) while tci - mep - 1 - and tci - apy - 1 - specific igg levels were significantly higher at the day 112 necropsy . a joint biplot representation of animals and antigen - specific mucosal igg responses ( fig1 a and 15b ) illustrates the relationships between treatments , between animals within groups , with respect to igg responses to the different antigens and overall differences between immunized and control , adjuvant only sheep . mucosal tci - apy - 1 - and tci - mep - 1 - specific iga levels were significantly higher than those directed against the other six recombinant antigens in trial 1 and 2 ( fig1 b and 14b ). the overall differences between immunized sheep and adjuvant only recipients are represented in joint biplots of animals and antigen - specific mucosal iga responses in fig1 c and 15d . here , we demonstrated that immunisation of sheep with a cocktail of eight recombinant t . circumcincta proteins results in significant levels of protection in terms of fecs and parasite burdens when compared to challenge control sheep . as far as we are aware , this is the first published report of successful vaccination against this nematode species using a recombinant vaccine . indeed , the levels of protection are higher than observed in any other system using a recombinant vaccine against a parasitic nematode in the definitive ruminant host . the level of protection achieved , in terms of fec and abomasal luminal burden , is similar to the highest reported levels following vaccination with detergent extracts of t . circumcincta l3 ( wedrychowicz et al ., 1992 ; 1995 ). in those experiments immune anti - parasite responses were variable , but parasite burdens were significantly reduced ( by up to 72 %) and fecs were reduced by more than 70 %. the antigens that stimulated protection in the previous trials ( wedrychowicz et al ., 1992 ; 1995 ) were not characterised in detail and their identity remains elusive . other attempts to protect sheep against t . circumcincta using native antigen preparations , for example lectin - binding integral membrane glycoproteins , have not been successful ( smith et al ., 2001 ). this general lack of success in immunisation against t . circumcincta is in contrast to the situation in other , closely related , parasitic nematode species . for example , the closest homologues of tci - asp - 1 , the n - type single domain asps , oo - asp - 1 and oo - asp - 2 , are the principal components of an asp - enriched native extract of adult ostertagia ostertagi which has been used with success in vaccination trials in cattle ( geldhof et al ., 2002 , 2004 ; meyvis et al ., 2007 ). however , vaccination with a recombinant version of oo - asp - 1 has failed to induce either protective immunity or native - antigen specific antibodies in vaccinated calves ( geldhof et al ., 2008 ). this reflects the outcomes of many nematode vaccine trials using recombinant versions of native proteins / complexes where the native molecules show great promise , but where recombinant versions fail to induce protective immunity ( geldhof et al ., 2007 ). this “ pragmatic ” approach to antigen identification , where protective native extracts are identified by an iterative process of fractionation and vaccination and recombinant versions of single ( or multiple e . g . see cachat et al ., 2010 ) protective antigens are produced and tested in vivo , therefore appeared to be of limited value for the development of a vaccine against t . circumcincta . the approach to antigen identification described herein was substantially different to the pragmatic approach , and followed a more targeted approach by attempting to mimic and exploit elements of the natural , successful immune response to t . circumcincta in infected sheep . first , we identified potential vaccine candidate molecules by immunochemical and proteomic analyses ; this was done by screening immunoblots of t . circumcincta es material with iga from infected , immune sheep and comparing these responses to those observed in infected , non - immune sheep or non - infected sheep ( smith et al ., 2009 ). we also identified a homologue of a known protective antigen [ ac - saa - 1 ( zhan et al ., 2004 )] using bioinformatic analysis of stage - specific cdna libraries ( nisbet et al ., 2008 ; 2009 ). finally , using a combination of these technologies , we identified a suite of potentially immunosuppressive molecules produced by the parasite ( mcsorley et al ., 2010 , nisbet et al ., 2010a ; 2011 ). we produced recombinant versions of each of these molecules , examined that they were targets of iga present in mucus derived from immune sheep and then combined them into a multi - component vaccine which aimed to provoke the host immune system to respond to potentially immunostimulatory molecules ( tci - cf - 1 , tci - mep - 1 , tci - es20 , tci - asp - 1 and tci - saa - 1 ) and to produce a possible neutralising effect on putatively immunosuppressive components . the rationale behind using a combination of recombinant molecules , as opposed to single antigens , is as follows : previous vaccination trials using single recombinant antigen preparations of homologues of some of the molecules described herein , in different nematode / host models , have failed . in o . ostertagi , for example , the astacin - like metalloproteinase met - 1 , which shares & gt ; 50 % amino acid identity with tci - mep - 1 , was selected by immunoscreening but failed to give any protection when used as a single recombinant antigen in a vaccine trial ( de maere et al ., 2005 ). similarly , recombinant oo - asp1 , which shares & gt ; 75 % sequence identity with tci - asp - 1 ( nisbet et al ., 2010b ), has failed to induce protective immunity in vaccinated calves ( geldhof et al ., 2008 ) and a recombinant version of the necator americanus orthologue of tci - saa - 1 ( na - saa - 1 , 71 % amino acid identity ) failed to induce significant protection against l3 challenge in a hamster model ( xiao et al ., 2008 ). the mechanism of action of the vaccine used herein is not yet clear . these nematodes are acquired by ingestion of l3 from pasture . thereafter , the developing parasites ( l3 and l4 ) and adult worms reside in the host &# 39 ; s abomasum . protective immunity against t . circumcincta in sheep exposed to continuous field or experimental trickle challenge has been associated with decreased larval establishment ( l3 ) and development ( l3 and l4 ) in the mucosa and reduced egg output from female worms in the lumen ( balic et al ., 2003 ; seaton et al ., 1989 ; smith et al ., 1985 , 1986 ; stear et al ., 2004 ). in the current study , in trial 2 , adult worm burdens in vaccinated and adjuvant only groups were similar at day 84 , so it seems unlikely that exclusion and expulsion of incoming l3 or death / delayed development of l4 worms was responsible for the observed reduction in adult parasite numbers at day 112 of that trial . the reduction in the numbers of adult worms may therefore be ascribed to either a direct effect anti - parasitic effect of the induced immune response against the adult worms or a cumulative fitness - reducing effect throughout the life of the worm , culminating in the lower level , or shorter duration , of adult survival . the immune mechanisms responsible for the observed effects on the parasites are likely to be complex : in naturally - acquired immunity to t . circumcincta in sheep roles for immediate hypersensitivity reactions and for larval antigen - specific iga in gastric secretions have been indicated ( smith et al ., 1986 ; 1987 ; stear et al ., 1995 ; 1999 ; halliday et al ., 2007 ; smith et al . 2009 ). cellular effectors of the immune response , e . g . γδtcr + t cells , cd4 + t cells , eosinophils , globular leukocytes and mast cells may also play a role in immunity against t . circumcincta in naturally - or experimentally - exposed sheep ( e . g . stear et al ., 2002 ; 2009 , balic et al ., 2003 ; halliday et al ., 2010 , williams 2012 ). in conclusion , we have developed a multi - component vaccine against t . circumcincta which , in experimental circumstances , reduced mean fecs and mean luminal parasite burdens by & gt ; 70 %. it should be noted that , according to barnes et al ., ( 1995 ) it is not essential for a vaccine against parasitic nematodes to be 100 % effective in sheep , and “ substantial benefits ” can be gained by using a vaccine that is 60 % effective in 80 % of the flock , if the vaccine is based on the stimulation of ‘ natural immunity ’. on this basis , the results of this study would clearly indicate that the vaccine used here holds much potential . it is not yet clear whether all of the eight recombinant protein components of the vaccine are required for this level of efficacy and further work will seek to clarify this and also to confirm the anti - parasite effects of the 8 - protein cocktail vaccine . balic , a ., bowles , v . m ., liu , y . s . & amp ; meeusen , e . n . local immune responses in sensitized sheep following challenge infection with teladorsagia circumcincta . parasite immunol . 25 , 371 - 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