Title of Invention | NEMATODE LARVAL SURFACE ANTIGEN |
---|---|
Abstract | An isolated monoclonal antibody mAb PAB-1, deposited at ATCC on 24 Janaury 2002 and accorded accession PTA-4005, which binds to a surface antigen on nematodelL3, wherein the antigen runs substantially between 20-35 kDa or at substantially 9 kDa and 12kDa on SDS PAGE gel reducing conditions. |
Full Text | NOVEL MONOCLONAL ANTIBODY AND NEMATODE LARVAL ANTIGENS Technical Field The present invention relates to a monoclonal antibody and nematode larval antigens. In particular the present invention relates to a monoclonal antibody specific for surface antigens on third stage larvae (L3) of parasitic nematodes. Background Art The infestations by nematode parasites of animals such as sheep and cattle are of economic importance to those in the agriculture industry. Traditionally, nematode infection has been treated by the administration of anthelmintics. However, a major drawback with conventional anthelmintics is that nematode resistance to a broad spectrum of anthelmintics is now becoming increasingly more widespread and is therefore of serious concern (Waller, 1997; Sangster et al, 1999; Van Wyketal, 1999) A number of mechanisms have been proposed to explain expulsion of nematodes from the intestine of immune sheep (Rothwell 1989). There is evidence for the involvement of elements of an immediate hypersensitivity response, where antigenic stimulation of IgE-sensitised mucosal mast cells leads to an accumulation of substances in mucus which may affect nematode survival (Miller 1996; Emery et al 1997). Anti-nematode properties of mucus include the presence of chemical mediators (Douch et al 1983; Jones et al 1990) and antibody (Lee & Ogilvy I9S1; Miller 1987; Carlisle et al 1991). Recently, the present inventors showed that intestinal mucus obtained from sheep immunised by multiple truncated infections could alter the normal pattern of larval establishment after incision of a mixture of larvae and mucus into the duodenum of naive recipient sheep (Harrison et al 1999). Mucus collected from the small intestine of sheep immune to the parasitic nematode Trichostrongylus colubriformis was found to have anti-larval activity, causing larvae to clump in vitro and resulting in significant reduction of numbers of larvae establishing in naive sheep after infusion of larvae and mucus via a duodenal canola. Immunoblotting showed that immune mucus contained IgG and IgA antibodies that recognised predominantly an antigen with an estimated molecular weight of 35 kDa, Antibodies eluted from the surface of larvae incubated in immune mucus also reacted with the 35 kDa antigen on blots of larval homogenate. Immnunofluonescence and immunogold electron microscopy showed that the 35 kDa antigen was present on the epistyle of L3 and was shed during the molt to L4, The antigen was not present in eggs, LI, L2, L4 or adult worms and was only seen in extracts of L3 before infection and up to 5 days after infection. The results suggest that the binding of antibody to the larval surface prevented larvae from establishing at their preferred site, causing them to be eliminated from the intestine. Lnmunisatioo of sheep with partially purified 35 kDa antigen resulted in a significant reduction of egg count following challenge with T. colubriformis, indicating the potential usefulness of this antigen in a vaccine. A monoclonal antibody designated PAB-1 was prepared against the larval surface antigen. MAb PAB-1 and sheep mucus antibody both recognised the 35 kDa T. colubriformis larval antigen and also cross reacted with an antigen of similar molecular weight on blots of 13 extracts of the parasitic nematodes Haemonchus contorts and Ostertagia circumcincta; and with a 22 kDa antigen on blots of L3 antigens extracted from Coopery cortices and Nematodirus spottier. This indicated that a common surface antigen with immunising potential was present on other nematode species and could be identified by rag PAB-1, The 35 kDa larval antigen and related molecules are likely to be novel targets for host immunity and can thus be utilized in a vaccine or other immunotherapy against nematode infections. Monoclonal antibody PAB-l can be used to immunopurity the surface antigen by standard affinity chromatography techniques. Monoclonal antibody PAB-l coupled to a solid phase support such as agars or sparse beds the surface antigen from a crude extract of L3. The surface antigen can be eluted from the antibody matrix using a low pH buffer and shown to be substantially pure by SDS PAGE. The surface antigen purified in this manner is detected by immunoblotting against sheep antibody from immune mucus and can be stained by methods used for detecting carbohydrates. The 35 kDa larval antigen and related molecules are known to have a predominantly carbohydrate stmbture. This is because the antigen is resistant to digestion by protein’s K: does not stain In gels treated with sensitive protein stains; does stain with carbohydrate stains and can be labeled with carbohydrate labeling reagents such as biotin-hydrazide. Accordingly, mAb PAB-l may be useful in identifying and isolating the surface antigen for development into a vaccine or other immunotherapy against nematode infections. Serum and intestinal mucus from sheep infected with T. colubriformis contains antibody that recognises the 35 kDa larval antigen and related molecules. Accordingly, as the presence of antibody to the larval antigen indicates exposure to the parasite, monoclonal antibody PAB-l may be useful as a diagnostic tool for the identification of infected animals. All references, including any patents or patent applications, cited in this specification are hereby incorporated by reference. No admission is made that any reference constitutes prior art. The discussion of the references states what their authors assert, and the applicants reserve the right to challenge the accuracy and pertinence of the cited documents. It will be clearly understood that, although a number of prior art publications are referred to herein, this reference does not constitute an admission that any of these documents forms part of the common general knowledge in the art, in New Zealand or in any other country. Summary of Invention According to a first aspect of the present invention there is provided an isolated monoclonal antibody mAb PAB-1, deposited at ATCC on 24 Januaiy 2002 and accorded accession PTA-4005, which binds to a surface antigen on nematode L3. According to a second aspect of the present invention there is provided an isolated monoclonal antibody as described above wherein the antibody binds to an antigen sourced from l.colubriformis L3, wherein in said antigen runs at substantially 35kDa on SDS PAGE gel under reducing conditions. According to a third aspect of the present invention there is provided an isolated monoclonal antibody as described above wherein the antibody binds to surface antigens on L3 selected from the group consisting of: a) a siuface antigen on C.curticei which runs at substantially 46 kDa and at substantially 22l£Da on SDS PAGE gel under reducing conditions; b) a surface antigen on N.spathiger which runs at substantially 22kDa on SDS PAGE gel under reducing conditions; c) a surface antigen on H.contortus which runs at substantially 35kDa on SDS PAGE gel under reducing conditions; and d) a surface antigen on O.circumcincta which runs at substantially 35-39kDa on SDS PAGE gel under reducing conditions; e) a surface antigen on T,axei or T.vitrinus which runs at substantially 35kDa on SDS PAGE gel under reducing conditions; f) a surface antigen on O.ostertagi which runs at substantially 30-45 kDa on SDS PAGE gel under reducing conditions; g) a surface antigen on C.oncophera which runs at substantially 20 kDa and at substantially 45 kDa on SDS PAGE gel under reducing conditions; h) a surface antigen on N.brasiliensis which runs at substantially 9 kDA and at substantially 12 kDa on SDS PAGE gel under reducing conditions; i) a surface antigen on Decertify which runs at substantially 30 kDa on SDS PAGE gel under reducing conditions. According to a fourth aspect of the present invention there is provided an isolated monoclonal antibody as described above wherein the antibody when coupled to a solid support can be utilised to purify the surface antigen by immune-affinity chromatography. According to a fifth aspect of the present invention there is provided an isolated carbohydrate surface antigen from a nematode L3, wherein the antigen binds to monoclonal antibody mAb PABl, deposited at ATCC on 24 January 20ft2 and accorded accession PTA-4005. Most preferably Said antigen also resists boiling in 1 M NaOH. According to a sixth aspect of the present invention there is provided an isolated antigen substantially as described above wherein the antigen runs at substantially between 20-35 kDa or at substantially 9 kDa and 12 kDa on SDS PAGE gel under reducing conditions. According to a seventh aspect of the present invention tasks is provided an isolated antigen substantially as described above wherein the antigen is sourced from Tcotubriformis L3. According to an eighth aspect of the present invention there is provided an isolated antigen substantially as described above wherein the antigen is sourced from nematode L3 isolated from the group consisting of C.curticei, N. spathiger, H.contortus, Oxircumcincta, Taxed, T.vitrinus, O.ostertagi, C.oncophera, N.brasiliensis and Decertify. According to a ninth aspect of the present invention there is provided a composition that comprises an antigen substantially as described above together with a pharmaceutically or veterinary acceptable carrier or diluents According to a tenth aspect of the present invention there Is provided the use of an antigen substantially as described above in the manufacture of a composition for preventing, treating, or reducing the susceptibility to, nematode infection. According to an eleventh aspect of the present invention there is provided the use of a composition substantially as described above for preventing, treating, or reducing the susceptibility to, nematode unification in susceptible sheep from nematodes selected from the group consisting of T.colubriformis, Ccurticei, N.spathiger, H.contortus, O.circumcincta T.axei, T.vitrinus, O.ostertagi, C.oncophera, N.brasiliensis and Decker. According to a twelfth aspect of the present Invention there Is provided a composition substantially as described above for preventing, treating, or reducing the susceptibility to, nematode infestation in susceptible animals other than sheep wherein these other species of nematodes also possess a larval surface antigen identified by reaction with monoclonal antibody PAB-1 as described above. Preferably, these other animals, may be any animals susceptible to nematode infection as a foresaid, and may include mice, rats, guinea pigs, rabbits, goats, sheep, horses, pigs, dogs, cats, chickens, cattle, deer or the like. According to a thirteenth aspect of the present invention there is provided a composition substantially as described above wherein the composition also includes at least one adjuvant or cytokine. According to a fourteenth aspect of the present invention there is provided a method of diagnosing nematode infection in susceptible animals comprising the steps of: a) obtaining a blood sample from an animal; and b) analyzing the sample for the presence of an antibody against the antigens described in the third aspect of the invention above via a suitable gassy. Preferably, the assay may be an EUSA or western blotting assay although this should not be seen as limiting as other types of assay are envisioned. According to a fifteenth aspect of the present invention there is provided an isolated antibody substantially as described above wherein the antibody has been sourced from the gastrointestinal mucus of animals which has been immunised by truncated infections with nematodes selected from the group consisting of T.colubriformis, C.curticei, N.spathiger, H.contortus, O.circumcincta T.axei, Tvitrinus, O.ostertagi, C.oncophera, N.brasiliensis and D.eckerti. According to a sbtteenth aspect of the present invention there is provided a method of preventing or treating animal nematode infections, by administering the composition of the present invention. According to a seventeenth aspect of the present invention there is provided the use of an antigen of the present invention to elicit an antibody response in the gut mucus of sheep or other susceptible animals to treat, prevent or reduce susceptibility to, nematode infections in sheep. According to an eighteenth aspect of the present invention there is provided a use for monoclonal antibody substantially as described above to detect nematode infection in sheep. The term "isolated" means that die monoclonal antibody or carbohydrate of the present invention is removed from its original environment and is separated from some or all of the co-ejcisting materials in the natural system from which the antibody or carbohydrate has been obtained. The term "L3" refers to a particular larval stage of development in a nematode life cycle. The terra 35 antigen generally refers, unless context dictates otherwise, to the 7". Colubriformis antigen which runs at substantially this molecular weight. The term "susceptible animal" refers to sheep prone to nematode infection by the following species of nematode T.colubriformis., C.curticei, N.spathiger> H. contorts, O.circwncincta, T.axei, T.vitrinus, O.osiertagi, C.oncophera, N.brasiliensis and D.eckerti or to other animals prone to nematode infection where trios nematodes possess an antigen detected by monoclonal antibody PAB-1 as described. Disclosure of Invention The monoclonal antibody of the present invention is a monoclonal antibody which recognises carbohydrate surface antigens on L3 of parasitic nematodes. The monoclonal antibody has been found by the inventors to have the same specificity as the anti-larval antibody present in intestinal mucus from sheep immunised against The following outlines in general non-limiting terms the procedures for identifying and producing the antibody of the present invention. Sheep prone to nematode infection were raised nematode free from birth till four months old when a set number were immunised by a series of truncated infections with T.colubriformis L3. The remainder of the immunised sheep continued to be raised under nematode free conditions. Preferably the sheep to be used were subjected to 3 truncated infections over a period of time, each infection being terminated after a set time frame. Preferably, the set time frame may be 14 days with re-infection occurring approximately 7 days after termination, although it should be appreciated that these time frames should not be seen as limiting. After termination of the last infection the sheep were slaughtered and mucus was obtained from the small intestine, substantially in accordance with the method of Harrison et al, 1999, although this method should not be seen as limiting, as other methods may also be employed. Mucus from was also taken as outlined above. Once obtained, immune and navel mucus samples were then analyzed for differences in protein profiles, for example by SDS PAGE gel and stoning with Compassion blue or silver. The mucus antibody can then be characterised. Preferably this may be achieved by iimnunoblotting L3 homogenate antigen and probing with immune and knife mucus samples. Antibody binding may be detected by reaction with commercially available antihero raised against sheep immunoglobulins and conjugated with an enzyme. Preferably, the antibody binding may be detected by RAS/IgG-HRP. The L3 homogenate may be prepared by disruption of unsheathed L3 of any of the parasitic nematode species listed herein, using mechanical or chemical means, in the presence or absence of suitable detergents or denaturants, followed by clarification of the extract by centrifugation and/or filtration. Most preferably the L3 homogenate may be prepared by disruption of exsheatiied L3 of T.colubriformis frozen in liquid N2, using a mortar and pestle to grind the frozen L3 until disrupted. Larval components are then extracted into a neutral buffer e.g. 50mM Tris-HCl pH 7.5 containing 1-2% of a solubilising agent such as CHAPS, sodium deoxycholate, urea or SDS. The extract is clarified by centrifugations at 100 000 x g for 1 h or by filtration through a series of membranes with decreasing pore size e.g. 5.0 mm down to 0.2 m. The method for producing the monoclonal antibody mAb PAB-1 may be any suitable method such as that of Kohler and Milstein (1975). For example, the 35fcDa antigen may be excised from polyacrylamide gel slices, macerated and mixed with equal volumes of an incomplete oil adjuvant and then administered to the abdominal cavity, sub cutis, foot)ads or the like of an animal to be immunized such as mouse, rat, guinea pig, rabbit, goat, sheep, horse, pig, dog, cat, chicken, cattle, deer or the like. Among these animals preferably a mouse is used. Antibody producing cells such as spleen cells, lymphocytes or peripheral blood cells may be collected from the immunized animal, and fished with yeoman cells, (a tumor cell strain) to form a hybrid. Spleen cells are preferable as antibody producing cells. The yeoman cells used for the cell fusion are preferably those cell lines allergenic to the immunized animal. However, cell lines of various animals can also be used. Preferably, NS-1 cells may be used as the cells. However, this should not be seen as limiting the scope of the present invention. Though the monoclonal antibody of the present invention is typically an antibody produced by a hybridism, antibody fragments obtained by treating such an antibody with a protease not degrading the antigen-binding site (Fab) such as plantains, pepsin and papa in, i.e., Fab, F(ab')2, Facb and the like, or antibody fragments produced by molecular cloning techniques, are encompassed by the monotone antibody of the present invention, so long as they have the properties of the monoclonal antibody of the present invention. The carbohydrate surface antigen of the present invention is found on the surface of L3 of T.colubriformis, C.curticei, N.spathiger, H. contortus , O.circumcincta, T.axei, Tvitrinus, O.ostertagi, C.oncophera, N.brasiliensis and D.eckerti. The following outlines in general non-limiting terms the procedures for identifying and isolating the carbohydrate antigen of the present invention. The carbohydrate surface antigen of the present invention can be isolated from extracts of L3 of the nematodes listed herein. Preferably, the carbohydrate antigen may be isolated from extracts of T.colubriformis L3 prepared as described above. Monoclonal antibody PAB-1 may be first coupled to a solid phase support medium, preferably Protein A-agrees or Protein G-agarose and covalently linked to prevent antibody leakage from the gel. The gel may then be packed into a chromatography column and L3 extract applied. After washing with a neutral buffer, preferably PBS containing 0.05% Twine 20 to prevent non-specific binding, the bound carbohydrate antigen can be eluted from the column by applying an elution buffer of high or low pH or high salt concentration. Preferably, glycine-HCl buffer pH 2.5-2.8 may be used to elute the antigen. After elution, the pH of the carbohydrate antigen can be raised to neutrality by addition of 1 M tiis. The carbohydrate antigen is then identified by further analysis using electrophoresis and blotting against antibody from immune sheep mucus. The nature of the carbohydrate antigen may be determined by staining with a carfjohydrate detecting silver stain and by labeling on blots with the carbohydrate-binding reagent biotin-hydra2ide. It will be appreciated by those skilled in the art that other carbohydrate detecting methods may also be used. Such methods may include but should not be limited to lection binding, HPLC, TLC, fiuorophore assisted carbohydrate electrophoresis, MS andNMR. Methods and pharmaceutical carriers for preparation of pharmaceutical compositions are well known in the art, as set out in textbooks such as Remington's Pharmaceutical Sciences, 19th Edition, Mack Publishing Company, Easton, Pennsylvania, USA. The compounds, vaccines and compositions of the invention may be administered by any suitable route, and the person skilled in the art will readily be able to determine the most suitable route and dose for the condition to be treated. Dosage will be at the discretion of the attendant physician or veterinarian, and will depend on the nature and state of the condition to be treated, the age and genera! state of health of the subject to be treated, the route of administration, and any previous treatment which may have been administered. The carrier or diluent’s, and other recipients, will depend on the route of administration, and the person skilled in the art will readily be able to determine the most suitable formulation for each particular case. For the purposes of this specification it will be clearly understood that the word "comprising" means "including but not limited to", and that the word "comprises" has a corresponding meaning. Brief Description {tf Drawings Further aspects of the present invention will become parent from the following description which is given by way of example only and with reference to the accompanying drawings in which: Figure 1 Shows the number of larvae in halve sheep after incubating larvae with various amounts of mucus from naive sheep or mucus from immune sheep; Figure 2 Shows the numbers of larvae in naive sheep after incubating larvae with mucus from naive or immune sheep for various times; Figures Shows the number of larvae io proximal and distal sections of naive sheep intestine after infusing naive recipient sheep with mixtures of L3 in naive or immune mucus; Figure 4 Shows the anti-larval activity of immune mucus at various times after immunization; Figures Shows the results of an SDS PAGE analysis of immune and naive mucus; Figure 6 Shows the results of pectin blotting of immune and naives mucus. A: UEA-1 (a-L-fructose). B; JAC (cc-gal-Me-pyrauoside) C: WGA (N-acetylglucosamine) D: UL (mannose, glucose) Figure? Shows the results of pectin blotting of immune and naive mucus. A: PNA (p-galactic-N- acetylgalactosamine) B: EcorA (P-galactose-N- acetylglucosamine) C; SBA (N- acetylgalactosanaine) D: ECA (p-galactose-N- acetylgalactosamine) Figures Shows the results of lectin blotting of immune and naive mucus A: SNA (sialic acid) B: immunoblot probed with RAS/IgG-HRP Figure 9 Shows the results of an immunoblot (^ T.colubnjormis L3 antigen probed with impersonal mucus from immune sheep (lanes 1,5, 10,11, 12 and 19) or naive sheep (lanes 13-18), 100 000 x g simian of immune mucus Oane 3), immune mucus supernatant purified from Protein G-agarose (lanes 4 and 7), antibody eluted from unsheathed T.colubriformis L3 OaiKS 6 and 20), antibody from ammonium caliphate precipitated gut lumen fluids from immune sheep (lanes 8 and 9). Lane 2 shows T.colubriformis 13 proteins stained with colloidal gold. IgG antibody was detected with RAS/O-HRP (lanes 1-18) and IgA was detected with MAS/IgA fooled by RAM/IgG-HRP acnes 19 and 20). Figure 10 Shows the results of T.colubriformis L3 antigen probed with naiVe or immune mucus. Antigen strips were reacted with naive mucus or immune mucus followed by either RAS/IgG; mAB to sheep IgGt; mAB to sheep IgG2; mAB to sheep IgA; mAB to sheep IgM Figure 11 Shows the results of an immvraoblot of T.colubrifortnis 13 antigen, C. cortically antigen and. spathigerLi angst. Figure 12 Shows the results of an immunoblot analysis of extracts from L3 of H.contortus, O.circumcincta, N.spathiger, C.curticei and T.colubriformis. Fipure 13 Shows the coirelation of protection against infection with intestinal mucus IgG and %A antibody titre against T.colubriformis 13 antigen. Figure 14 Shows the decline of IgG and IgA antibody liters in intestinal mucus over time. Figure 15 Shows unsheathed T.colubriformis L3 reacted with immune or naive mucus (top panels) and shows T.colubriformis larvae collected 5 days after infection and reacted with immune mucus (lower panels). Figure 16 Shows electronmicrographs of unsheathed T.colubriformis 13 after reaction with naive (A) or immune mucus (B). Panels C-F show T.colubriformis larvae collected at 2, 3, 4 or 5 days after infection and reacted with immune mucus. Figure 17 Shows the results of SDS PAGE and immunoblotting analysis of T.colubriformis eggs, larvae and adults. Panels A, C and D reacted with immune mucus. Panel B silver stained proteins. Figure 18 Shows the results of SDS PAGE and immunoblotting analysis of T.colubriformis L3 before infection and at various times after infection. Figure 19 Shows the results of an immunoblot analysis of T.colubriformis 13 extracts and proteins K digested 13 extracts reacted with immune mucus or monoclonal antibody PAB-1. Figure 20 Shows an immunoblot analysis of L3 antigen extracts and proteinase K digested 13 extracts from five nematode species reacted with monoclonal antibody PAB-1. Figure 21 Shows surface fluorescence or exstieatbed T.colubriformis L3 reacted with control monoclonal antibody (left and centre panels) or with monoclonal antibody PAB-1 (right panel). Figure 22 Shows analysis of Tc larval surface antigen purified by immuno-affinity chromatography using monoclonal antibody PAB-1. Figure 23 Shows the results of an immunoblot analysis of T.colubriformis L3 extracts after heating, oxidation, digestion or precipitation by organic solvents. Figure 24 Shows the results of an immunoblot analysis of T.colubrtformis L3 extracts after digestion by proteases or lipases. Figure 25 Shows the results of an immunoblot analysis of T.colubriformis L3 extracts after digestion by proteases. Figure 26 Shows the results of an immunoblot analysis of T.colubriformis L3 extracts after digestion by glycosidase. Figure 27 Shows the results of an immunoblot analysis of T.cohibrifoTmis L3 extracts after allcaline degradation. Figure 28 Shows the results of an immunoblot analysis of T.colubriformis L3 extracts after heating and alkaline or acid degradation. Figure 29 Shows the results of an immunoblot analysis of T.colubriformis L3 extracts after heating and alkaline or acid degradation. Figure 30 Shows the results of an immunoblot analysis of T.colubriformis L3 extracts after heating, alkaline degradation or protease digestion. Figure 31 Shows the results of an immunoblot analysis and protein stain of 1 .cotubnformis L3 extracts after electrophoresis under native conditions or in the presence of urea or sodium deoxycholate. Figure 32 Shows the results of an immunoblot analysis and protein stain of T.colubriformis L3 extract after 2-dimensional electrophoresis. Figure 33 Shows the presence of carbohydrate staining molecules in L3 extracts of 6 additional nematodes. Fi|gure34 Shows a Gel electrophoresis (8 % PAGE) and immunoblot analysis of r. colubriformis L3 extract (L3) and purified carbohydrate larval antigen (C) run under non-denaturing conditions (no detergent or reducing agent). Best Modes -for carrvinf^ out the invention 1. Materials and methods 1.1 Sheep immunizations by truncated infections All sheep experiments were conducted with the approval of Aliceville Animal Ethics Committee. Romney sheep were raised aematode-firee from birth, housed in pens and fed commercial sheep pellets, hay and water ad lib. Sheep were at least 4 months old at the start of the immunising infections. Sheep were immunised by truncated infections with 40 000 T. colubriformis L3 on at least three occasions. Each infection was terminated after 14 days by oral drenching with oxfendazole (System, Schering Plough Ltd., 4.5 mg kg"') and sheep were re-infected 7 days after drenching. In some experiments, sheep were given a fourth infection (booster dose), which was not terminated by drenching, as these sheep were slaughtered 2-3 days after boosting. 1.2. Sample collection Sheep slaughtered by captive bolt gun and exsanguinations. The small intestine was tied off into 5 m sections and each section was washed through with 4 x 150 ml saline to collect larvae. For biochemical analysis and in vivo challenges, mucus was collected from the first 6 ra of small intestine and processed as described (Harrison et al 1999) with the following modifications. After gentle rinsing with 100 ml saline to remove gut contents, the intestine was held at 4°C for 2 h and mucus was then squeezed out by firm pressure between thumb and fogger, followed by 2 x 5 ml washes with saline. Mucus and washings were pooled and processed as described (Harrison et al 1999) and stored at-20'C. Biopsy samples of mucus were collected from groups of 4 truncated infection sheep at 3 days, 16 days and 35 days after the last immunizations. At surgery, the duodenum was located and a 5 cm section was isolated by gentle clamping with forceps. 3 ml saline was injected using a blunt ended 18-gauge needle. The liquid was teased back and forth 10 times to mix mucus with the saline and a 2-3 ml sample was then withdrawn. The incision was closed and the sheep allowed to recover. 1.3 Effect of various treatments on mucus activity in vitro Ability of mucus to bind larvae was assessed by a larval clumping test where 2000 unsheathe were incubated with 0.4 ml mucus in an Splendor tube at 37°C on a rocking platform. After 4 h, samples were examined and the degree of larval clumping was estimated, compared to controls of L3 incubated with naive mucus or saline. Immune mucus was subjected to various treatments and then analysed for larval clumping activity. Aliquots of 1 ml immune mucus IPS were dialyzed for 24 h against saline at 4°C; cenlrifoged at 10 000 x g, 50 000 x g or 100 000 x g; heated at 60°C or lOO°C for 5 min; reduced and calculated by treatment with 10 mM DTT for 1 h then reaction with 20 mM iodoacetamide for 30 min on ice followed by dialysis against TBS pH 7.4 overnight to remove excess sails. for peeps u-eruct, adjusted to pH 4,5 with I M BCl and 3 mg pepsin in O.I M acetate burlap 4.5 was added to 3 ml mucus and incubated for 20 h at 37*^0 on a rocking platoon. The reaction was stopped by adding tris to 2 M. Protease treatment was conducted by adding 1 mg promise in 0.1 M tris pH 7.5 to each ml of mucus and incubating for 20 h at 37°C on a rocking platform. The reaction was stopped by adding protease inhibitors. Mucus was treated with 1 mg Ukase in PBS pH 7.2 per ml mucus, incubated at 37**C for 20 h, then stored frozen. Mucus was oxidized by adjusting the pH to 4.5 with acetic acid, adding period ate to 20 mM in 50 mM sodium acetate buffer pH 4.5 and incubating in the dark at RT for 2 h with stirring. Sodium borohydride was then added to 50 mM and incubated for 1 h with stirring. Mucus was ultra filtered by diluting 5 ml iimnune mucus IP5 into 250 ml PBS pH 7.2 and concentrating back to 5 ml on a Filtering 100 000 mw membrane. The filtrate was then concentrated to 5 ml on a 10 000 mw membrane and this filtrate was reduced to 5 ml on a 3 000 mw membrane. The low mw filtrate was lyophilized, rediscover in 5 ml d.H20 and dialyzed in 1 000 mw tubing against d-HsO. After treatment as described above, mucus samples were stored frozen until assayed. 1.4 In vivo mucus assay 40 000 unsheathed L3 were incubated with 2.5-10 ml volumes of immune or naive mucus for 4-24 h before infusion into the duodenum of parasite-naive sheep via a surgically implanted catheter (Harrison et al 1999). One week later, sheep were slaughtered and the numbers of larvae establishing in each 5 m section of intestine were estimated, 40 000 unsheathed L3 were incubated at 37 " C for 4 h with 10 ml volumes of unman or naive mucus, or with 2 x 10 ml volumes of mucus supernatant after centrifugation at 100 000 X g. After incubation, one aliquot of naive and immune supernatant was centrifuged at 200 x g for 3 min to pellet the larvae. The supernatant was removes oy aspiration and the L3 were washed with 10 ml saline, centrifuged as above, the supernatant removed and the L3 resuspended in 10 ml saline. Each 10 ml aliquot was then infused via a duodenal cannel, into the intestine of a naive sheep. One week later, the sheep were slaughtered and larval counts obtained. 1.5 Biocheniical analysis of mucus A panel of immune and naive mucus series was analysed for differences in protein profiles by SDS PAGE and staining with Compassion blue or silver. Differences in glycosylalion were examined by lectin Wetting using biotin labeled lections, detected by streptaviditi-peroxidase. Presence of IgG in mucus was demonstrated by blotting against RAS/IgG-HRP. 1.6 Characterizations of mucus antibody Immunoblots of L3 homogenate antigen were probed with immune and naive mucus samples. Antibody binding was detected with RAS/IgG-HRP, or with mAb's to sheep IgGi, IgGa. IgM and IgA. followed by GAM/Ig-HRP. Exsheathed L3 were incubated for 4 h al ST^C with mucus supernatant, 45 % ammonium caliphate precipitated antibody from mucus or Protein G purified antibody from mucus. After incubation, larvae were washed 3 times with TBS-Tw and any bound antibody was eluted by incubation for 5 mins in 0.1 M glycine-HCl pH 2.4. The equals were neutralised with 1 m tris and used to probe blots of L3 antigen from Tc, Ns and Cc. 500 ml volumes of gut contents tom immune sheep were treated with 45 % ammonium sulphate to recover antibody. After dialysis, these antibodies were used to probe blots of L3 antigen. Larvae wert incubated for 2h with mucus supernatant or mucus antibody eluted from Protein G-Sparse, washed 3 tines with TBS-Tw and reacted with FTTC-RAS/IgG. After washing, larvae were examined by fluorescence microscopy. Larvae were collected from sheep at various times after infection and were analysed by immunofluorescence and immunoblotting as described above and by immunogold electron microscopy, larvae were fixed in BGPA fixative (1% glutaraldehyde, 15% saturated picric acid in O.IM phosphate buffer pH 7.2, at 90*^0). Embedded sections were stained with Protein G purified mucus antibody followed by gold labeled anti-sheep %. Antibody liters of mucus samples used for in vivo challenge experiments were estimated by EIA. Microstates plates were coated with Tc L3 antigen and reacted with dilutions of mucus. After washing, bound antibody was detected with RAS/lgG-HRP or mAb to sheep IgA (Serotek) followed by RAM/Ig-HRP. 1.7 Preparation of monoclonal antibody PAB-1 Mice Were immunised with polyacrylamide gel slices containing the Tc larval surface antigen. The location of the antigen in the gel was determined by blotting adjacent lanes and detecting the antigen with mucus antibody as described. Antigen containing gel slices were macerated, mixed with an equal volume of an incomplete oil adjuvant and injected into mice on two occasions two weeks apart. Ten days later, test bleeds were taken and screened against crude Tc L3 antigen and partially purified surface antigen. Spleen cells from the strongest positive mouse were fused with NS-1 cells using standard methods for preparing monoclonal antibodies. Primary and secondary screening was performed using ELBA and blotting to confirm specificity. A bulk culture of mAb PAB-1 was prepared and aliquots stored at -20" C. Monoclonal antibody PAB-1 was used to probe blots of larval antigens. Bound antibody was detected with RAM/IgG-HRP. Exsheathed larvae were fixed by heating at 90°C for 20 minutes, reacted with PAB-l, washed extensively with TBS-Tw, reacted with RAM/IgG-FTTC and examined under uv light. A mAb raised against an unrelated protein (sheep cytokine) and of the same subclass as PAB-1 was used as a negative control. 1.8 Immuno-affinity purification of larval antigen Monoclonal antibody PAB-1 was reacted with Protein A-agar’s to allow the antibody to bind. After washing with PBS to remove unbound antibody, the bound antibody was permanently immobilised to the Protein A by reaction with the cross-Inking agent DSS (disuccinimidy! sunbathe). After further washing, L3 extract was run through the PAB-1-Proiein A-agarose column, washed extensively in PBS containing 0.05% Twin 20 and any bound antigen was eluted in 0.2 M glycine-HCl pH 2.5. The elate was neutralised with 1 M Tris, dialyses against 5mM Tris pH 8.0 and concentrated in a Speedway concentrator. The antibody column was re-equilibrated by extensive washing with PBS. Samples of the antigen eluted from the column were analysed by SDS PAGE and blotting (Fig.23). Carbohydrate was detected in gels by staining with a modified silver strain (Kittelberger, et al, 1993) or on blots by reaction with biotin-hydrazide (Bouchez-Mahiout, acted, 1999). 1.9 Characterizations of larval antigen Exsheathed Tc L3 were frozen in liquid N2, ground with a mortar and pestle and proteins extracted by solubilisation in either 2 % Ch^s + 2 % Tween 20, 1 % sodium deoxychoiate (DOC), 2% SDS or 9 M urea. The extracts were centriiuged at 10 000 g and the supernatant stored at -20° C. Eggs, LI, L2 and adult nematodes were solubilised directly in SDS PAGE sample buffer (2% SDS. 20niM DTT in 50 mM tris-HCI pH 6.8). SDS antigen extract was used for electrophoresis and blotting studies; Ch^s and urea exu-act was used for 2D electrophoresis; urea extract was dialyses against 50 mM tris-HCl pH 7.4 for 2 days to remove urea prior to chemical or enzymatic treatments. Electrophoresis was also carried out using buffer only, 0.5 % DOC or 6 M urea, with the appropriately solubilised antigen. 2D electrophoresis was performed by running Tc L3 urea extract on Immobilized on pi 3-10 strips using the foghorn (Phoenicia), followed by SDS PAGE. Proteins were either stained with Compassion blue or silver, or reacted on blots with antibody from mucus to detect antigens. Tc L3 urea-solubilised antigen was dialyzed as above and subjected to precipitation by addition of either an equal volume of 10% TCA; 10 volumes of cold acetone; 9 volumes of chloroform:methanol (2:1); or 9 volumes of hexane;isopropano! (3:2). Samples were vorfcxed and rocked for 10 min, centrifuged at for 10 min and the precipitated pellets analysed by immunoblotting. The role of carbohydrates was investigated by chemical and enzymatic degradation. Antigen was treated with 20 mM periodic acid at 37° C for 24 h; or with 1 M NaOH ± 18 hat 60°C. Samples were dialyses before electrophoresis. Antigen was treated with hydrazine for 7 and 14 days at lOO°C, or with trifluoroacetic acid for 4 and 16 h at ^ C, after which the chemicals were evapourated using a Speedvac centrifuge and residual antigen was resolubiiised in SDS PAGE sample buffer, Enzymatic digestions were carried out by dissolving each enzyme in the buffer recommended by the manufacturer and incubating with antigen for 22 h at 37° C. Enzymes used were N-glycosidase F, trypsin, pepsin, palm, promised, proteinase K, subdivision, lipase, lysozyme, lactase, collagen’s, phosphoinositol-phospholipase C, phospholipids A2, phospholipase D. Coloured substrates casein-restrain and elastic-Congo Red were used as controls for protease and lactase activity. In one experiment, antigen was heat denatured at 90" C for 20 min prior to digestion with trypsin or NaOH. Proteinase K digestion was also performed at 50" C for 18 h with or without 0.5 %SDS, ISraMDTT, 50 mMEDTA or 2 mMCaaa. Larval extracts of Haemonchus contortus, Ostertagia circumcincta, Coopery cortices and Nematodirus spcuhiger were also treated with proteinase K under similar conditions. 1.10 Immunizations with the 35 kDa antigen. Five Romney sheep aged 12 months were injected i.p. on 3 occasions, 2 weeks apart, with 35 kDa antigen in a vegetable oil adjuvant containing Span 85, Twecn 85 and sesame oil (ratio 5.4: 4.6; 90). The antigen was obtained from gel slices of electrophoreses aerated Tc L3 antigen. After electrophoresis, the side strips of each gel were blotted to nititxreJIulose aud reacted with immune mucus to detect the 35 kDa antigen. After development with RAS/IgG-HRP. the blots were re-aligned with the main porous of the gel and a slice was excised corresponding to the location of the 35 kDa antigen. The gel slice was placed in dialysis tubing in 100 mM tris HQ pH 7.8 and the antigen was electro eluted from the gel by placing the dialysis tubing In a blotting tank at 50 v for 3 h. Multiple elates were pooled and protein yield estimated to be 0.2 mg/ml by BCA protein assay. The antigen was blended with an equal volume of vegetable oil adjuvant using an Ultraturrax homogenizers. Each sheep received approximately 0.2 mg total protein at each injection although the amount of carbohydrate antigen was not known. Control sheep were injected i.p. with saline plus adjuvant. Two weeks after the third injection, all sheep were challenged infected orally with 40000 Tc L3. Faecal egg comit data were obtained 3 and 4 weeks after challenge. 2. Results 2.1. In vitro assays The ability of whole mucus or mucus subjected to various treatments to cause larval clumping in vitro is shown in Table I (refer page 33). The results indicate that dialysis or low speed centrifugation did not affect the ability of immune mucus to clump larvae. Centrifugation at 100 000 x g reduced the larval clumping effect unless the detergents or CHAPS were present. Larval clumping activity was still present after heating at 60°C for 5 min but not after heating at lOO^C. Mucus treated with protease digestion or period ate oxidation lost activity but lipase treatment had no effect. The larval clumping activity was associated with the high molecular weight fraction of mucus. 2.2. In vivo assays The effect of incubating L3 with increasing volumes of mucus, on subsequent displacement and reduction of numbers of larvae in naive recipient sheep is shown in Fig 1. Larvae that were incubated in 5 or 10 ml of naive mucus were able to establish normally in the first 5 m of small intestine. Larvae that were incubated in immune mucus were progressively displaced or rejected as the volume of mucus was increased. Incubation of larvae with 10 ml immune mucus resulted in 82 % reduction of larvae establishing and 100 % displacement of larvae out of the first 5 m of intestine, compared to naive mucus. The effect of incubating L3 with 10 ml volumes of mucus for different times is shown in Fig. 2. Incubation of immune mucus and L3 for as little as 1 h resulted in 46 % reduction of larval establishment and 81 % displacement from the first 5 m. Incubation for 4,10 or 24 h resulted in >94 % reduction and >93 % displacement. The effect on larval establishment of incubating 13 with 16 naive mucus samples and 25 immune mucus samples is shown in Fig. 3. Overall there was 67 % reduction of larvae establishing in recipients of L3 + immune mucus (range 0-95%) and there were 80 % fewer larvae establishing in the first 5 m of intestine (P The effect of incubating L3 with the 100 000 x g supematants of naive or immune mucus, with or without subsequent washing, is shown in Table 2 (refer page 34). The result shows that L3 incubated in naive mucus, supernatant or supernatant plus washing, were able to establish in naive sheep. In contrast, L3 that had been incubated in immune mucus, supematant or supernatant plus washing, were mostly prevented from establishing and there were 91 % fewer L3 than in sheep receiving L3 treated with naive mucus. 2.3 Mucus biochemistry Electrophoreses separation of mucus is shown in Fig. 5. The protein profiles of immune and naive mucus were highly complex and no clear cut differences were observed between the two sets of mucus. Leda blotting also showed complex glycoprotein profiles for both sets of mucus (Figs 6, 7, 8) indicating that ranges of carbohydrate moieties were present. Again there was no clear difference in the binding of lecterns to immune or naive mucus, with the exception of peanut agglutinin (Fig. 7A) where increased staining was seen with most of the immune samples at mw's of approximately 70 000 and 28 000 which may correspond to Ig heavy and light chains. However, when mucus was reacted with RAS/IgG-HRP, major bands were seen in all samples at 55 000 and 27 000, which probably correspond to IgG heavy and light chains (Fig 8B). 2.4 Mucus blotting Immunoblots of TcLS antigen probed with mucus or antibodies recovered from mucus are shown in Fig. 9. Six naive mucus samples Oanes 13-18) did not react with L3 antigen. Immune mucus samples reacted predominantly with a 35 kDa band as did antibody recovered by ammonium sulphate precipitation of gut contents from 2 humane sheep (lanes 8 and 9). Antibody from immune mucus supernatant purified on Protein G-agarose and antibody acid-eluted from L3 incubated with immune mucus also reacted with the 35 kDa band Oases 4,7 and 6,20). Both IgG and IgA antibodies could be eluted off the L3 (Fig 9, lanes 6 and 20). Serum from sheep given 3 truncated infections with Tc also contained antibodies that recognised the 35 kDa band plus many others (not shown). Antibody isotope specificity of the antibodies in mucus reacting with the 35 kDa band are shown in Fig. 10. IgGj and IgA ecotype antibodies were present but IgG2 or IgM antibodies were not detected. Immunoblots of L3 antigen extracts from the intestinal parasitic nematodes Nematodirus spathiger Q^s) and Cooperia curticei (Cc) probed with mucus from Tc immune sheep showed predominant reactivity wifli bands at 22 kDa (Fig. 11, lanes 9 and 13). Senim from sheep given truncated infections of Ns reacted with these antigens in both Ns and Cc Oanes 12 and 16) and also with the 35 kDa band in Tc (laneg). Incubating 2 ml immune mucus with 260000 exsheathed Tc L3 resulted in complete depletion of antibody fii^m the mucus (lane I). Colloidal gold protein stain was used to detect proteins on the blot (lane 4). No staining was seen in the region corresponding to that detected by antibody from immune mucus (lanes 3 and 4). Extracts ftt)m L3 of the intestinal nematodes N. spathiger and C curticei and the abomasal nematodes H. contorlus and O. circumcincta were probed with Tc immune sheep mucus and showed reactions at 35 kDa for Tc and He; 39 kDa for Oc; 46 and 22 kDa for Cc; and 22 for Ns (Fig 12). Figure 33 shows blots of 1 M NaOH extracts of the intestinal nematodes T.axei(Ta), T.vitrinus (Tv), O.ostertagi (Ooi, C.oncophera (Co) and D.eckerti (De) and of the abomasal nematodes H. contortus (He) and O. circumcincta (Oc) the blots were probed with Tc immune sheep mucus and showed reactions at 35 kDa for Ta, Tv and He; 45, 35, 33 and 30 kDa for Oo; 45 and 20 kDa for Co; 12 and 9 kDa for ^n>; and 30 kDa for De. The correlation between mucus IgG and IgA antibody litres and the protection affforded by mucus used for in vivo challenges was analysed by linear regression (Fig 13). There was a significant relationship between the titres of IgG and IgA antibodies against L3 antigen and protection (R^ = 0.6; P Antibody tires of mucus biopsy san^>les were high at day 3 after immunizations (Fig 14) but lx>Th IgG and IgA titers fell away by 16 days but were still above backroom at 37 days after immunizations. Immunofluorescent staining of larvae is shown in Hg 15. Exsheathed L3 showed strong surface fluorescence after incubation with antibody from immune mucus but not with naive mucus (top panel). Larvae collected from sheep infected for 2, 3 or 4 days also showed surface staining (not shown) but at day 5 after infection, many larvae did not stain with antibody and some were observed in the process of moulting Gower panel). The shed L3 cuticle reacted with antibody from immune mucus but the emerging L4 did not stain. L4 collected at day 6 and 7 after infection also did not show surface staining. Immunogold electron microscopy revealed a similar pattern of results where sections of L3 showed surface labelling with gold particles on the epicuticle (panel B, Fig 16). Gtold labelling was also observed on day 2 after infection, was weaker at day 3 and 4 and absent at day 5 (panels C, D, E and F, respectively). Immunoblots of antigen extracts from eggs, LI, 12, L3 and from larvae collected at various times after infection were probed with mucus antibody (Figs 17 & 18). The 35 kDa antigen was seen in L3 before infection and up to 5 days after infection but was not present in the egg stage, LI or L2, or in L4 at days 7 or 14 after infection, or in adult nematodes. 2.5 Monoclonal antibody PAB-1 Comparative blotting reactions of mAb PAB-1 and Tc immune sheep mucus antibody against Tc L3 antigen are shown in Fig 19. The mAb reacted with the main Tc L3 antigen at 35 kDa, a diffuse antigen at 35-40 kDa and a number of lower molecular weight antigens. Identification of antigens in other nematode species is shown in Fig 20. Extracts from L3 of the intestinal nematodes N. spathiger and C. curticei and the abdominals nematodes H. contortus and O. circumcincta were probed with mAb PAB-1 and showed reactions at approximately 35 kDa for Tc and He; 39 kDa for Oc; 46 and 22 kDa for Cc; and 22 for Ns (Fig 20). After digestion of L3 extracts with proteinase K, immunoblotting against antibody from immune mucus or nnAb PAB-1 showed that the larval antigens were not destroyed by this enzyme (Figs 19 and 20). Reaction of mAb PAB-1 with escheated Tc L3 showed strong surface fluorescence after staining with anti-mouse FTTC conjugate (Fig.2l). An IgGa control mAb did not react with the larval surface. 2.6 Immune-affinity purification of larval antigen The results of immuno-affinity purification of larval antigen using the monoclonal antibody PAB-1 coupled to Protein A-agarose are stiown in Figure 22. Silver staining of the eluate showed that no protein-staining band was visible in the region where the larval antigen was expected to run. A single carbohydrate staining band was detected in the eluate which ran at the same molecular weight as the antigen detected by immunoblotting with antibody from immune sheep mucus. Tliis band was also libeled in situ with biotin-hydrazide reagent which binds to exposed sugar residues after period ate oxidation. 2.7 Characterizations of larval antigen The effect of various chemical and enzymatic treatments of L3 antigen on the immunoblot reaction of mucus antibody against the 35 kDa antigen is shown in Pigs 23-30. Heating the antigen 813?" C for 18 h had no effect on the unmunoblot reaction to the 35 kDa antigen (Fig 23, lane 2). Treatment with periodic add or lipase slightly reduced the signal strength (Fig 23, lanes 3, 5) but pronase had no effect Qane 4). The 35 kDa antigen was found in the precipitate after either acid or solvent precipitation (lanes 6-9). Treatment of L3 antigen with trypsin, pepsin, proteinase K or phospholipase A2 caused the blot reaction to become more diffuse but did not reduce the molecular weight (Fig 24, lanes 2, 3,5,11). Treatment with pepsin, subdivision or lying enzymes reduced the signal but did not alter the molecular weight (lanes 6-8). Promise, lipase, lysozyme, phosphoinositol-phospholipase C and phospholipase D had no effect flanes 4, 9, 10, 12, 13). Treatment with lactase resulted in the appearance of a slightly lower molecular weight band (Fig 25, lane 1). CoUagenase and proteinase K at 37" C had no effect (lanes 2, 3, 4). Proteinase K treatment at SO'^C for 18 h under various conditions also did not destroy the 35 IcDa antigen whichh could still be detected on blots (lanes 6-9). Treatment of L3 antigen with N-glycosidase r signup reduce UK blot signal but did not decrease the molecular weight of the 35 kDa antigen (Fig 26, lane 4) under conditions where the control glycoprotein feting was degraded (lane 2) indicating that the enzyme was active. Treatment with 1 M NaOH at 60° C for IS h resulted in an increase in the number of lower molecular weight bands seen on the blot but the reaction at 35 kDa was still dominant (Fig 27, lane 2). After treatment with NaOH plus NaBH4 , no protein was visible by silver staining although the blot reaction of the 35 kDa antigen was undiminished compared to the control antigen (Fig 27, lane 3). Treatment of L3 antigen with hydrofluorous acid for 48 h at 4^* C or with hydrazine for I h at 20° C or for 16 h at lOO" C, did not destroy the 35 kDa antigen (Fig 28). Treatment with hydrazme for 7 or 14 days at 100° C reduced the blot signal compared to untreated control antigen (Fig 29, lanes 1, 2). Treatment with trifluoroacetic acid for 4 h or 16 h destroyed the antigen (Fig 29, lanes 4, 5). ligament of L3 antigen by the following procedures did not destroy the 35 kDa antigen as shown by Immunoblotting (Fig 30): proteinase K + SDS for 4 h or 20 h at 50°C (lanes I & 2): O.l-I.O M NaOH treatment at 37"c for 18 h (Fig 30, lanes 3,6,7,8): heat menstruation at 90'^ C for 20 min prior to digestion with I M NaOH Games 4): trypsin digestion at 37° C for 22 h with or without heat penetration at 90° C for 20 min Wanes 10 & 14); proteinase K ■¥ SDS + DTT at 50° C for 22 h (lane 12). Proteinase K digestion of L3 extracts from five nematode species did not destroy the Tc 35 kDa antigen or the cross-reacting antigens of the other species present at 46, 35 or 22 kDa (Fig 20). Tc L3 extract was analysed by electrophoresis and blotting under native conditions and in the presence of 0.5 % DOC or 6 M urea. The antigen ran as a high molecular weight sraear under these conditions (Fig 32). Addition of reducing agent (20 mM DTT) to the samples and the electrophoresis buffer did not alter these profiles (not shown). 2D electrophoretic analysis of Tc L3 urea extract showed a strong immunoblot reaction at 35 kDa, which extended across the range pH 3-10 (Fig 33). Despite the strong blot signal, no protein was visible in the corresponding region. 3.6. Sheep immunisation trial FEC data are shown in Table 3 (refer page 34). At week 3 after challenge, there was no significant difference in FEC between groups but at week 4, the counts were significantly lower in the immunised group (i'<:0.05 when counts from both weeks were combined there was also a significant reduction of fec overall in the immunised group> Figure 34 shows a Gel electrophoresis (8 % PAGE) and inmiunoblot analysis of T. colubriformis L3 extract (L3) and purified carbohydrate larval antigen (C) run under non-denaturing conditions (no detergent or reducing agent). Gels were stoned for protein or carbohydrate. Blots were reacted with mAb PAB-1 followed by rabbit anti-mouse Ig-HRP conjugate, or with immune sheep mucus followed by rabbit anti-sheep Ig-HRP conjugate. obsei-ved that larvae were frequently clumped together after incubation in immune mucus and that these larvae were prevented from establishing normally when infused into naive sheep via a duodenal cannel (Harrison et al 1999). These observations were extended in the present study and showed conclusively that immune mucus can effectively prevent establishment of larvae. The degree of protection gains infection depended on the time of mucus collection after immunization as well as dose volume. This correlates with the declining level of antibody in mucus over time as seen in mucus biopsy samples taken from truncated infection sheep up to 5 weeks after immunization. The observation that the 100 000 x g supernatant of immune mucus could also prevent larval establishment indicates that this activity sides in the soluble fraction of mucus and does not result from physical blocking by mucus e.g. by viscosity. Washing the larvae after incubation did not affect the abuts of immune mucus supernatant to prevent establistiment, indicating that the activity factor was bound to the larvae. In vitro analysis of larval clumping after treatment of immune mucus by dialysis, centrifugation or molecular weight filtration, indicated that the clumping activity was associated wifli the high molecular weight fraction of mucus. Heat treatment and protease digestion suggested that clumping required the protein component of mucus. However, SDS PAGE analysis and protein detection with Compasses blue or silver staining did not reveal differences in the crude protein profiles of a panel of immune and naive mucus samples. Similarly, lectin blotting did not show differences in glycoprotein composition between the two panels of mucus, with the exception of peanut agglutinin, which may have detected carbohydrates present on heavy and light chains and seen in immune mucus samples. The heavy chains were at 70 kDa which could indicate the presence of IgA. Blotting also showed the presence of IgG in all mucus samples. The above observations and presence of IgG and IgA in immune mucus suggested that antibodies recognising nematode antigens were responsible for larval clumping and for in vivo protection, taimunoblots of larval antigen probed with immune mucus showed the presence of IgGi and IgA antibodies which reacted predominantly with a major antigen at 35 kDa plus diffuse regions at 9, 12, 20, 30-45 kDa. Significantly, blots of L3 antigens probed with antibodies eluted from intact exsheathed larvae after incubation in immune mucus also showed predominant reaction to this antigen. This result, plus the surface fluorescent staining and immunogold electron microscopy, show that the epitopes are present on the surface of the larvae. Anti-35 kDa antibody was present in mucus samples used for in vivo challenge experiments and there was a significant correlation between the degree of protection afforded by immune mucus and the titer of Fig and . Mucus antibody from T. colubriformis immune sheep also recognised antigens on blots of larval extracts from other intestinal nematodes C. cortices,. N. spathiger, T.axei, Tvitrinus, O.ostertagi, C.oncophera, N.brasiliensis and D.eckerti and from aromas nematodes H. contortus and O. circwncincta. This cross-reactivity indicates that a surface molecule with similar function to the T. colubriformis 35 kDa antigen exists in other nematode species and could be a target for immunizations. Monoclonal antibody PAB-1 also reacted with these antigens and could thus be used to identify and purify these surface antigens from parasitic nematode species. The finding that ail the cross-reacting antigens tested so far are resistant to digestion by proteinase K is evidence that they are also not proteins and thus share similar properties to the T. colubriformis 35 kDa antigen. Monoclonal antibody PAB-1 coupled to Protein A-I arose was able to purify T.colubrifonnis larval surface antigen. This T.colubriformis larval surface antigen was found to be predominantly carbohydrate as shown by its resistance to digestion with a range of proteases including proteinase K; by staining with a silver stain modified to detect carbohydrate groups and by labeling with a biotin-hydrazide reagent which binds to exposed sugar residues. The antig°en did not stain with protein detecting methods such as silver stain, Compasses blue or gold. The antigen was resistant to degradation by the action of lipases and was not soluble in organic solvents which suggests that lipid components are not present or not accessible. N-glycosidase F treatment did not affect the antigen indicating either that the sugars ait not N-Inked or that they are not accessible to enzyme attack. Alkali treatment or extensive hydrazinolysis did not destroy the antigen which may indicate an unusual carbohydrate structure. Strong acid hydrolysis with trifluoroacetic acid destroyed the antigen. The observation of a multiple banding pattern in the form of a ladder of lower molecular weight antigens on blots of T. colubriformis larval extent probed with mAb PAB-1, could indicate that the structure of the 35 kDa antigen consists of a polymer of a smaller unit. In its native state on the larval surface, however, the antigen is a high molecular weight complex as shown by the electrophoresis results using non-denaturing conditions. Solubilisation in SDS + DTT reduced the complex to an antigen detectable on blots at 35 kDa suggesting that the complex is a polymer of the 35 kDa antigen or a heteropolymer of 35 kDa antigen plus other components as yet unidentified. The antigen shows charge heterogeneity when started by is electric focussing, again indicating a complex structure. The results suggest that this molecular complex, present on the outer surface of larvae, is likely to resist degradation by all physiological conditions found in the stomach and intestines of the nematode' s host, The functional implications of these properties of the larval surface antigen have yet to be determined but it seems likely that this complex has evolved to protect the larva during transit through the hostile environment of the host system until it reaches it's site of predilection in the small intestine. The 35 kDa antigen was only found in the L3 before infection and up to 5 days after infection, suggesting that the coating was required for protection during transit through the stomach. During the moult to L4 stage in the small intestine, the protective coating is shed as it is no longer required. It will be appreciated that an immune response directed against this protective coat could severely compromise the nematode's ability to establish succession in its host and could therefore have wide implications for nematode control. In a preliminary vaccine trial in sheep, immunizations with a vaccine containing partially purified 35 kDa antigen and an oil adjuvant resulted in a significant reduction of faecal egg count in the vaccinated group compared to controls. Aspects of the present invention have been described by way of example only and it should be appreciated that modifications and additions may be made thCTeto without departing from the scope of the appended claims. References Bouchez-Mahiout L., Doyen C, Lauriere M. 1999. Accurate detection of both glycoproteins and total proteins on blots: control of side reactions occurring after periodate oxidation of proteins. Electrophoresis: 20, 1412-1417. Carhsle MS, McGregor DD, Appleton JA. Intestinal raucus entrapment of Trichinella spiralis larvae induced by specific antibodies. Immunology 1991;74: 546-551. Douch PGC, Harrison GBL, Buchanan LL, Greer KS. In vitro bioassay of sheep gastrointestinal mucus for nematode paralysing activity mediated by substances with some properties characteristic of SRS-A. Iht J Parasitol 1983; 13:207-212. Emery DL, McCIure SJ, Bendixsen T, Windon RG. Investigations of the role of hypersensitivity responses in immunity against ovine gastrointestinal nematodes. In: Husband AJ, editor. Mucosal Solutions: Advances in Mucosal Immunology. University of Sydney Press, 1997;359-366. Harrison GBL, Pulford HD, Gatehouse TK, Shaw RJ, Pfeffer A, Shoemaker CB. Studies on the role of mucus and mucosal hypersensitivity reactions during rejection of Trichostrongylus colubriformis from the intestine of immune sheep using an experimental challenge model. Int J Parasitol 1999; 29:459-468. Jones WO, Windon RG, Steel JW, Outteridge PM. Histamine and leukotriene concentrations in duodenal tissue and mucus of lambs selected for high and low responsiveness to vaccination and challenge with Trichostrongylus colubriformis. hit J Parasite 1990;20;1075-1079. Kittelbergw R. and Milbank F. 1993. Sensate silver-staining detection of bacterial lipopoiysaccharides in polyacrylamide gels. J. Brioche. Biophysics. Methods 26: 81-6 Copeland Mislaid, Nature, 256, 495-497"(1975). Lee GB, Ogilvy BM. The mucus layer in intestinal nematode infections. GHz: Okra PL and Bienenstock J, editors. The Mucosa] Immune System in Health and Disease. Columbus.-Ross Laboratories 1981 175-183. Miller HRP. Gastrointestinal mucus, a medium for survival and for elimination of parasitic nematodes and protozoa. Parasitology 1987; 94:S77-S100. Miller HRP. Mucosal mast cells and the allergic response agents nematode parasites. Vet Immunology Imraunopathol 1996; 54:331-336. Rothwell TLW. Immune expulsion of parasitic nematodes from the alimentary tract. Int Parasite 1989;19:139-168. Sangster and Gill. Pharmacology of Anthelmintic Resistance Parasitology Today. 1999, Vol 15, No. 4 Van Wyk, Stenson, Van Der Merwe, Vorster, Viljoen. Anthelmintic Resistance in South Africa: Surveys indicate an extremely serious situation in sheep and goat farming. 1999. Waller, Anathematic Resistance. Veterinary Parasitology, 1997, 391-412. 1 We claim; 1. An isolated monoclonal antibody mAb PAB-1, deposited at ATCC on 24 January 2002 and accorded accession PTA-4005, which binds to a surface antigen on nematodeL3, wherein the antigen runs substantially between 20-35 kDa or at substantially 9 kDa and 12kDa on SDS PAGE gel under reducing conditions. 2. An isolated monoclonal antibody as claimed in claim 1 wherein the antibody binds to an antigen sourced from T.colubriformis L3, wherein in said antigen runs at substantially 35kDa on SDS PAGE gel under reducing conditions. 3. An isolated monoclonal antibody as claimed in claim 1 wherein the antibody binds to surface antigens on L3 selected from the group consisting of: a) a surface antigen on C.curticei which nms at substantially 46 kDa and at substantially 22kDa on SDS PAGE gel under reducing conditions; b) a surface antigen on N.spathiger which nms at substantially 22kDa on SDS PAGE gel under reducing conditions; c) a surface antigen on H.contortus which nms at substantially 35kDa on SDS PAGE gel under reducing conditions; and d) a surface antigen on O.circumcincta which nms at substantially 35-39kDa on SDS PAGE gel under reducing conditions; e) a surface antigen on Zajei or Strums which runs at substantiality 35kDa on SDS PAGE gel undo reducing conditions; f) a surface antigen on O.ostertagi which runs at substantially 30-45 kDa on SDS PAGE gel under reducing conditions; g) a surface antigen on Comic-opera which runs at substantially 20 kDa and at substantially 45 kDa on SDS PAGE gel under reducing h) a surface antigen on N.brasUiensis which runs at substantially 9 kDA and at substantially 12 kDa on SDS PAOE gel under deducing conditions; i) a surface antigen on Decertify which runs at substantially 30 kDa on SDS PAGE gel under reducing conditions. 4. An isolated monoclonal antibody as claimed in claim 1 wherein the antibody wiles coupled to a solid support can be utilised to purify the surface antigen hy immuno-ability chromatogrqjhy. 5. An isolated carbohydrate surface antigen from a nematode L3, wherein the antigen binds to monoclonal antibody mAb PABl, deposited at ATCC on 24 January 2002 and accorded accession PTA-4005. 6. An isolated antigen as claimed in claim 5 wherein the antigen is sourced from Colubriformis L3, 7, An isolated antigen as claimed in claim S wherein the antigen is-sourced from nematode L3 isolated from ttie group consisting of C.curticei, N. sponger, H.contortm, O.circumcincta. T.axel, T.vitrima, O.ostertagi, C.oncophera, H.brasilmisis stand D.eckertL 8, A composition that comprises an antigen as claimed in claim 5 together with a known phammaceutically or sedentarily acceptable carrier or diluents. 9. A process for the manufacturing a composition for preventing, treating reducing the susceptibility to, nematode infection characterised by the step of using an antigen as claimed in claim 5. 10. A process as claimed in claim 8, wherein the nematode is selected from the group consisting of T.colubriformis, C.curticei, N.spathiger, H.contortus, O.circumcincta T.axei, T. Vishnu’s, O.stertagi, C. encipher, N. brasiliensis and D. Eckert. 11. A composition as claimed in claim 8, for preventing, treating, reducing the susceptibility to, nematode infestation in susceptible animals other than sheep wherein these other species of nematodes also possess a larval surface antigen identified by reaction with monoclonal antibody PAB-1 as described above. 12. A composition as claimed in claim 8, wherein the composition also includes at least one known adjuvant or cytokine. 13. An isolated antibody as claimed in claim 3 wherein the antibody has been sourced from the gastrointestinal mucus of an animal which has been immunised by truncated infections with nematodes selected from the group consisting of T.colubriformis, C. cortices, N.spathiger, H. contortus, O.circumcincta T.axei, T.vitn'nus, O.ostertagi, C.oncophera, N.brasiliensis. 14. A kit for detecting nematode infection in sheep which includes an antibody as claimed in any one of claims 1 -3. 15. A kit for detecting nematode infection in animals which includes an antigen as claimed in any one of claims 5-7. 16. An assay to detect nematode infection in animals which includes an antigen as claimed in any one of claims 5-7. 17. An assay to measure the degree of nematode infection which uses an antigen as claims in any one of claims 5-7. |
---|
1644-chenp-2004 correspondence-others.pdf
1644-chenp-2004 correspondence-po.pdf
1644-chenp-2004 description (complete)-duplicate.pdf
1644-chenp-2004 description (complete).pdf
1644-chenp-2004 drawings-duplicate.pdf
1644-chenp-2004 pct search report.pdf
Patent Number | 222653 | |||||||||||||||
---|---|---|---|---|---|---|---|---|---|---|---|---|---|---|---|---|
Indian Patent Application Number | 1644/CHENP/2004 | |||||||||||||||
PG Journal Number | 47/2008 | |||||||||||||||
Publication Date | 21-Nov-2008 | |||||||||||||||
Grant Date | 20-Aug-2008 | |||||||||||||||
Date of Filing | 26-Jul-2004 | |||||||||||||||
Name of Patentee | OVITA LIMITED | |||||||||||||||
Applicant Address | LEVEL 4, NZI HOUSE, 9 MORAY PLACE, DUNEDIN | |||||||||||||||
Inventors:
|
||||||||||||||||
PCT International Classification Number | CO7K16/18 | |||||||||||||||
PCT International Application Number | PCT/NZ03/00010 | |||||||||||||||
PCT International Filing date | 2003-01-30 | |||||||||||||||
PCT Conventions:
|