Cloning, Characterization, and Expression of a 200-Kilodalton Diagnostic Antigen of Babesia bigemina

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Journal of Clinical Microbiology, June 2000, p. 2240-2247, Vol. 38, No. 6
0095-1137/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Cloning, Characterization, and Expression of a 200-Kilodalton Diagnostic Antigen of Babesia bigemina

N. Tebele,¹^, R. A. Skilton,¹ J. Katende,¹ C. W. Wells,¹ V. Nene,¹ T. McElwain,² S. P. Morzaria,¹ and A. J. Musoke¹^,^*

International Livestock Research Institute, Nairobi, Kenya,¹ and Department of Veterinary Microbiology and Pathology, Washington State University, Pullman, Washington²

Received 16 September 1999/Returned for modification 6 February 2000/Accepted 29 March 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Current serological tests for Babesia bigemina use semipurified merozoite antigens derived from infected erythrocytes. Oneof the major drawbacks of these tests is that antigen qualitycan vary from batch to batch. Since the quality of the antigencontributes to the sensitivity and specificity of serologicaltests, the use of standardized recombinant antigens should ensureconsistency in assay quality. Previously, a 200-kDa merozoiteantigen (p200) was identified as a candidate diagnostic antigenfor use in a serological assay for the detection of B. bigeminaantibodies in infected cattle. In this study, we have cloned,characterized, and expressed p200. A 3.5-kbp cDNA clone encodingp200 was isolated and shown to be almost full length, lackingapproximately 300 bp at the 5' end. The predicted amino acid sequenceshows that p200 consists of a long, highly charged central repeatregion of an uninterrupted $alpha$ helix, indicative of a fibrous protein.Immunoelectron microscopy localized p200 to the merozoite cytoplasm,suggesting that the antigen may be a structural protein involvedin forming filament structures within the cytoskeleton. The 3.5-kbpcDNA was expressed in bacteria as a fusion protein with glutathioneS-transferase (GST), but the yield was poor. To improve the yield,cDNA fragments encoding antigenic domains of p200 were expressedas fusions with GST. One of these fusion proteins, C1A-GST, iscomposed of a 7-kDa fragment of the p200 repeat region and containsepitopes that react strongly with sera from cattle experimentallyinfected with B. bigemina. Recombinant C1A-GST should permit thedevelopment of an improved enzyme-linked immunosorbent assay forthe detection of antibodies against B. bigemina.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Babesia bigemina is a tick-borne protozoan parasite of cattle that causes a disease variously referred to as Texas fever,redwater fever, or cattle tick fever. The disease is characterizedby fever, hemolytic anemia, hemoglobinuria and, in acute cases,death (8). The parasite is widely distributed throughout Africa,southern Europe, southern Asia, southeastern Asia, Australia,Central America, and South America, coincident with its main tickvectors Boophilus decoloratus, Boophilus microplus, and Boophilusannulatus (2). Economically, it is most important as a causeof heavy losses in susceptible cattle, particularly in importedtaurinebreeds.

The classical diagnosis of animals acutely infected with Babesia is made by the light microscopic demonstration of intraerythrocyticparasites in Giemsa-stained blood smears (7). However, wheninfections are subclinical or latent, parasites may not alwaysbe demonstrable by microscopy because of low levels of parasitemia(13). Alternatively, infection of an animal by Babesia can bedetermined directly by PCR-based tests (4, 21) or indirectlyby measurement of the humoral response using serological tests(27). While PCR can provide good sensitivity and specificityand is able to detect current, carrier infections, such testsare complex and time-consuming, requiring specialized laboratoryequipment and highly trained personnel. As such, PCR-based testsare currently not applicable for use in many of the regions wherebabesiosis causes high economic losses. Serodiagnostic methods,however, are generally much simpler to perform and can provideimportant information for implementing control measures and forepidemiological studies. Several serological tests for the detectionof antibodies to B. bigemina have been developed, including complementfixation, passive hemagglutination, capillary tube agglutination,card agglutination, indirect immunofluorescence test, and enzyme-linkedimmunosorbent assay (ELISA) (17, 27). The indirect immunofluorescencetest and the ELISA are most widely used because of their superiorsensitivity, robustness, and ease of use. These tests, however,use either whole parasites or semipurified antigens, whose qualitiescan vary from batch to batch. Also, the production of antigensfor these tests requires experimentally infected cattle, makingproduction time-consuming andexpensive.

A merozoite antigen of approximately 200 kDa (p200) in B. bigemina is a candidate diagnostic antigen (18), and it was shownthat 98% of sera collected from cattle in areas in which B. bigeminais endemic recognized this antigen (J. M. Katende, unpublisheddata). Monoclonal antibodies (MAbs) to p200 were used to immobilizenative antigen in an indirect antibody ELISA. This ELISA was shownto be specific for B. bigemina antibodies, lacking cross-reactivitieswith sera from cattle infected with Babesia bovis, Theileria parva,Theileria taurotragi, or Anaplasma marginale (18). A major improvementin this assay would be obtained through the use of standardizedrecombinantp200.

In this study, the expression of recombinant p200 in bacteria was undertaken to facilitate the production of large quantitiesof standardized antigen for the development of a serodiagnostictest. Major bovine B-cell epitopes were identified within p200,and these were expressed as a recombinant 7-kDa fragment. Thisrecombinant p200 fragment is a strong candidate diagnostic antigenthat should facilitate the development of an improved antibodyELISA for B. bigemina.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Parasite stocks. B. bigemina (Kikuyu stock) from Kiambu District, Kenya, was provided by A. Kelly, National Veterinary Laboratories, Kabete,Kenya. The Pongola strain of B. bigemina was obtained from D.T. de Waal, Onderstepoort Veterinary Institute, Onderstepoort,SouthAfrica.

Purification of B. bigemina merozoites. B. bigemina merozoites were prepared from blood collected at peak parasitemia from experimentally infected, splenectomizedFriesian calves. Infected blood was collected into an equal volumeof heparinized Alsever's solution. The blood was centrifuged at2,500 × g for 30 min at 4°C, and the packed cells were washedfour times with Alsever's solution by centrifugation as before.For RNA preparation, an aliquot of the packed infected erythrocytepellet was lysed with an equal volume of 1% cold acetic acid inwater, and unlysed cells were removed by centrifugation at 2,500× g for 10 min at 4°C. The supernatant was centrifuged at 9,000× g for 10 min at 4°C. The pellet was resuspended in an equalvolume of Dulbecco's phosphate-buffered saline (DPBS) and centrifugedagain. The resulting pellet of B. bigemina merozoites and erythrocyteghost membranes was immediately snap frozen as droplets in liquidnitrogen and stored at $-$ 70°C. For genomic DNA extraction, packedinfected erythrocytes were lysed in an equal volume of 1 mg ofsaponin per ml in water for 10 s. Lysis was stopped by the additionof four volumes of 20 mM Tris-HCl (pH 8.0)-10 mM EDTA-100 mM NaCl(TEN buffer) and followed by centrifugation at 1,000 × g for 15min at 4°C to remove leukocyte nuclei and unlysed erythrocytes.The supernatant was recovered and further centrifuged at 8,000× g for 30 min at 4°C to pellet the merozoites. The pellet ofmerozoites was washed with TEN buffer by further centrifugationuntil it was free of hemoglobin and stored at $-$ 70°C.

Genomic DNA preparations. DNA was prepared from purified merozoites by standard methods of proteinase K digestion, phenol-chloroform extraction, andethanol precipitation (22). The B. bigemina DNA preparationsfrom Argentina (pathogenic strain S₂P), Brazil (wild-type strainB.68Cpo6dc), and Mexico (cloned strain J629) were obtained fromthe Department of Veterinary Microbiology and Pathology, WashingtonState University, Pullman. DNA from B. bovis (strain K_R) was obtainedfrom A. Lew and W. Jorgensen, Animal Research Institute, Yeerongpilly,Queensland,Australia.

Production of antibodies. Hyperimmune polyclonal antiserum BJ28 was prepared by intravenously inoculating a Boran steer with B. bigemina (Kikuyu) bloodstabilate. Three booster inoculations were given subcutaneouslyat 2-week intervals after the primary inoculation. Serum was collected2 weeks after the final inoculation. Bovine immunoglobulins (immunoglobulinG1 [IgG1] and IgG2) were purified by DE52 chromatography by standardprocedures (11) from sera pooled from 28 cattle that had recoveredfrom B. bigemina infection. Rat polyclonal antisera to p200 wasraised by inoculation with p200 purified by preparative sodiumdodecyl sulfate (SDS)-polyacrylamide gel electrophoresis (PAGE).MAbs Bb F4/86.6, Bb F4/86.11, Bb F4/86.19, and Bb F4/86.34, withspecificity for the B. bigemina p200 antigen, were derived fromBALB/c mice inoculated with B. bigemina (Kikuyu) merozoite lysateby methods described previously (19). Bb F4/86.6, Bb F4/86.11,and Bb F4/86.19 are isotype IgM, while Bb F4/86.34 is isotypeIgG1. For sequential bovine infection sera, Boran steer BJ26 wasinfected with B. bigemina sporozoite stabilate 3899, and serawere collected at approximately 5-day intervals over a 228-dayperiod.

ELISA, SDS-PAGE, and immunoblotting. The indirect antibody ELISA was carried out essentially as described previously (14). Bound antibodies were detected withhorseradish peroxidase (HRP)-conjugated secondary antibodies andABTS [2,2'-azino-bis(3-ethylbenzthiazoline-6-sulfonic acid)] asa chromogen. Optical densities (OD) were measured at 414 nm. Resultswere expressed as OD values or as percent positivity (PP) values.PP was calculated as follows: (OD of test serum/OD of a strongpositive serum) × 100 (13). SDS-PAGE under reducing conditionsand immunoblotting were performed as detailed previously (11).For immunoblotting, secondary antibodies were conjugated to HRP(14) or ¹²⁵I (Amersham International, Aylesbury, United Kingdom). For blotsincubated with HRP-labeled conjugates, antibody binding was visualizedby the addition of a substrate-chromogen (hydrogen peroxide-diaminobenzidine)solution. For filters incubated with ¹²⁵I-labeled conjugates, antibody binding was visualized by exposureto X-rayfilm.

Construction and immunoscreening of a B. bigemina cDNA expression library. Total RNA was isolated from B. bigemina (Kikuyu) merozoites by the hot phenol-SDS method (25). mRNA isolated by oligo(dT)-cellulosechromatography was used to construct an expression library in $lambda$ gt11 by methods described previously (22). Immunoscreeningof $lambda$ gt11 phage plaques propagated on Escherichia coli strain Y1090was carried out by standard methods (22). The library was screenedwith MAb Bb F4/86.6 diluted to 10 mg/ml, bovine recovery serumimmunoglobulins at 20 µg/ml, hyperimmune antiserum BJ28 dilutedto 1:100, and polyvalent rat antisera to p200 diluted to 1:50.Phage plaques that were positive with all the sera were selectedfor furtherstudy.

Southern and Northern hybridization. Southern hybridization was carried out by standard methods (22). Five micrograms of Babesia genomic DNA and 15 µg of bovinelymphocyte DNA were digested with EcoRI, electrophoresed througha 1% agarose gel, transferred to a Hybond-N nylon membrane (Amersham),and hybridized with an [ $alpha$ -³²P]dCTP-labeled probe. Blots were washed at a high stringency (0.1×SSC [1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate]-0.1% SDSat 65°C). Northern hybridization was carried out by publishedmethods (20). Two micrograms of B. bigemina merozoite mRNA waselectrophoresed through a 1% agarose gel and transferred to Hybond-N.Hybridization and washing of Northern blots were as describedfor Southernblots.

Sequencing of the cDNA encoding p200. The 3.5-kbp cDNA encoding p200 (designated Bb3.5) was subcloned into pUC18 for sequencing. Sequencing was performed with thefmol (Promega Corp., Madison, Wis.) and Sequenase (United StatesBiochemicals, Cleveland, Ohio) sequencing systems according tothe manufacturers' instructions and with primers to the vectorand primers based upon acquired sequences. Additional sequenceswere obtained from fragments of Bb3.5 cDNA that were generatedby PvuI, Sau3AI, and BAL 31 digestions, subcloned into pUC18,pBluescript II KS(+) (Stratagene, La Jolla, Calif.), or pNEB193(New England Biolabs), and sequenced with vector primers. Sequenceanalysis was performed with DNASIS V2.5 for Windows (Hitachi SoftwareEngineering America Ltd., San Bruno, Calif.) and PC/gene 6.80software (IntelliGenetics Inc., Mountain View, Calif.). The predictionof protein secondary structure and hydrophobicity was done withpublished algorithms (8, 11). The BLAST facility of the NationalCenter for Biotechnology Information was used for sequence homologysearches (http://www.ncbi.nlm.nih.gov/blast/blast.cgi).

Bacterial expression of the p200 antigen. Recombinant proteins were produced in bacteria as fusion proteins with 26-kDa glutathione S-transferase (GST) by use of thepGEX1 $lambda$ T expression system (Pharmacia Biotech, Uppsala, Sweden).Recombinant proteins were produced in E. coli strain XL1-Blue(Stratagene) and affinity purified on glutathione-Sepharose (Pharmacia)according to the manufacturer's instructions. Parental GST wasproduced from nonrecombinant vector pGEX1N (24).

Construction and immunoscreening of a subfragment library of the p200 3.5-kbp cDNA. Random DNA fragments of approximately 100 to 500 bp were created by digestion of the 3.5-kbp cDNA in pUC18 with a DNase ShotgunCleavage Kit (Novagen Inc., Madison, Wis.) according to the manufacturer'sinstructions. The fragments were cloned into $lambda$ gt11, and approximately10,000 recombinant plaques were immunoscreened with hyperimmuneantiserum BJ28. Immunopositive clones were also screened withMAbs Bb F4/86.6, Bb F4/86.11, Bb F4/86.19, and Bb F4/86.34. Insertsfrom selected clones were subcloned into pGEX1 $lambda$ T and expressedas GST fusionproteins.

Epitope mapping with synthetic peptides. A set of 11 overlapping peptides on pins was synthesized by Chiron Mimotopes (Clayton, Victoria, Australia) to represent thefragment of p200 encoded by clone C1A (see below). Each peptidewas 12 residues long and overlapped the preceding and subsequentpeptides by 7 residues, except for the last peptide, which overlappedthe preceding peptide by 10 residues. A 12-residue peptide withan irrelevant amino acid sequence was used as a control. The peptideswere tested in an ELISA with hyperimmune antiserum BJ28 dilutedto 1:100, naive bovine serum diluted to 1:100, and MAb Bb F4/86.6at a concentration of 10 µg/ml. For reuse, the pins were treatedin a sonication bath with 1% SDS-0.1% 2-mercaptoethanol in 0.1M phosphate buffer (pH 7.2) for 10 min at 60°C, followed by rinsingin distilled water at 60°C.

Localization of the B. bigemina p200 antigen in merozoites by immunoEM. A 200-µl aliquot of blood from a calf that had 10% parasitemia with B. bigemina (Kikuyu stock) was collected directly into2% parafomaldehyde in 0.1 M phosphate buffer (pH 7.3) and fixedin suspension for 1 h at room temperature. Fixed cells were centrifugedat 13,000 × g for 5 min, and the cell pellet was processed intoLowicryl K4M resin (Chemische Werke Lowi GmbH & Co., Waldkraiburg,Germany) by the method described previously (1). Cells wereprepared for immunogold electron microscopy (immunoEM) by themethod described previously (3). Briefly, 60-nm sections ofembedded cells were cut and collected on Parlodion-coated coppergrids. The sections were preincubated by flotation on 20-µl dropletsof 5% bovine serum albumin (BSA) in DPBS in a humidified chamberfor 30 min. The sections were then incubated for 1 h with MAbBb F4/86.11 diluted 1:50 in 5% BSA-DPBS. After being washed in5% BSA-DPBS, the sections were incubated for 1 h with goat antimouseIgG-5-nm colloidal gold (British Biocell, Cardiff, United Kingdom)diluted 1:10 in 5% BSA-DPBS. The sections were washed twice withDPBS, followed by two washes with distilled water. Sections werethen contrasted for 2 min with 2% aqueous osmium tetroxide, washed,and stained for 20 min with 2% aqueous uranyl acetate. The sectionswere examined with a Zeiss EM 10A electron microscope (Carl Zeiss,Oberkochen, Germany) operating at 80kV.

Nucleotide sequence accession number. Nucleotide sequence data reported in this paper are available in the GenBank database under accession number AF142406.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Characterization of antibodies to the B. bigemina p200 antigen. Anti-p200 antibodies that were used for immunoscreening an expression library were characterized by immunoblotting. Antigensrecognized by bovine hyperimmune serum BJ28, bovine recovery serumimmunoglobulins, rat antisera, and MAbs to the p200 antigen areshown in Fig. 1. All sera recognized the p200 antigen as a diffuseband extending from approximately 150 to 250 kDa. Hyperimmuneand recovery sera also recognized other proteins between 58 and125 kDa, but p200 appeared as the most immunodominant. Rat polyvalentantisera and MAbs were specific for p200. None of the antibodiesreacted with bovine erythrocyte proteins (data not shown).

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FIG. 1. Immunoblotting of B. bigemina merozoite lysate with antibodies to the p200 antigen. B. bigemina merozoite proteins were separated by SDS-PAGE through a 7.5 to 17.5% gradient gel, transferred to a nitrocellulose membrane, and probed with B. bigemina hyperimmune serum BJ28 diluted to 1:100 (lane 1), 20 µg of bovine recovery serum immunoglobulins per ml (lane 2), polyclonal rat antisera to p200 diluted to 1:50 (lane 3), and 10 µg each of anti-p200 MAbs Bb F4/86.6 (lane 4), Bb F4/86.34 (lane 5), and Bb F4/86.11 (lane 6) per ml. The positions of molecular mass standards are indicated to the left.

Isolation of cDNA encoding the p200 antigen. Approximately 80,000 PFU from a B. bigemina (Kikuyu) cDNA expression library in $lambda$ gt11 were immunoscreened for the p200 antigen.Thirty-five plaques were positive with all screening sera: MAbBb F4/86.6, bovine hyperimmune serum BJ28, bovine recovery serumimmunoglobulins, and rat antisera to p200. The clone that gavethe strongest signals on immunoscreening was selected for furtherstudy. The cDNA in this clone was estimated to be 3.5 kbp (datanot shown) and was designated Bb3.5.

Southern and Northern hybridization. In Southern blotting, Bb3.5 cDNA hybridized to a single band of approximately 20 kbp in EcoRI-digested DNA of B. bigeminaisolated from Kenya, South Africa, Australia, Brazil, Argentina,and Mexico (Fig. 2A), indicating that the p200 gene is conservedamong B. bigemina stocks and strains from different geographicalregions. There was no hybridization of Bb3.5 cDNA to B. bovisDNA (Fig. 2A) or to bovine lymphocyte DNA (data not shown). Bb3.5cDNA hybridized to a single band of 3.8 kb in a Northern blotof B. bigemina (Kikuyu) mRNA (Fig. 2B). A transcript of 3.8 kbis sufficient to encode a protein of approximately 140 kDa.

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FIG. 2. Southern and Northern hybridization. (A) Southern hybridization. Conservation of the gene encoding the p200 antigen among stocks of B. bigemina from different geographical locations. Genomic DNA (between 5 and 10 µg) was digested with EcoRI, electrophoresed through a 1% agarose gel, transferred to a nylon membrane, and probed with [ $alpha$ -³²P]dCTP-labeled Bb3.5 cDNA. The DNA samples were Kikuyu stock from Kenya (lane 1), Pongola strain from South Africa (lane 2), strain S₂P from Argentina (lane 3), strain J629 from Mexico (lane 4), wild-type strain B.68Cpo6dc from Brazil (lane 5), and B. bovis strain K_R from Australia (lane 6). The positions of DNA size markers are indicated on the left. (B) Northern hybridization. Two micrograms of B. bigemina (Kikuyu) mRNA was electrophoresed through a 1% agarose gel, transferred to a nylon membrane, and probed with [ $alpha$ -³²P]dCTP-labeled Bb3.5 cDNA (lane 1). RNA size markers (lane M) are indicated to the left.

Sequence analysis of the p200 Bb3.5 cDNA. Sequence analysis of the p200 Bb3.5 cDNA showed that it is composed of 3,464 bp (DNA data not shown) with a large open readingframe from bases 1 to 3324, sufficient to encode a protein of133 kDa. A TAG stop codon at position 3325 and a poly(A) tailat positions 3446 to 3464 demonstrated that the 3' end of Bb3.5cDNA was complete. There was no ATG initiation codon near the5' end of the sequence (the first ATG codon occurred at bp 253),indicating that Bb3.5 is a partial-length cDNA. Because the p200transcript is 3.8 kb (Fig. 2B), it was deduced that Bb3.5 couldbe lacking ~300 bases from the 5' end. The p200 amino acid sequencededuced from the open reading frame in Bb3.5 cDNA is shown inFig. 3. The amino acid sequence could be divided into three distinctregions: N- and C-terminal regions flanking a large central regioncontaining complex repeating peptide sequences.

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FIG. 3. Partial-length amino acid sequence of B. bigemina (Kikuyu) p200 as deduced from Bb3.5 cDNA. Amino acids 186 to 966 are vertically aligned to show the structure of repeat sequences. The left and middle columns (amino acids 186 to 741) are composed of R1 and R2 repeats, while the right column is composed of R3, R4, and R5 repeats. Potential sites for N-linked glycosylation are indicated by <UNL>N</UNL>

. The boxed and circled amino acid residues indicate potential sites for protein kinase C phosphorylation and casein kinase II phosphorylation, respectively. The sequence marked by single underlining represents overlapping regions (amino acids 213 to 270 and 257 to 314) which have 100% identity to the p200 fragment encoded by clone C1A. The sequence marked by double underlining (amino acids 883 to 960) represents a region which has 100% identity to the p200 fragment encoded by clone C3A.

Deduced amino acids 1 to 185 of the N terminus do not contain peptide repeats. Of these, 19% are charged, 44% are hydrophilic,and 37% are hydrophobic. Two asparagines at amino acid positions118 and 141 are potential sites for N-linked glycosylation. Serinesat positions 59 and 120 and a threonine at position 107 are potentialsites for protein kinase C phosphorylation, while the serine atposition 111 is a potential site for casein kinase IIphosphorylation.

The central repeat region of p200 is composed of 781 amino acids (positions 186 to 966), of which 74% are charged, 20% arehydrophobic, and 6% are hydrophilic. Fifty-one percent of thecharged residues are glutamic acid, and the remainder are arginine,histidine, lysine, and aspartic acid. The central region lackspotential sites of posttranslationalmodification.

Vertical alignment of the amino acids using a backbone of EKAERE identified five types of related repeating sequences, designatedR1 to R5 (Fig. 3). These repeats can be divided into two domains:amino acids 186 to 741, containing R1 and R2 repeats, and aminoacids 742 to 966, containing R3, R4, and R5repeats.

The R1 repeat has 8 amino acids with the consensus sequence EKAEREAK/R, while the R2 repeat has 10 amino acids with the consensussequence EKAEREQRER. There are 37 R1 repeats and 26 R2 repeats.The arrangement of amino acids in R1 and R2 is that of alternatingnegatively and positively charged residues interrupted by a hydrophobicor hydrophilic residue at positions 3 and 7. The sequences ofR1 and R2 are highly conserved, with only eight R1 repeats andone R2 repeat having amino acid substitutions. R1 alternates withR2 imperfectly, since there are one, two, or three R1 repeatsafter every R2repeat.

The R3 repeat has the consensus sequence EEAERLAREQ, which is similar to that of R2 except for substitutions at positions2, 6, 7, and 10. The consensus sequence of the R4 repeat, AEREAREK,is similar to that of amino acids 2 to 8 of R2 except for substitutionsat positions 5 and 8. The five-amino-acid R5 repeat sequence AEREAis identical to amino acids 3 to 7 of R1. The amino acid arrangementof charged, hydrophobic, and hydrophilic residues of the R3, R4,and R5 repeats is similar to that of R1 and R2. Seven of 13 R3repeats and 9 of 10 R4 repeats have at least one amino acid substitution.The three R5 repeats are conserved. The repeats are arranged suchthat an R3 repeat alternates with an R4 or R5repeat.

The C terminus of p200 (amino acids 967 to 1108) is composed of nonrepeating amino acid sequences, of which 35% are charged,25% are hydrophilic, and 40% are hydrophobic. The asparagine atposition 1029 is a candidate for N-linked glycosylation, whilethe serines at positions 986, 1006, and 1020 are potential sitesfor casein kinase IIphosphorylation.

From a search of protein databases, the predicted amino acid sequence of p200 showed similarities with several proteins thatwere also rich in glutamic acid. These proteins included troponinT, trichohyaline, calreticulin, and Plasmodium falciparum glutamicacid-rich protein, although the overall level of homology withthese proteins was insignificant (data notshown).

Predicted secondary structure of the p200 antigen. Computer analysis predicted that the highly charged central repeat region of p200 has a secondary structure of an uninterrupted $alpha$ helix (data not shown). All of the $alpha$ helix was predicted tobe hydrophilic. In contrast, the N and C termini were predictedto be composed of short fragments of coil, $beta$ -sheet, and $alpha$ -helixconformations, forming several regions of hydrophobicity (datanotshown).

ImmunoEM localization of the p200 antigen in B. bigemina merozoites. The p200 antigen is highly labile (data not shown) and therefore required mild fixation with 2% paraformaldehyde. These mildconditions, however, resulted in poor fixation, obscuring somedetail of the parasite ultrastructure. Labeling was predominantlycytosolic, with no labeling of rhoptries or the nucleus. The spheroidbody appeared to be labeled to a similar degree as the cytosol(Fig. 4).

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FIG. 4. Immunogold localization of the p200 antigen in B. bigemina merozoites by electron microscopy. The electron micrograph shows a longitudinal section through a merozoite in the erythrocyte cytoplasm. The spheroid body (S), rhoptries (R), and nucleus (N) of the merozoite are indicated. MAb Bb F4/86.11 immunogold labeling was mainly located in the merozoite cytoplasm, although some was also present in the spheroid body. Bar = 0.5 µm.

Expression of the p200 Bb3.5 cDNA. Bb3.5 cDNA was cloned into the EcoRI site of the pGEX1 $lambda$ T bacterial expression plasmid. The yield of GST-p200 fusion protein(Bb3.5-GST) was poor, equivalent to only 0.5 µg/ml of bacterialculture. SDS-PAGE analysis demonstrated that the Bb3.5-GST preparationcontained a diffuse band at approximately 150 to 250 kDa, a nonrecombinantGST-sized protein of 26 kDa, and several other bands of from 20to 100 kDa (Fig. 5A). On immunoblotting with MAb Bb F4/86.6, therewas a very strong signal extending over approximately 150 to 250kDa, indicating successful expression of recombinant Bb3.5-GST,albeit at low levels (Fig. 5B). Bb3.5-GST also reacted similarlywith bovine recovery sera (data not shown). Several bands of 20to 100 kDa in the Bb3.5-GST preparation were immunologically nonreactiveand may have been of bacterial origin.

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FIG. 5. SDS-PAGE and immunoblot analyses of p200 recombinant antigen. (A) One microgram of Bb3.5-GST fusion protein preparation was analyzed by SDS-PAGE and stained with Coomassie blue (lane 1). The bracket indicates a small amount of a high-molecular-weight protein. Five micrograms of GST was also electrophoresed (lane 2). (B) Immunoblot of gel arranged as in panel A and probed with MAb Bb F4/86.6. (C) Two micrograms of GST (lane 1) and 10 µg each of C1A-GST (lane 2) and C3A-GST (lane 3) were analyzed by SDS-PAGE and stained with Coomassie blue. (D) Immunoblot of gel arranged as for panel C and probed with hyperimmune serum BJ28. (E) Immunoblot of gel arranged as for panel C and probed with MAb Bb F4/86.6. The sizes of molecular mass standards (lanes M) are shown.

Identification and expression of antigenic regions of p200. A subfragment library of Bb3.5 cDNA was created in $lambda$ gt11. Ten thousand plaques were immunoscreened with hyperimmune serumBJ28, and 34 positive clones were identified; 5 of these alsoreacted with MAbs Bb F4/86.6, Bb F4/86.11, Bb F4/86.19, and BbF4/86.34. Two clones were selected for further study: clone C1A,which gave the strongest signal on immunoscreening with hyperimmuneserum BJ28, and clone C3A, which reacted weakly with serum BJ28but gave the strongest signal on immunoscreening with MAbs. Theinserts from C1A and C3A were subcloned into pGEX1 $lambda$ T, sequenced,and expressed. The protein encoded by the insert in C1A has identitywith two overlapping regions in p200 at positions 213 to 270 and257 to 314 (Fig. 3) and is therefore composed of R1 and R2 repeats.The protein encoded by the C3A insert has identity with residues883 to 960 of the p200 antigen (Fig. 3) and is therefore composedof R3, R4, and R5 repeats. Yields of C1A-GST and C3A-GST wereequivalent to 20 µg/ml of bacterial culture. On SDS-PAGE, C1A-GSTand C3A-GST appeared as stable fusion proteins of 33 and 39 kDa,respectively (Fig. 5C). This result demonstrates that the p200portion of C1A-GST is 7 kDa, while for C3A-GST, it is 11 kDa.On immunoblotting, C1A-GST reacted strongly with hyperimmune serumBJ28 but showed no reactivity with MAb Bb F4/86.6 (Fig. 5D andE). In contrast, C3A-GST reacted strongly with MAb Bb F4/86.6and weakly with hyperimmune serum BJ28 (Fig. 5D and E). Theseresults demonstrate that the major epitopes for these bovine andmurine antibodies are located within different regions ofp200.

Antibody epitope mapping with synthetic peptides. Eleven overlapping peptides representing the C1A fragment of p200 all reacted strongly with hyperimmune serum BJ28 (data notshown). C1A peptides showed no reactivity with a control bovineserum or with MAb Bb F4/86.6 (data not shown). A control peptidewith an irrelevant amino acid sequence showed no reactivity withBJ28 serum, control bovine serum, or MAb Bb F4/86.6 (data notshown).

Antibody responses in an experimentally infected animal. Steer BJ26 infected with a B. bigemina sporozoite stabilate developed a significant antibody response to p200 by day 14, asdetermined by an ELISA with C1A-GST as the antigen. The antibodyresponse was maintained at high levels until day 179, after whichthe response fell to approximately 60% its maximal level by day228 (Fig. 6). These results indicate that soon after infectionan animal can develop a detectable antibody response which isthen maintained over a long period.

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FIG. 6. Antibody responses to C1A-GST in sequential sera from a steer experimentally infected with B. bigemina. Boran steer BJ26 was infected with B. bigemina sporozoites, and sequential sera were collected over a period of 228 days. Sera were diluted to 1:100 and tested by an ELISA with C1A-GST as the antigen. ELISA OD values were expressed as PP.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Screening of a B. bigemina $lambda$ gt11 cDNA expression library with MAbs and polyclonal antibodies to the p200 antigen identifiedan immunoreactive clone that contained a 3.5-kbp insert (Bb3.5).Hybridization to DNA of B. bigemina that originated from Kenya,South Africa, Australia, Mexico, Argentina, and Brazil demonstratedthat the gene encoding the p200 antigen is geographically conserved.It was shown by Northern hybridization that the mRNA encodingp200 is 3.8 kb, indicating that the Bb3.5 cDNA was missing approximately300 bases from the 5' end. A transcript of 3.8 kb would encodea protein with a predicted mass of approximately 140,000, in contrastto the mass of 150 to 250 kDa on immunoblots of merozoite p200.The discrepancy in molecular mass is most likely due to the presenceof highly charged repeating amino acid residues, which may havedisrupted the binding of SDS to the protein (10). Similar migrationpatterns have been observed for a highly charged, glutamic acid-richprotein encoded by the Pf332 gene of P. falciparum and for whichthe predicted molecular mass of 700,000 is in marked contrastto the actual mass of 2,500 kDa (16).

A striking feature of the p200 protein is the presence of a central, highly charged, glutamic acid-rich region composed offive types of related repeat sequences, designated R1 to R5. Unlikerepetitive proteins of Plasmodium and Trypanosoma, where repeatsare arranged tandemly (6, 15), the repeats within p200 alternateimperfectly. The N-terminal end of the central repeat region iscomposed of highly conserved R1 and R2 repeats, suggesting thatthis region may be critical for the function of the protein. Incontrast, the C terminus of the central repeat region containsdivergent R3 and R4repeats.

Secondary structure analysis of p200 predicted a long $alpha$ -helical central domain flanked by short N- and C-terminal regionseach composed of alternating short segments of coil, $beta$ -sheet,and $alpha$ -helix conformations. The high propensity for an $alpha$ -helicalconformation in the repeats is due to the high proportion of helix-stabilizingamino acid residues, such as glutamic acid, alanine, lysine, andglutamine (29). The $alpha$ -helix of the central region of p200 ispredicted to form an elongated, uninterrupted, inflexiblerod.

Unlike the central repeat region, the N- and C-terminal regions contained consensus sites for posttranslational modification.Three sites for N-linked glycosylation, with typical NXS/T consensussequences, were identified. Also present were seven sites forcasein kinase II and protein kinase C phosphorylation. Restrictionof posttranslational modification sites to the C and N terminiis typical of proteins containing central regions of repeatedamino acids. A good example is the intermediate filaments (IF)of the cytoskeleton, which contain consensus sites for phosphorylationat the nonrepeating "head" and "tail" domains of the molecule(23). For IF, phosphorylation sites close to the repeat regionappear to affect filament assembly, while sites further away appearto be important for interactions with other cellular components.It has been shown that phosphorylation plays an important rolein the regulation of IF dispersal throughout the nucleus and thecytoplasm, especially during cell division (5). It is temptingto speculate that phosphorylation of the p200 antigen may be necessaryfor the molecule to perform its cellular functions. Immunogoldlocalization of the p200 antigen to the merozoite cytoplasm supportsthe idea that this protein may function as a cytoskeletal structuralprotein.

The p200 Bb3.5 cDNA was expressed as a fusion with GST. On immunoblotting, Bb3.5-GST appeared as a diffuse band that extendedfrom approximately 150 to 250 kDa, similar to native p200. Bb3.5-GSTreacted strongly with MAb Bb F4/86.6 and with bovine recoveryserum, indicating that it contained immunodominant epitopes. Amajor drawback in the use of Bb3.5-GST as a potential diagnosticantigen was the very low yield of fusion protein. It has beenobserved that fusions of GST with proteins that are larger than100 kDa are insoluble (24). It is possible that the low yieldsof Bb3.5-GST were due, at least in part, to poor solubility resultingfrom the large size of the p200 fragment being expressed. To improveyields of recombinant p200, we expressed small fragments of theantigen that contained the critical diagnostic epitopes. We producedtwo smaller constructs, C1A-GST and C3A-GST, containing 7- and11-kDa fragments of p200, respectively. C1A-GST reacted stronglywith bovine sera, whereas C3A-GST reacted strongly with MAbs top200. Since C1A was derived from the region containing R1 andR2 repeats and C3A was derived from the region containing R3,R4, and R5 repeats, it appears that the epitopes for the bovineand murine antibodies used in this study are located within differentregions of p200. ELISA analysis of synthetic peptides representingthe C1A protein showed that bovine epitopes are distributed throughoutthis fragment. C1A peptides did not react with MAb Bb F4/86.6,confirming that bovine and murine epitopes in p200 are distinct.Since the R1 and R2 repeats are well conserved in p200, it isassumed that the entire R1 and R2 repeat region (amino acids 186to 741 of the p200 antigen) is immunodominant incattle.

We have shown that an ELISA with C1A-GST as an antigen can detect a significant antibody response in an animal soon afterexperimental infection with B. bigemina (day 14). Also, this antibodyresponse was still detectable on day 228 postinfection, indicatingthat this assay can detect antibodies during both early and latestages of infection. Furthermore, it has been demonstrated thatELISAs with C1A-GST or native p200 are equally efficient at detectingantibodies in B. bigemina-infected cattle (26), indicating thatC1A contains major p200 epitopes recognized by bovine infectionsera. Detailed descriptions of the field and laboratory validationsof an ELISA with C1A-GST for the detection of antibodies to B.bigemina in cattle will be publishedelsewhere.

	ACKNOWLEDGMENTS

We sincerely thank W. Mwangi and P. Pandit for assistance with sequencing, C. Nkonge and L. Gichuru for assistance with theprotein analysis, and D. Lugo, T. Njoroge, A. Tonui, and S. Njugunafor monitoring infected animals. For artwork we thank D. Elsworth,F. Shikhubari, and J.Mwaura.

	FOOTNOTES

^* Corresponding author. Mailing address: International Livestock Research Institute (ILRI), P.O. Box 30709, Nairobi, Kenya.Phone: 254 (2) 630 743. Fax: 254 (2) 631 499. E-mail: a.musoke{at}cgiar.org.

ILRI publication 99/0164.

Present address: Linds Agricultural Services, Harare,Zimbabwe.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Berryman, M. A., and R. D. Rodewald. 1990. An enhanced method for post-embedding immunocytochemical staining which preserves cell membranes. J. Histochem. Cytochem. 38:159-170[Abstract].

2. Brown, C. G. D., A. G. Hunter, and A. G. Luckins. 1990. Diseases caused by protozoa, p. 161-226. In M. M. H. Sewell, and D. W. Brocklesby (ed.), Handbook on animal diseases in the tropics, 4th ed. Baillière Tindall, London, England.

3. Burleigh, B. A., C. W. Wells, M. W. Clarke, and P. R. Gardiner. 1993. An integral membrane glycoprotein associated with an endocytic compartment of Trypanosoma vivax: identification and partial characterization. J. Cell Biol. 120:339-352[Abstract/Free Full Text].

4. Calder, J. A., G. R. Reddy, L. Chieves, C. H. Courtney, R. Littell, J. R. Livengood, R. A. Norval, C. Smith, and J. B. Dame. 1996. Monitoring Babesia bovis infections in cattle by using PCR-based tests. J. Clin. Microbiol. 34:2748-2755[Abstract].

5. Chou, Y. H., E. Risevear, and R. D. Goldman. 1989. Phosphorylation and disassembly of intermediate filaments in mitotic cells. Proc. Natl. Acad. Sci. USA 86:1885-1889[Abstract/Free Full Text].

6. Cotrim, P. C., G. Paranhos-Baccala, M. R. Santos, C. Mortensen, M. I. Cano, M. Jolivet, M. E. Camargo, R. A. Mortara, and J. F. Da Silveira. 1995. Organization and expression of the gene encoding an immunodominant repetitive antigen associated to the cytoskeleton of Trypanosoma cruzi. Mol. Biochem. Parasitol. 71:89-98[CrossRef][Medline].

7. de Vos, A. J., and W. K. Jorgensen. 1991. Bovine babesiosis, p. 1/14-14/14. In Manual of recommended diagnostic techniques and requirements for biological products. Office International des Epizootics, Paris, France.

8. de Vos, A. J., F. T. Potgieter, D. T. De Waal, and J. van Heerden. 1994. Babesioses, p. 278-308. In J. A. W. Coetzer, G. R. Thompson, and R. C. Tustin (ed.), Infectious diseases of livestock with special reference to southern Africa. Oxford University Press, Oxford, United Kingdom.

9. Garnier, J., D. J. Osguthorpe, and B. Robson. 1978. Analysis of the accuracy and implications of simple methods for predicting the secondary structure of globular proteins. J. Mol. Biol. 120:97-120[CrossRef][Medline].

10. Hames, B. D. 1990. One-dimensional polyacrylamide gel electrophoresis, p. 1-147. In B. D. Hames, and D. Rickwood (ed.), Gel electrophoresis of proteins. A practical approach. Oxford University Press, Oxford, United Kingdom.

11. Harlow, E., and D. Lane. 1988. Antibodies: a laboratory manual. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

12. Janin, J. 1979. Surface and inside volumes in globular proteins. Nature 277:491-492[CrossRef][Medline].

13. Jorgensen, W., A. J. de Vos, and J. R. Dalgleish. 1994. Methods for diagnosis of babesiosis in developing countries. Present and future trends, p. 65-84. In G. Uilenberg, A. Permin, and J. W. Hansen (ed.), Use of applicable biotechnological methods for diagnosing haemoparasites. FAO, Rome, Italy.

14. Katende, J., S. Morzaria, P. Toye, R. Skilton, V. Nene, C. Nkonge, and A. Musoke. 1998. An enzyme-linked immunosorbent assay for detection of Theileria parva antibodies in cattle using a recombinant polymorphic immunodominant molecule. Parasitol. Res. 84:408-416[CrossRef][Medline].

15. Kemp, D. J., R. L. Coppel, and R. F. Anders. 1987. Repetitive proteins and genes of malaria. Annu. Rev. Microbiol. 41:181-208[CrossRef][Medline].

16. Mattei, D., and A. Scherf. 1992. The Pf322 gene of Plasmodium falciparum codes for a giant protein that is translocated from the parasite to the membrane of infected erythrocytes. Gene 110:71-79[CrossRef][Medline].

17. Montenegro, S., M. A. James, M. G. Levy, M. D. Preston, H. Esparza, and M. Ristic. 1981. Utilization of culture derived soluble antigen in the latex agglutination test for bovine babesiosis and anaplasmosis. Vet. Parasitol. 8:291-297[CrossRef].

18. Morzaria, S., J. Katende, A. Kairo, V. Nene, and A. Musoke. 1992. New methods for the diagnosis of Babesia bigemina infection. Mem. Inst. Oswaldo Cruz 87:201-205.

19. Pearson, T. W., M. Pinder, G. E. Roelants, S. K. Kar, L. B. Lundin, K. S. Mayor-Withey, and R. S. Hewett. 1980. Methods for derivation and detection of anti-parasite monoclonal antibodies. J. Immunol. Methods 34:141-154[CrossRef][Medline].

20. Pellé, R., and N. B. Murphy. 1993. Northern hybridization: rapid and simple electrophoretic conditions. Nucleic Acids Res. 21:2783-2784[Free Full Text].

21. Salem, G. H., X. Liu, J. D. Johnsrude, J. B. Dame, and G. Roman Reddy. 1999. Development and evaluation of an extra chromosomal DNA-based PCR test for diagnosing bovine babesiosis. Mol. Cell. Probes 13:107-113[CrossRef][Medline].

22. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

23. Shaw, G. 1989. Identification of previously unrecognised sequence motifs at the extreme carboxyterminus of the neurofilament. Biochem. Biophys. Res. Commun. 162:294-299[CrossRef][Medline].

24. Smith, D. B., and K. S. Johnson. 1988. Single-step purification of polypeptides expressed in Escherichia coli as fusions with glutathione-S-transferase. Gene 67:31-40[CrossRef][Medline].

25. Taylor, D. W., J. S. Cordingley, and A. E. Butterworth. 1984. Immunoprecipitation of surface antigen precursors from Schistosoma mansoni messenger RNA in vitro translation products. Mol. Biochem. Parasitol. 10:305-318[CrossRef][Medline].

26. Tebele, N. 1996. Ph.D. thesis. Brunel University, Uxbridge, United Kingdom.

27. Weiland, G., and I. Reiter. 1988. Methods for the measurement of the serological response to Babesia, p. 143-162. In M. Ristic (ed.), Babesiosis of domestic animals and man. CRC Press, Inc., Boca Raton, Fla.

28. Wright, I. G. 1990. Immunodiagnosis of and immunoprophylaxis against the haemoparasites Babesia sp. and Anaplasma sp. in domestic animals. Rev. Sci. Tech. 9:345-356[Medline].

29. Zubay, G. 1988. Methods for characterization and purification of proteins, p. 100-130. In Biochemistry. MacMillan Publishing Company, New York, N.Y.

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1.	Berryman, M. A., and R. D. Rodewald. 1990. An enhanced method for post-embedding immunocytochemical staining which preserves cell membranes. J. Histochem. Cytochem. 38:159-170[Abstract].
2.	Brown, C. G. D., A. G. Hunter, and A. G. Luckins. 1990. Diseases caused by protozoa, p. 161-226. In M. M. H. Sewell, and D. W. Brocklesby (ed.), Handbook on animal diseases in the tropics, 4th ed. Baillière Tindall, London, England.
3.	Burleigh, B. A., C. W. Wells, M. W. Clarke, and P. R. Gardiner. 1993. An integral membrane glycoprotein associated with an endocytic compartment of Trypanosoma vivax: identification and partial characterization. J. Cell Biol. 120:339-352[Abstract/Free Full Text].
4.	Calder, J. A., G. R. Reddy, L. Chieves, C. H. Courtney, R. Littell, J. R. Livengood, R. A. Norval, C. Smith, and J. B. Dame. 1996. Monitoring Babesia bovis infections in cattle by using PCR-based tests. J. Clin. Microbiol. 34:2748-2755[Abstract].
5.	Chou, Y. H., E. Risevear, and R. D. Goldman. 1989. Phosphorylation and disassembly of intermediate filaments in mitotic cells. Proc. Natl. Acad. Sci. USA 86:1885-1889[Abstract/Free Full Text].
6.	Cotrim, P. C., G. Paranhos-Baccala, M. R. Santos, C. Mortensen, M. I. Cano, M. Jolivet, M. E. Camargo, R. A. Mortara, and J. F. Da Silveira. 1995. Organization and expression of the gene encoding an immunodominant repetitive antigen associated to the cytoskeleton of Trypanosoma cruzi. Mol. Biochem. Parasitol. 71:89-98[CrossRef][Medline].
7.	de Vos, A. J., and W. K. Jorgensen. 1991. Bovine babesiosis, p. 1/14-14/14. In Manual of recommended diagnostic techniques and requirements for biological products. Office International des Epizootics, Paris, France.
8.	de Vos, A. J., F. T. Potgieter, D. T. De Waal, and J. van Heerden. 1994. Babesioses, p. 278-308. In J. A. W. Coetzer, G. R. Thompson, and R. C. Tustin (ed.), Infectious diseases of livestock with special reference to southern Africa. Oxford University Press, Oxford, United Kingdom.
9.	Garnier, J., D. J. Osguthorpe, and B. Robson. 1978. Analysis of the accuracy and implications of simple methods for predicting the secondary structure of globular proteins. J. Mol. Biol. 120:97-120[CrossRef][Medline].
10.	Hames, B. D. 1990. One-dimensional polyacrylamide gel electrophoresis, p. 1-147. In B. D. Hames, and D. Rickwood (ed.), Gel electrophoresis of proteins. A practical approach. Oxford University Press, Oxford, United Kingdom.
11.	Harlow, E., and D. Lane. 1988. Antibodies: a laboratory manual. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
12.	Janin, J. 1979. Surface and inside volumes in globular proteins. Nature 277:491-492[CrossRef][Medline].
13.	Jorgensen, W., A. J. de Vos, and J. R. Dalgleish. 1994. Methods for diagnosis of babesiosis in developing countries. Present and future trends, p. 65-84. In G. Uilenberg, A. Permin, and J. W. Hansen (ed.), Use of applicable biotechnological methods for diagnosing haemoparasites. FAO, Rome, Italy.
14.	Katende, J., S. Morzaria, P. Toye, R. Skilton, V. Nene, C. Nkonge, and A. Musoke. 1998. An enzyme-linked immunosorbent assay for detection of Theileria parva antibodies in cattle using a recombinant polymorphic immunodominant molecule. Parasitol. Res. 84:408-416[CrossRef][Medline].
15.	Kemp, D. J., R. L. Coppel, and R. F. Anders. 1987. Repetitive proteins and genes of malaria. Annu. Rev. Microbiol. 41:181-208[CrossRef][Medline].
16.	Mattei, D., and A. Scherf. 1992. The Pf322 gene of Plasmodium falciparum codes for a giant protein that is translocated from the parasite to the membrane of infected erythrocytes. Gene 110:71-79[CrossRef][Medline].
17.	Montenegro, S., M. A. James, M. G. Levy, M. D. Preston, H. Esparza, and M. Ristic. 1981. Utilization of culture derived soluble antigen in the latex agglutination test for bovine babesiosis and anaplasmosis. Vet. Parasitol. 8:291-297[CrossRef].
18.	Morzaria, S., J. Katende, A. Kairo, V. Nene, and A. Musoke. 1992. New methods for the diagnosis of Babesia bigemina infection. Mem. Inst. Oswaldo Cruz 87:201-205.
19.	Pearson, T. W., M. Pinder, G. E. Roelants, S. K. Kar, L. B. Lundin, K. S. Mayor-Withey, and R. S. Hewett. 1980. Methods for derivation and detection of anti-parasite monoclonal antibodies. J. Immunol. Methods 34:141-154[CrossRef][Medline].
20.	Pellé, R., and N. B. Murphy. 1993. Northern hybridization: rapid and simple electrophoretic conditions. Nucleic Acids Res. 21:2783-2784[Free Full Text].
21.	Salem, G. H., X. Liu, J. D. Johnsrude, J. B. Dame, and G. Roman Reddy. 1999. Development and evaluation of an extra chromosomal DNA-based PCR test for diagnosing bovine babesiosis. Mol. Cell. Probes 13:107-113[CrossRef][Medline].
22.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
23.	Shaw, G. 1989. Identification of previously unrecognised sequence motifs at the extreme carboxyterminus of the neurofilament. Biochem. Biophys. Res. Commun. 162:294-299[CrossRef][Medline].
24.	Smith, D. B., and K. S. Johnson. 1988. Single-step purification of polypeptides expressed in Escherichia coli as fusions with glutathione-S-transferase. Gene 67:31-40[CrossRef][Medline].
25.	Taylor, D. W., J. S. Cordingley, and A. E. Butterworth. 1984. Immunoprecipitation of surface antigen precursors from Schistosoma mansoni messenger RNA in vitro translation products. Mol. Biochem. Parasitol. 10:305-318[CrossRef][Medline].
26.	Tebele, N. 1996. Ph.D. thesis. Brunel University, Uxbridge, United Kingdom.
27.	Weiland, G., and I. Reiter. 1988. Methods for the measurement of the serological response to Babesia, p. 143-162. In M. Ristic (ed.), Babesiosis of domestic animals and man. CRC Press, Inc., Boca Raton, Fla.
28.	Wright, I. G. 1990. Immunodiagnosis of and immunoprophylaxis against the haemoparasites Babesia sp. and Anaplasma sp. in domestic animals. Rev. Sci. Tech. 9:345-356[Medline].
29.	Zubay, G. 1988. Methods for characterization and purification of proteins, p. 100-130. In Biochemistry. MacMillan Publishing Company, New York, N.Y.