Use of the 27-Kilodalton Recombinant Protein from Paracoccidioides brasiliensis in Serodiagnosis of Paracoccidioidomycosis

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Clinical and Diagnostic Laboratory Immunology, November 1998, p. 826-830, Vol. 5, No. 6
1071-412X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Use of the 27-Kilodalton Recombinant Protein from Paracoccidioides brasiliensis in Serodiagnosis of Paracoccidioidomycosis

B. L. Ortiz, S. Díez, M. E. Urán, J. M. Rivas, M. Romero, V. Caicedo, A. Restrepo, and J. G. McEwen^*

Biochemistry and Molecular Biology Units and Mycology Group, Corporación para Investigaciones Biológicas (CIB), Medellín, Colombia

Received 21 July 1998/Returned for modification 17 August 1998/Accepted 10 September 1998

	ABSTRACT

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Paracoccidioidomycosis (PCM) is one of the most important endemic mycoses in Latin America; it is usually diagnosed by observationand/or isolation of the etiologic agent, Paracoccidioides brasiliensis,as well as by a variety of immunological methods. Although thelatter are effective, two circumstances, cross-reactions withother mycotic agents and antigen preparation that is marked byextreme variability among lots, hinder proper standardizationof the procedures. To circumvent this lack of reproducibility,molecular biology tools were used to produce a recombinant 27-kDa-molecular-massantigen from this fungus; a sizable quantity of this antigen wasobtained through fermentation of Escherichia coli DH5 $alpha$ , whichis capable of expressing the fungal protein. The latter was purifiedby the Prep-Cell System (Bio-Rad); the recovery rate of the pureprotein was approximately 6%. A battery of 160 human serum samples,consisting of 64 specimens taken at the time of diagnosis frompatients with PCM representing the various clinical forms plus15 serum specimens each from patients with histoplasmosis andaspergillosis, 10 each from patients with cryptococcosis and tuberculosis,6 from patients with coccidioidomycosis, and 40 from healthy subjects,were all tested by an indirect enzyme-linked immunosorbent assaywith the purified 27-kDa recombinant protein. The latter was usedat a concentration of 1.0 µg/well; there were three serum dilutions(1:1,000, 1:2,000, and 1:4,000). The experiment was repeated atleast twice. The average sensitivity for both experiments was73.4%; in comparison with the healthy subjects, the specificityfor PCM patients was 87.5% while for patients with other mycoses,it was 58.7%. Important cross-reactions with sera from patientswith aspergillosis and histoplasmosis were detected. The positivepredictive value of the test was 90.4%. These results indicatethat it is possible to employ recombinant antigenic proteins forthe immunologic diagnosis of PCM and, by so doing, achieve highcoverage rates. Furthermore, antigen reproducibility can now beensured, thus facilitating inter- and intralaboratorystandardization.

	INTRODUCTION

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Paracoccidioidomycosis (PCM), a disease caused by the thermally dimorphic fungus Paracoccidioides brasiliensis, is prevalentin most countries of Latin America, where it afflicts mainly adultmales engaged in agriculture (5, 18, 20, 22, 27). Thedisorder causes an important number of deaths (9, 14, 18,22, 26, 27). The disease varies in severity, and both thehost and the pathogen contribute to this end, as reflected inthe various clinical forms (5, 14, 15, 18, 20, 27).Prompt and accurate diagnosis is of the outmost importance sinceit allows initiation of specific therapy and thus avoidance ofcontinuous organ system damage (5, 15, 26, 27). Laboratorydiagnosis relies on the visualization of the causative agent indirect KOH preparations or biopsy specimens, as well as on itsisolation in culture (5, 18, 20). Serologic testing alsoplays an important role in diagnosis and is widely used for thispurpose (5, 25) and also for follow-up studies (5, 20,26).

In spite of their usefulness, serologic tests have certain important limitations such as cross-reactivity with tests for othermycotic disorders, mainly histoplasmosis, and the difficultiesencountered in the proper standardization of the various testsand reagents (5, 10, 25). One of the most difficult problemsto address is the lack of reproducibility of P. brasiliensis antigens(12, 13). Similar antigenic preparations exhibit strain variation,with antigens differing according to fungal form, incubation time,and culture medium employed; even under controlled conditionsand following identical protocols, there is variability in thefinal products (12, 13). Several important attempts have beenmade to circumvent this situation by employing purified and well-characterizedimmunologically reactive antigens derived from this pathogen,such as the 43-kDa (gp43) and the 58-kDa glycoprotein antigens,described by Camargo et al. and others (6, 29, 34) andby Figueroa et al. (12), respectively. In the last decade, theformer antigen has been used successfully in various types ofserologic tests and its reproducibility is higher than that ofother preparations (6, 25).

Advancements in molecular biology have allowed production of reproducible and characterized antigenic proteins through cloningand sequencing. In the case of P. brasiliensis, the gp43 antigenwas the first product to be thus studied in 1989 by Taba et al.(33); however, the clone was lost, and only recently (in 1996)was it prepared anew by Cisalpino et al. (7). Shortly thereafter,our group cloned and sequenced a 27-kDa antigenic protein fromthe fungus (23); in preliminary studies, this product was recognizedby antibodies present in sera from patients with PCM and appearedto be free of significant cross-reactivity (28). The presentreport extends the findings described above and shows that batchproduction of the recombinant 27-kDa antigenic product (p27) isfeasible. Additionally, the availability of this antigen allowedus to standardize an enzyme-linked immunosorbent assay (ELISA)for the diagnosis ofPCM.

	MATERIALS AND METHODS

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Recombinant protein. The original 27-kDa recombinant protein was cloned in the pBluescript II phagemid (Stratagene, La Jolla, Calif.) (1) andexpressed in Escherichia coli Sure (23) by using a cDNA libraryconstructed in the $lambda$ Zap II vector (Stratagene) (2, 32).

However, further trials with this strain of E. coli revealed that there was no expression of the transcript, and a differenthost cell, E. coli DH5 $alpha$ , was employed. The new host successfullycarried and expressed the recombinant protein. Plasmid DNA extractionand host cell transformation were done in accordance with themethods of Sambrook et al. (31).

Batch production and characterization of the recombinant protein. The recombinant bacterium was scale-grown in a Bioflo 4000 bioreactor (New Brunswick Scientific Co., New Brunswick, N.J.),under the conditions described in Table 1. To the culture mediumemployed, Luria broth base (Miller's Luria broth base; Oxoid Limited,Basingstoke, Hampshire, United Kingdom) (21), we added 50 to1,000 µg of ampicillin (aminobenzylpenicillin; Sigma, St. Louis,Mo.) per ml to control the purity of the transformed bacteriumand, at the higher concentrations, to retard the loss of expression(19). Finally, an antifoaming product, SAG 710 (Wiptcol Corporation,OSI Specialties, Sisterville, W. Va.), was employed (38).

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TABLE 1. Fermentation conditions

The inoculum consisted of a 24-h culture of the recombinant bacteria incubated at 37°C under continuous shaking (orbital incubatormodel INR-200; Sanyo-Gallenkamp plc, Leicester, Leicestershire,United Kingdom) that had an optical density (OD) at 595 nm of0.6. The optimal proportion of the inoculum was 3 to 10% of thetotal fermentation volume (24). During fermentation, the bioreactorcontrols all the parameters that influence the process (30).

At the end of the process, cell mass was determined by dry weight and the yield of protein was calculated by the Bradfordtechnique (Bradford kit 500-0001; Bio-Rad, Hercules, Calif.) (37).The expression of the recombinant protein was assessed by sodiumdodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE)(with a 12% polyacrylamide gel) run under denaturing conditions(37). The antigenic activity of the protein thus obtained wasassessed by transferring the gels to nitrocellulose membranes(Hybond-C; Amersham Life Sciences, Buckinghamshire, United Kingdom)by Western blot analysis (4, 35) if the protein was recognizedby the antibodies present in a pool of sera from patients withPCM.

Characterization and purification of the batch-produced recombinant protein. Purification was done by preparative electrophoresis using the Prep-Cell system (model 491; Bio-Rad) (3). The separatinggel at 12% was prepared under denaturing conditions with a totalof 35 to 90 mg of bacteria. The purified protein was precipitatedwith 2.25 volumes of chilled acetone per 150-µl sample volumeand left at $-$ 20°C for 6 h; the sediment was then centrifuged at9,280 relative centrifugal force at 5°C for 5 min. The supernatantwas discarded, and the sediment was collected and resuspendedin the sampling buffer and electrophoresed in an SDS-12% PAGEgel (37). The gels were stained with Coomassie blue. Once thepurified fractions corresponding to the recombinant protein wereidentified, they were dialyzed against phosphate-buffered saline(PBS) diluted 1:5 and concentrated by per-evaporation to 1/10their original volume and their protein content was measured bythe Bradford technique (Bio-Rad Bradford kit) (37).

Serum specimens employed. As shown in Table 2, 160 serum specimens were examined, 64 from patients with the various clinical forms of PCM, 15 eachfrom histoplasmosis and aspergillosis patients, 10 each from cryptococcosisand tuberculosis patients, 6 from coccidioidomycosis patients,and 40 from healthy subjects.

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TABLE 2. Human serum samples tested

ELISA testing. The purified recombinant antigen was initially titrated to determine its reactivity by using microtitration plates (Nunc ImmunoModule Star Well Maxisorp; Nunc-Intermed, Naperville, Ill.). Dilutionsof the 27-kDa recombinant antigen varied and ranged between 1and 0.125 µg per well. Serum dilution ranged from 1:1,000 to 1:4,000;the second antibody was used at concentrations of 1:8,000 to 1:64,000.A carbonate buffer described by Voller et al. was used throughout(36).

The indirect ELISA procedure described by Engvall and Perlmann was used (11). Plates were sensitized with the purified proteindiluted in carbonate buffer, pH 9.6 (36), in concentrationsranging from 0.5 to 4 µg per well. Incubation was carried outfor 30 min at 25 to 26°C and left at 4°C overnight. The plateswere allowed to stabilize at 22 to 26°C for 30 min. They werethen saturated with 5% bovine serum albumin dissolved in 1× PBSplus 0.05% Tween and incubated at the same temperature for 2 h(11, 36).

The plates were washed three times with the same PBS formulation, and the excess fluid was eliminated. Then, 100 µl of eachone of the three serum dilutions (1:1,000, 1:2,000 and 1:4,000)was applied to the respective well. Incubation was for 1 h at22 to 26°C. Washing and drying as described above were repeated,and then 100 µl of the peroxidase-labelled second antibody atthe indicated dilution (peroxidase-conjugated Affinipure goatanti-human antibody; Jackson Immunoresearch, West Grove, Pa.)was added to each well. The plates were incubated at the sametemperature for 1h.

After another cycle of washing and drying, the reaction was visualized with 100 µl of OPD (o-phenylenediamine; Sigma) 10 mgin 4 µl of hydrogen peroxide (Sigma), and dissolved in phosphatecitrate, pH 5.0. Incubation was for 15 min at 22 to 26°C. Thereaction was then stopped by using 100 µl of H₂SO₄ (4 N) per well.The plates were read at 450 nm in an ELISA reader (Bio-Rad microplatereader model 550). All tests were run induplicate.

Statistical procedures. The significance of positive values was determined by the Student t test (Microsoft Excel). Sensitivity and specificity weredetermined by the statistical method of Gallen and Gambino (16).

	RESULTS

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Recombinant protein. The expression of the 27-kDa recombinant protein by the transformed E. coli DH5 $alpha$ was poor during fermentation in culturesthat had low concentrations of ampicillin; it was then necessaryto increase its concentration to 1,000 µg/ml. A larger bacterialmass was thus obtained, and the expression of the 27-kDa proteinbecame significant. Furthermore, it was shown that this proteinwas antigenically active as it was recognized by anti-P. brasiliensisantibodies present in a pool of 16 PCM patient serum specimens(data notshown).

Batch production of the recombinant protein. The conditions under which the transformed E. coli cells were grown are given in Table 1. Optimal mass production was obtainedafter 6 h of fermentation when the OD was at its highest and thentapered off until the end of the fermentation at 8 h. The antifoamingagent did not influence the expression of the protein (data notshown).

At this time, the dry weight of the bacterial mass varied between 4 and 5 g/liter of culture medium. Total bacterial masswas 20 to 25 g/5liters.

Characterization and purification of the recombinant protein. Once batch production was accomplished, purification ensued as described previously (Prep-Cell). From approximately 45 mgof the bacterial mass, 3.0 mg of purified protein (6.6%) was obtained.The final product was tested by Western blotting in the presenceof the positive control (pooled PCM patient sera) and found tobe reactive (Fig. 1).

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FIG. 1. SDS-PAGE gel (A) and immunoblot (B) of the 27-kDa recombinant protein of P. brasiliensis. (A) SDS-12% PAGE gel with Coomassie blue stain; (B) immunoblot developed with a mixture of sera from patients with PCM. Lanes: 1, E. coli nonrecombinant; 2, E. coli recombinant; 3, purified protein. This figure was obtained through scanning with the NIH Image 1.61/ppc computer program (Power Macintosh) (ftp://zippy.nimh.nih.gov).

Diagnostic tests. As shown in Fig. 2, the indirect ELISA procedure revealed that the sera from patients with PCM as well the positive control(pool of PCM patient sera) demonstrated higher reactivity in comparisonwith those of the specimens from patients with other mycoses ortuberculosis and from healthy individuals, regardless of the serumdilution.

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FIG. 2. Indirect ELISA with P. brasiliensis 27-kDa recombinant protein. The sera evaluated were positive control p27 (pool of 15 sera from PCM patients) ( $bullet$ ), PCM patient sera (

) (n = 64), histoplasmosis patient sera ( $black-triangle$ ), (n = 15), aspergillosis patient sera ( $black-down-triangle$ ) (n = 15), cryptococcosis patient sera ( $||$ ) (n = 10), coccidioidomycosis patient sera ( $cross$ ) (n = 6), tuberculosis patients () (n = 10), and healthy subjects (

) (n = 40).

According to statistical procedures, the cutoff point of sensitivity and specificity was estimated to be 1.4 times the medianpoint of those of the controlsera.

The results of the ELISA with the p27 recombinant protein (Fig. 3) revealed that 47 (73.4%) of the 64 PCM patient serum sampleswere reactive while 35 (87.5%) of the 40 samples from healthyindividuals were nonreactive. Important cross-reactions were noticedin the case of serum samples from aspergillosis and histoplasmosispatients, with 11 of 15 (73.3%) and 6 of 15 (40%) samples givingpositive results, respectively.

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FIG. 3. Comparison of reactivity and nonreactivity of serum samples. The numbers along the bottom of the figure represent the following sources of serum samples: 1, healthy subjects; 2, tuberculosis patients; 3, coccidioidomycosis patients; 4, cryptococcosis patients; 5, aspergillosis patients; 6, histoplasmosis patients; 7, PCM patients.

The ELISA had specificities of 87.5% for PCM patients when compared with healthy subjects (P < 0.001), 58.7% for patientswith other mycoses (P < 0.005), and 90% for patients with tuberculosis(P < 0.001).

Table 3 shows the sensitivities, specificities, and predictive values obtained for patients with the various clinical formsof PCM. Sensitivities were 66.7% for the chronic unifocal form,71.4% for the acute form, and 75.6% for the multifocal form. Incomparison with the heterologous sera, specificity was higherfor sera from patients with the acute form (87.5%) than for thosefrom patients with the chronic unifocal (83.3%) and chronic multifocal(84.4%) forms. Positive predictive values were similar, being80% for patients with the unifocal form and 83.3 and 82.9% forpatients with the acute and multifocal forms, respectively. Whenthese parameters were used without regard for the clinical form,the sensitivity was 73.4%, the specificity was 87.5%, and thepositive predictive value was 90.4%.

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TABLE 3. p27 recombinant protein: sensitivity, specificity, and predictive value of the ELISA

	DISCUSSION

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The p27 recombinant protein, cloned and sequenced previously by our group (23, 28) and expressed in the E. coli DH5 $alpha$ vector,was produced in sizable quantities by fermentation techniques.After purification by preparative electrophoresis, yields werein the range of 6%. The purified protein was found to be reactivewhen used as an antigen in the immunologic diagnosis of PCMpatients.

The p27 product is the second P. brasiliensis recombinant protein that has been cloned and sequenced; the first one was gp43,an immunodominant antigen cloned in 1989 (33) and characterizedfurther by Cisalpino et al. (7). The gp43 fraction has beenextensively and successfully employed as an antigen in the serologicaldiagnosis of PCM, but for this particular purpose, it has beenextracted directly from P. brasiliensis cultures and not by recombinantprocesses (6, 25).

Standardization of antigens for the immunologic diagnosis of PCM has been difficult to accomplish partly because of the variationsin antigen lots. As demonstrated by Franco et al. (13), differencesin activity, specificity, and potency of the final products varyeven with rigorous adherence to the same protocol. Such variationhinders inter- and intralaboratory comparisons (10, 13, 25).This problem could be solved by using recombinant antigens since,once cloned, the same antigenic moiety will be expressed by thetransformed vector (31). Furthermore, large quantities can beproduced, thus permitting standardization of diagnostic methods(8, 33).

As shown here, the ELISA required minimal amounts (1 µg/well) of the recombinant antigen and was able to detect anti-P. brasiliensisantibodies in the sera of 73.4% of the PCM patients tested atthe time of diagnosis. This figure is lower than the one reportedfor the traditional tests that employ complex antigens, such ascomplement fixation and agar gel immunodiffusion, which detectantibodies in 90 to 95% of the cases (5, 10, 25). The p27recombinant protein may well represent a single dominant antigenicepitope and, as such, may not be recognized for all patients.In the future, it might be necessary to use a cocktail of recombinantproteins to achieve higher sensitivityvalues.

In spite of the fact that previous testing by Western blotting (28) revealed no cross-reactions with sera from patientswith mycoses other than PCM, the ELISA procedure turned out tobe more sensitive, as it revealed important cross-reactivity withthe sera from patients with aspergillosis (73.3%) and histoplasmosis(40%). This is a point that should be addressed, since the smallnumber of specimens tested in each case could have influencedstatistical interpretations. Nonetheless, all the serologicalmethods presently in use have shown cross-reactions with serafrom patients with these mycotic disorders, regardless of theantigen utilized (10, 12, 25). More recently, aspergillosispatient sera have been shown to react in a monoclonal antibody-basedtechnique employed for the detection of P. brasiliensis circulatingantigens (17).

In comparison with the specificity for patients with other mycoses, the ELISA was less specific (58.7%) for PCM patients thanexpected, even if test results were still statistically significant(P < 0.005). The assay was much more specific for PCM patientswhen compared with healthy subjects (87.5%, P < 0.001) and patientswith tuberculosis (90%, P < 0.001). For all persons tested, specificitywas higher (73.4%) as was the positive predictive value (90.4%).

When the PCM patient sera were grouped according to clinical forms (14), variations were observed although the lower sensitivityvalues exceeded 66%. The lower positive predictive values (80%)were obtained in patients with the unifocal form since, in thisform, cellular immunity is still functional and as a consequencethe patients are capable of restricting fungal development (14).

It may well be that this particular 27-kDa antigenic epitope is not recognized by all PCM patients. These results furtherstrengthen the need for antigens that contain multiple reactiveepitopes.

The potential contributions of molecular biology to the production of suitable antigens for immunologic testing of this andother deep-seated mycoses is now beginning to be understood, andtheir future appears to bepromising.

	ACKNOWLEDGMENTS

This work was supported by a grant from COLCIENCIAS, Santafé de Bogotá, Colombia, project 2213-05-017-94.

We appreciate the valuable support received from the Instituto de Immunologia and its Director, Manuel Elkin Patarroyo, Santaféde Bogotá, Colombia. We are indebted to Diego Luis Alvarez forits advice with thestatistics.

	FOOTNOTES

^* Corresponding author. Mailing address: Molecular Biology Unit, Corporación para Investigaciones Biológicas (CIB), Carrera72A#78B-141, Medellín, Colombia. Phone: 57 4 441 0855. Fax: 574 441 5514. E-mail: cib{at}epm.net.co.

Present address: Department of Biology, Universidad de Antioquia, A.A. 1226 Medellín,Colombia.

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Abstract
Introduction
Materials & Methods
Results
Discussion
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Antimicrob. Agents Chemother.	Clin. Microbiol. Rev.	Infect. Immun.
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