Exocellular components of Paracoccidioides brasiliensis: identification of a specific antigen.

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Infect Immun. 1986 July; 53(1): 199-206

Exocellular components of Paracoccidioides brasiliensis: identification of a specific antigen.

R Puccia, S Schenkman, P A Gorin and L R Travassos

ABSTRACT

Yeast forms of Paracoccidioides brasiliensis grown in liquidmedium produced exocellular components. Immunodiffusion reactionsand immunoprecipitations of 131I-radiolabeled antigenic componentswith sera from patients having paracoccidioidomycosis (PCM)were used to monitor the isolation of specific constituents.Components having the main antigenic activity (fCon A) wereisolated by exclusion from a Bio-Gel P30 column, followed bysuccessive binding of eluted material to a Sepharose-concanavalinA column, and elution. The product contained, from sodium dodecylsulfate-polyacrylamide gel electrophoresis analysis, a minor43,000-molecular-weight (MW) component (gp43), a polydispersehigh-MW glycoconjugate, and a diffusely migrating 55,000-MWglycoprotein (gp55). Other components, including a 72,000-MWglycoprotein, were irregularly expressed. The high-MW glycoconjugatecomplex contained, on the basis of methylation and 13C nuclearmagnetic resonance data, a branched structure of mainly mannopyranosylunits. These were nonreducing ends, 6-O-, 2-O-, and 2,6-di-O-substituted,and the specific rotation of +16 degrees indicated that theglycosidic configurations of the units were alpha and beta ina ratio of ca. 1:1 (concanavalin A binding indicated that nonreducingends or 2-O-substituted units or both of alpha-D-mannopyranosewere present). A small proportion of nonreducing end units ofD-galactopyranose were also present in this polysaccharide.gp55 is a glycoprotein containing a complex carbohydrate moietywith fucose, mannose, galactose, and glucose, either as terminalnonreducing units or substituted in positions indicated by methylationdata. Both PCM and normal human sera precipitated the high-MWglycoconjugate from 131I-labeled fCon A preparations, whereasgp55 was unreactive with human sera. gp43 was a specific antigeniccomponent of P. brasiliensis culture filtrates which could beisolated in a pure form by gel filtration column chromatography(Sephadex G150) or by Sepharose-patient immunoglobulin G affinitychromatography. 131I-labeled gp43 reacted equally well with10 PCM sera and hyperimmune rabbit serum against the band Eantigen of Yarzabal at a 10(-3) dilution. At the same dilution,no reaction was detected with sera from normal individuals andfrom patients with other mycoses. Similarly, only PCM sera andthe hyperimmune anti-E serum gave precipitin lines with gp43in the less sensitive immunodiffusion tests. gp43 consistedof three components, with pI 6.7, 6.4 and 6.2, all of whichreacted with PCM serum.

Infect Immun. 1986 July; 53(1): 199-206

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