Mapping of Candida albicans oligomannosidic epitopes by using monoclonal antibodies

Trinel, Pierre-André; Faille, Christine; Jacquinot, Pierre Marie; Cailliez, Jean‐Charles; Poulain, D.

doi:10.1128/iai.60.9.3845-3851.1992

Cited by 64 publications

(59 citation statements)

References 35 publications

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“…The Candida mannan has long been recognized for its antigenic properties [2^4]. We have con¢rmed the reactivity of MAb EB-CA1 with NGLs constructed with mannan acid stable oligomannosides [14], and shown that within this pool of oligomannose residues, the length of the oligomannoside chain was a limiting factor for recognition. A minimal number of ¢ve mannose residues was required for binding.…”

Section: Discussionmentioning

confidence: 92%

“…The sequential depolymerization of the mannan has been previously described [14]. The ¢rst step consisted of a mild acid hydrolysis: 500 mg mannan was dissolved in 10 mM HCl and heated for 30 min at 100³C.…”

Section: Depolymerization Of the Mannanmentioning

confidence: 99%

“…Yeast cells were obtained on SDA after 24 h at 37³C. Cytoplasmic and cell wall components were prepared according to a method of alkali extraction in reducing conditions (AERC) previously described [14]. Electrophoresis of these extracts (100 mg ml 3I proteins) was performed for 5 h at a constant current of 30 mA on 7^20% gradient polyacrylamide gel slabs.…”

Section: Western Blottingmentioning

confidence: 99%

“…the`Pastorex Candida' used for detection of mannanemia in patient sera [11]. We further used a method which consisted in coating ELISA plates with neoglycolipids (NGLs) constructed from mannan released oligomannosides [13,14]. Binding experiments and NMR analysis have shown the MabEBCA1 minimal epitope to consist in an K-linked mannopentaose of the C. albicans mannan acid stable domain.…”

Section: Introductionmentioning

confidence: 99%

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Nature of Candida albicans-derived carbohydrate antigen recognized by a monoclonal antibody in patient sera and distribution over Candida species

Jacquinot

1998

FEMS Microbiology Letters

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The minimal epitope of an anti-Candida albicans mannan monoclonal antibody (MAb) EB-CA1, used to detect mannanemia in patient sera, was determined. MAb EB-CA1 exhibited reactivity with oligomannosides released from the mannan acid stable domain, converted into neoglycolipids (NGLs) and coated onto ELISA plates. Reactivity occurred with mannopentaose and higher oligomers, whereas mannotriose and mannotetraose were unreactive. MAb EB-CA1 binding to mannan acid stable mannopentaose NGL displayed a dose dependent and saturable specific reactivity curve whereas there was a complete absence of binding, even at high concentrations, with NGLs constructed from the L-1,2-linked mannopentaose derived from the mannan acid labile fraction. MAb EB-CA1 binding to acid stable mannopentaose NGL was inhibited by the homologous oligomannoside but not by mannotriose and mannotetraose. NMR analysis showed that mannotriose and mannotetraose contained exclusively K-1,2-linked D-mannopyranose units and that mannopentaose was a mixture of a mannopentaose K-1,2-linked and an isomer in which the fifth mannose was K-1,6-linked to the reducing unit of manno-K-1,2 tetraose. Western blot analysis has shown that MAb EB-CA1 epitope was expressed on a wide range of C. albicans manno-glycoconjugate as well as on manno-glycoconjugates of other pathogenic species of the genus Candida, viz. C. tropicalis, C. glabrata, C. parapsilosis and C. krusei. z

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Section: Discussionmentioning

confidence: 92%

Section: Depolymerization Of the Mannanmentioning

confidence: 99%

Section: Western Blottingmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Nature of Candida albicans-derived carbohydrate antigen recognized by a monoclonal antibody in patient sera and distribution over Candida species

Jacquinot

1998

FEMS Microbiology Letters

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“…We have reported the presence of three kinds of b-1,2 linkage-containing side chains in the mannans from Candida species [11][12][13][14][15][16][17]. Because the b-1,2-linked mannose unit is present among the pathogenic fungi only in the mannan of the genus Candida and the b-1,2 linkage-containing side chains behave as strong antigens, many workers [18][19][20][21][22][23][24][25] have produced monoclonal antibodies to b-1,2-linked mannose units to protect against candidiasis, for the serodiagnosis of candidiasis, or for the identification of mechanisms of Candida infection. Furthermore, studies have indicated the b-1,2-linked mannose units participate in the adherence of Candida cells to mammalian cells as the first step in infection [26][27][28].…”

mentioning

confidence: 99%

Existence of novel β‐1,2 linkage‐containing side chain in the mannan of Candida lusitaniae, antigenically related to Candida albicans serotype A

Shibata

Kobayashi

Okawa

et al. 2003

European Journal of Biochemistry

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The antigenicity of Candida lusitaniae cells was found to be the same as that of Candida albicans serotype A cells, i.e. both cell wall mannans react with factors 1, 4, 5, and 6 sera of Candida Check. However, the structure of the mannan of C. lusitaniae was significantly different from that of C. albicans serotype A, and we found novel b-1,2 linkages among the side-chain oligosaccharides, Manb1fi2Manb1fi 2Mana1fi2Mana1fi2Man (LM5), and Manb1fi2Man-b1fi2Manb1fi2Mana1fi2Mana1fi2Man (LM6). The assignment of these oligosaccharides suggests that the mannoheptaose containing three b-1,2 linkages obtained from the mannan of C. albicans in a preceding study consisted of isomers. The molar ratio of the side chains of C. lusitaniae mannan was determined from the complete assignment of its H-1 and H-2 signals and these signal dimensions. More than 80% of the oligomannosyl side chains contained b-1,2-linked mannose units; no a-1,3 linkages or a-1,6-linked branching points were found in the side chains. An enzyme-linked immunosorbent inhibition assay using oligosaccharides indicated that LM5 behaves as factor 6, which is the serotype A-specific epitope of C. albicans. Unexpectedly, however, LM6 did not act as factor 6.

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Synthesis and Immunological Screening of β‐Linked Mono‐ and Divalent Mannosides

et al. 2012

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Three different β‐linked divalent mannosides, along with their corresponding monovalent counterparts, have been designed and chemically synthesized by coupling the corresponding propargyl (propargyl alcohol in the case of the monovalent compounds) and 2‐azidoethyl glycosides by using an efficient click chemistry protocol. Crich's β‐mannosylation methodology was applied to the construction of the β‐mannosidic linkages. All the glycosylation reactions gave moderate‐to‐good yields with high selectivities. A competitive inhibition enzyme‐linked immunosorbent assay (ELISA) was performed to determine the inhibition, by the synthesized mannosides, of specific human IgG binding to low‐molecular‐weight Candida albicans mannan; moderate inhibition capacity was observed for some of the compounds.

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Mapping of Candida albicans oligomannosidic epitopes by using monoclonal antibodies

Cited by 64 publications

References 35 publications

Nature of Candida albicans-derived carbohydrate antigen recognized by a monoclonal antibody in patient sera and distribution over Candida species

Nature of Candida albicans-derived carbohydrate antigen recognized by a monoclonal antibody in patient sera and distribution over Candida species

Existence of novel β‐1,2 linkage‐containing side chain in the mannan of Candida lusitaniae, antigenically related to Candida albicans serotype A

Synthesis and Immunological Screening of β‐Linked Mono‐ and Divalent Mannosides

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