Analysis of the cross-reactivity and of the 1.5 Å crystal structure of the <i>Malassezia sympodialis</i> Mala s 6 allergen, a member of the cyclophilin pan-allergen family

Glaser, Andreas; Limacher, Andreas; Flückiger, Sabine; Scheynius, Annika; Scapozza, Léonardo; Crameri, Reto

doi:10.1042/bj20051708

Cited by 66 publications

(75 citation statements)

References 36 publications

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“…Therefore it can be concluded that the Asp f 9 cDNA sequence is correct, and that the published Asp f 16 peptide sequence results from frameshift, other sequencing errors, or derives from a different A. fumigatus strain; (iii) Asp f 17, originally described as a cDNA encoding a 191 amino acid protein [24], is incomplete and the complete gene encodes a protein of 284 amino acids; and (iv) the postulated sequence of the Asp f 56 kDa allergen not included in the official allergen database, which was derived from a short peptide obtained from a biochemically purified protein [28] is not predicted to be encoded in any of the sequenced Aspergillus genomes. All other A. fumigatus allergens reported in the official allergen database as well as the sequences of the recently cloned thioredoxins (Asp f 28, Asp f 29) [29], cyclophilins (Asp f 11, Asp f 27) [30], and Phi A cell wall protein (Asp f 34, Glaser unpublished) sequences showed virtually a 100% identity with the genome sequence, confirming at genomic level the validity of cDNA cloning approaches for the elucidation of allergen repertoires. The whole repertoire of A. fumigatus allergens included in the official allergen list reported in Table 2 have been produced as highly pure recombinant allergens and evaluated for their IgE-binding capacity in vitro.…”

Section: The Allergen Repertoire Of Aspergillus Fumigatusmentioning

confidence: 83%

“…However, only three crystal structures derived from fungal allergens, ribotoxin (Asp f 1) [45, 46], MnSOD (Asp f 6) [65] from A. fumigatus and a Xylanase from Paecilomyces variotii [66] have been reported so far. Recently the crystal structures of a cyclophilin of A. fumigatus (Asp f 11) [61] and Malassezia sympodialis (M. sympodialis) (Mala s 6) [30], as well as the crystal structure of thioredoxin of M. sympodialis (Mala s 13) [29], and Mala s 1, a major allergen of M. sympodialis with unknown function [67] have been determined at high resolution.…”

Section: Structural Aspects Of Fungal Allergensmentioning

confidence: 99%

“…Interestingly some of these proteins show cross-reactivity also with their homologous human proteins at both, humoral and cellular level. The best investigated structures at this level are human MnSOD [57,58], cyclophilin [30,61] and thioredoxin [29], which were shown to bind to serum IgE from A. fumigatus sensitised patients in vitro, to elicit specific skin test reactions in vivo, and to be potentially involved in the pathogenesis of ABPA and atopic eczema [18,63]. Although the role played by IgE-mediated autoreactivity to self-antigens remains controversial, the fact that the application of human MnSOD in patch test on healthy skin areas of atopic eczema patients sensitised to fungal MnSOD is sufficient to induce an eczematous reaction [57,63] strongly indicates that autoreactivity could contribute to the exacerbation of the symptoms in the absence of external exposure to environmental allergens.…”

Section: Cross-and Autoreactivitymentioning

confidence: 99%

“…The whole repertoire of A. fumigatus allergens included in the official allergen list reported in Table 2 have been produced as highly pure recombinant allergens and evaluated for their IgE-binding capacity in vitro. The majority of these proteins have also been tested for their ability to elicit positive skin tests in vivo [27,[29][30][31][32].…”

Section: The Allergen Repertoire Of Aspergillus Fumigatusmentioning

confidence: 99%

“…Basically cross-reactivity can be traced back to conserved proteins sharing common B and T cell epitopes as shown for many allergen structures [33]. Amongst these MnSOD (Asp f 6) [57,58], P 2 acidic ribosomal protein (Asp f 8) [59], cyclophilins (Asp f 11 and Asp f 27) [30,60,61] and thioredoxins (Asp f 28 and Asp f 29) [29] have been shown to belong to families of cross-reactive pan-allergens. Per definition pan-allergens share a high degree of sequence identity at primary structure level, thus belonging to protein families showing similar structural folding [33,62].…”

Section: Cross-and Autoreactivitymentioning

confidence: 99%

See 4 more Smart Citations

Overview of Aspergillus Allergens

Crameri¹,

Glaser²,

Vilhelmsson

et al. 2009

Aspergillosis: From Diagnosis to Prevention

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Fungi in general and, Aspergillus fumigatus (A. fumigatus) in particular, are able to produce complex patterns of IgE-binding molecules. Robotics-based high throughput screening of A. fumigatus cDNA libraries displayed on phage surfaces revealed at last 81 different sequences encoding structures potentially able to bind to serum IgE of sensitised individuals suffering from A. fumigatus-related complications. Although not all of these allergens have been characterised in detail, A. fumigatus still represents the best investigated allergenic source. A total of 23 A. fumigatus allergens are recorded by the official allergen list of the International Union of Immunological Societies ( www.allergen.org ) and this is by far the longest allergen list reported for a single allergenic source. The IgE-binding molecules include species-specific as well as phylogenetically highly conserved cross-reactive structures and such with unknown function. A subset of cDNAs have been used to produce and characterise the corresponding recombinant allergens which have proven to be useful diagnostic reagents allowing specific detection of A. fumigatus sensitisation and differential diagnosis of allergic bronchopulmonary aspergillosis. Structures highly conserved through different species like manganese-dependent superoxide dismutase, P 2 acidic ribosomal protein, cyclophilins and thioredoxins induce, beyond sensitisation, IgE antibodies able to cross-react with the corresponding homologous self-antigens. The frequently observed cross-reactivity is traceable back to shared discontinuous B-cell epitopes as shown by detailed analyses of the crystal structures.

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Section: The Allergen Repertoire Of Aspergillus Fumigatusmentioning

confidence: 83%

Section: Structural Aspects Of Fungal Allergensmentioning

confidence: 99%

Section: Cross-and Autoreactivitymentioning

confidence: 99%

Section: The Allergen Repertoire Of Aspergillus Fumigatusmentioning

confidence: 99%

Section: Cross-and Autoreactivitymentioning

confidence: 99%

See 3 more Smart Citations

Overview of Aspergillus Allergens

Crameri¹,

Glaser²,

Vilhelmsson

et al. 2009

Aspergillosis: From Diagnosis to Prevention

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show abstract

The Role of Fungal Agents in Atopic Dermatitis

Bond

2013

Veterinary Allergy

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In silico tools to assess the potential allergenicity of shiitake mushrooms (Lentinula edodes)

et al. 2022

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BACKGROUND Computational tools may have an edge over conventional methods for the preliminary evaluation of food allergenicity. In this study, the allergenic potential of Lentinula edodes was evaluated and validated using in silico tools. RESULTS The potential cross‐reactivity of mushroom proteins with fungal allergens was determined using sequence alignment – the Fast Alignment (FASTA) and Basic Local Alignment Search Tool (BLAST) algorithm. Eight L. edodes proteins were cross‐reactive with allergens from fungal origin, showing 52%–89% sequence identity using FASTA algorithm‐based alignment. The BLAST data were corroborated by percentage identity and query coverage. Physico‐chemical property‐based allergenicity was deciphered by AlgPred, Allermatch, and AllergenFP software, which predicted six out of eight proteins as potential allergens. Sequence alignment showed 66%–86% conservancy between mushroom protein and known fungal allergens. Secondary structure and amino acid composition supported structural affinity between query and fungal proteins. Three‐dimensional structures of five mushroom proteins were generated, quality assessed, and superimposed with fungal allergens, suggesting possible allergenicity of mushroom proteins. An enzyme‐linked immunosorbent assay (ELISA) demonstrated immunoglobulin E (IgE) binding in 13 out of 21 food‐hypersensitive patients' sera. CONCLUSION In silico tools provide preliminary indications about the potential allergenicity and cross‐reactivity of mushroom proteins. This approach may be used for the prelusive allergenicity assessment of allergen sources. © 2022 Society of Chemical Industry.

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Analysis of the cross-reactivity and of the 1.5 Å crystal structure of the Malassezia sympodialis Mala s 6 allergen, a member of the cyclophilin pan-allergen family

Cited by 66 publications

References 36 publications

Overview of Aspergillus Allergens

Overview of Aspergillus Allergens

The Role of Fungal Agents in Atopic Dermatitis

In silico tools to assess the potential allergenicity of shiitake mushrooms (Lentinula edodes)

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