Effect of structural stability on endolysosomal degradation and T‐cell reactivity of major shrimp allergen tropomyosin

Kamath, Sandip D.; Scheiblhofer, Sandra; Johnson, Christopher M.; Machado, Yoan; McLean, Thomas R.; Taki, Aya C.; Ramsland, Paul A.; Iyer, Swati; Joubert, Isabella Anna; Hofer, Heidi; Wallner, Michael; Thalhamer, Josef; Rolland, Jennifer M.; O’Hehir, Robyn E; Briza, Peter; Ferreira, Fátima; Weiss, Richard; Lopata, Andreas L.

doi:10.1111/all.14410

Cited by 30 publications

(26 citation statements)

References 33 publications

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“…This is in line with the enhanced susceptibility to proteases of L89G observed in the degradome assay. We have previously found that immunodominant peptides from Bet v 1.0101 or tropomyosin (55,62) are quickly degraded in the degradome assay, but nevertheless are effectively presented by BMDCs in vitro, supporting the concept of "bind first, cut later." Kim et al have shown that immunodominant epitopes are protected from further degradation by binding to MHC II, whereas epitopes sensitive to DM-mediated dissociation are destroyed by cathepsins (57,63).…”

Section: Discussionmentioning

confidence: 63%

In silico Design of Phl p 6 Variants With Altered Fold-Stability Significantly Impacts Antigen Processing, Immunogenicity and Immune Polarization

et al. 2020

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Conclusion: MAESTRO software was very efficient in detecting single point mutations that increase or reduce fold-stability. Thermal stability correlated well with the speed of proteolytic degradation and presentation of peptides on the surface of dendritic cells in vitro. This change in processing kinetics significantly influenced the polarization of T cell responses in vivo. Modulating the fold-stability of proteins thus has the potential to optimize and polarize immune responses, which opens the door to more efficient design of molecular vaccines.

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Section: Discussionmentioning

confidence: 63%

In silico Design of Phl p 6 Variants With Altered Fold-Stability Significantly Impacts Antigen Processing, Immunogenicity and Immune Polarization

et al. 2020

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“…The blocked-nitrocellulose membrane was incubated overnight with a pooled serum from five shellfish-allergic patients ( Table 2 ) diluted 1:20 in PBST with added casein. After the washing step, secondary anti-human IgE (1:10,000 dilution, DAKO Corporation, Lincoln, NE, USA) was added and incubated for 1 h. The membrane was subsequently incubated for 35 min with donkey anti-rabbit IgG antibody conjugated infrared IRDye 800CW (1:10,000 dilution, LI-COR, Lincoln, NE, USA), and IgE antibody binding was visualised using the Odyssey ® CLx Imaging System (LI-COR Biosciences, Mulgrave, VIC, Australia) [ 17 ]. IgE reactive spots were annotated to the protein profile on SDS-PAGE, and corresponding bands cut out, tryptic digested and analysed using mass spectrometry.…”

Section: Methodsmentioning

confidence: 99%

Effects of Extraction Buffer on the Solubility and Immunoreactivity of the Pacific Oyster Allergens

Nugraha

Ruethers

Johnston

et al. 2021

Foods

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Despite recent technological advances, novel allergenic protein discovery is limited by their low abundance, often due to specific physical characteristics restricting their recovery during the extraction process from various allergen sources. In this study, eight different extraction buffers were compared for their ability to recover proteins from Pacific oyster (Crassostrea gigas). The protein composition was investigated using high resolution mass spectrometry. The antibody IgE-reactivity of each extract was determined using a pool of serum from five shellfish-allergic patients. Most of the investigated buffers showed good capacity to extract proteins from the Pacific oyster. In general, a higher concentration of proteins was recovered using high salt buffers or high pH buffers, subsequently revealing more IgE-reactive bands on immunoblotting. In contrast, low pH buffers resulted in a poor protein recovery and reduced IgE-reactivity. Discovery of additional IgE-reactive proteins in high salt buffers or high pH buffers was associated with an increase in allergen abundance in the extracts. In conclusion, increasing the ionic strength and pH of the buffer improves the solubility of allergenic proteins during the extraction process for oyster tissue. This strategy could also be applied for other difficult-to-extract allergen sources, thereby yielding an improved allergen panel for increased diagnostic efficiency.

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“…Even with this expanded understanding it is important to remember that exceptions will always exist. For instance, a survey of tropomyosin allergens from both food (Pen m 1, Shrimp; Ani s 3, fish parasite) and environmental (Der p 10, dust mite; Bla g 7, cockroach) sources revealed significant variation in both thermodynamic stability and endosomal degradation kinetics ( 110 ). However, neither measure of stability was found to correlate with allergenicity.…”

Section: Antigen Presentation Kinetics and Stability Influence Allerg...mentioning

confidence: 99%

Abundance and Stability as Common Properties of Allergens

Foo¹,

Mueller²

2021

Front. Allergy

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There have been many attempts to identify common biophysical properties which differentiate allergens from their non-immunogenic counterparts. This review will focus on recent studies which examine two such factors: abundance and stability. Anecdotal accounts have speculated that the elevated abundance of potential allergens would increase the likelihood of human exposure and thus the probability of sensitization. Similarly, the stability of potential allergens dictates its ability to remain a viable immunogen during the transfer from the source to humans. This stability could also increase the resilience of potential allergens to both gastric and endosomal degradation, further skewing the immune system toward allergy. Statistical analyses confirm both abundance and stability as common properties of allergens, while epidemiological surveys show a correlation between exposure levels (abundance) and allergic disease. Additional studies show that changes in protein stability can predictably alter gastric/endosomal processing and immunogenicity, providing a mechanistic link between stability and allergenicity. However, notable exceptions exist to both hypotheses which highlight the multifaceted nature of immunological sensitization, and further inform our understanding of some of these other factors and their contribution to allergic disease.

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Effect of structural stability on endolysosomal degradation and T‐cell reactivity of major shrimp allergen tropomyosin

Cited by 30 publications

References 33 publications

In silico Design of Phl p 6 Variants With Altered Fold-Stability Significantly Impacts Antigen Processing, Immunogenicity and Immune Polarization

In silico Design of Phl p 6 Variants With Altered Fold-Stability Significantly Impacts Antigen Processing, Immunogenicity and Immune Polarization

Effects of Extraction Buffer on the Solubility and Immunoreactivity of the Pacific Oyster Allergens

Abundance and Stability as Common Properties of Allergens

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