Comparative study of the commonly used protein quantitation assays on different Hymenoptera venoms: A fundamental aspect of Hymenoptera venom proteome analysis

Troy Wanandy; Simon A Handley; Emily Mulcahy; Michael Wiese

doi:10.1016/j.toxicon.2024.107685

Comparative study of the commonly used protein quantitation assays on different Hymenoptera venoms: A fundamental aspect of Hymenoptera venom proteome analysis

Toxicon. 2024 Apr:241:107685. doi: 10.1016/j.toxicon.2024.107685. Epub 2024 Mar 19.

Authors

Troy Wanandy¹, Simon A Handley², Emily Mulcahy³, Michael Wiese⁴

Affiliations

¹ Department of Clinical Immunology and Allergy, Incorporating the Jack Jumper Allergy Program, Royal Hobart Hospital, Hobart, Tasmania, Australia; College of Health and Medicine, University of Tasmania, Hobart, Tasmania, Australia. Electronic address: troy.wanandy@ths.tas.gov.au.
² College of Health and Medicine, University of Tasmania, Hobart, Tasmania, Australia; Department of Pathology, Royal Hobart Hospital, Hobart, Tasmania, Australia.
³ Department of Clinical Immunology and Allergy, Incorporating the Jack Jumper Allergy Program, Royal Hobart Hospital, Hobart, Tasmania, Australia; College of Health and Medicine, University of Tasmania, Hobart, Tasmania, Australia.
⁴ Clinical and Health Sciences, University of South Australia, Adelaide, South Australia, Australia.

PMID: 38503352
DOI: 10.1016/j.toxicon.2024.107685

Abstract

Determination of protein concentration in Hymenoptera venoms requires an accurate and reproducible assay as the results will be used to support subsequent proteomic techniques employed in their analyses. However, all protein assay techniques have inherent strengths and weaknesses, demanding their assessment before selecting the most suitable platform for sample analysis. In this study, protein profiles of ant, honeybee, and wasp venoms, and bovine serum albumin (BSA) and hyaluronidase standards were qualitatively assessed using sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE). Their amino acid and protein concentration were quantitatively determined via Amino Acid Analysis (AAA). Amino acid concentration was determined via hydrolysis, derivatization, and chromatographic quantification. Protein concentration was estimated using four different protein concentration assays. The ratios of protein concentration in venom samples to protein standards were calculated, and the accuracy of the protein concentration assays was analysed relative to the concentration determined from AAA. SDS-PAGE analysis showed that BSA contained several protein bands, while hyaluronidase contained a mixture of peptide and protein bands. Ant and honeybee venoms contained a higher proportion of peptide bands, while wasp venom contained more protein bands. As determined by AAA, the ratio of protein concentration in Hymenoptera venoms varied between 1.01 and 1.11 to BSA, and between 0.96 and 1.06 to hyaluronidase. Overall, the Bradford assay was found to be the least accurate and the BCA assay was the most accurate in estimating protein concentration in Hymenoptera venoms. There was no significant advantage in using hyaluronidase as a standard or increasing incubation temperature of BCA assay when analysing Hymenoptera venoms. Diluent solutions containing phenol and human serum albumin interfered with Lowry-based assays.

Keywords: Allergen specific immunotherapy; Hymenoptera venom; Protein quantitation assays.

MeSH terms

Allergens
Amino Acids
Animals
Arthropod Venoms*
Bee Venoms*
Bees
Humans
Hyaluronoglucosaminidase / analysis
Hymenoptera*
Peptides
Proteome
Proteomics
Serum Albumin, Bovine
Venoms
Wasp Venoms

Substances

Arthropod Venoms
Proteome
Hyaluronoglucosaminidase
Wasp Venoms
Venoms
Bee Venoms
Amino Acids
Serum Albumin, Bovine
Peptides
Allergens