Thai Vegetable Extracts Affecting Human Red Blood Cell Surface Antigens in the ABO Blood Group System

Abstract

Plant proteins capable of agglutinating human red blood cells (RBCs) extend beyond traditional lectins to include ribosome-inactivating proteins (RIPs), antimicrobial peptides (AMPs), and various defense proteins. While these proteins have been extensively studied in legumes, their presence and activity in common vegetables remain largely unexplored. Understanding their distribution and specificity could reveal novel tools for glycobiology and human ABO blood typing applications. This study aimed to evaluate the agglutination activity of nine Thai vegetable extracts against human red blood cells, determine their ABO blood group specificity, and assess the correlation between protein content and agglutination strength. Additionally, we sought to identify potential plant proteins contributing to the observed agglutination patterns. In this study, crude protein extracts were prepared from nine different vegetables using phosphate-buffered saline (PBS) with pH 7.4. Total protein concentration was quantified using the Biuret method. Agglutination assays were performed using standardized human RBC suspensions from different blood groups. The specificity and strength of agglutination were evaluated using serial dilutions under controlled conditions. Among the nine extracts tested, five demonstrated significant agglutinating activity with varying specificities. Three extracts (L. polychrous mushroom, mulberry leaf, and winged bean) showed non-specific agglutination across all blood groups, suggesting the presence of broadly reactive proteins. Notably, D. biflorusseed and lima bean extracts exhibited specific agglutination against blood group A, indicating potential blood-type-specific proteins. Four extracts (C. serratumleaf, cucumber, L. leucocephalaseed and long bean)showed no detectable agglutination activity. This study reveals previously unreported agglutinating activities in common vegetable extracts, with some showing blood group specificity. The diverse agglutination patterns observed suggest the presence of both lectin and non-lectin proteins with distinct binding properties. While these findings indicate potential applications in ABO blood typing and glycobiology research, further protein characterization and improved quantification methods are needed. Future studies should focus on isolating and identifying the specific proteins or lectin responsible for the observed agglutination patterns.