Abstract
Although the activation of pathogen phagocytosis via complement system has been studied, erythrocyte-phagocyte interactions in pigs are not clearly understood. Therefore, we sought to investigate the ability of porcine erythrocytes to clear immune complexes (ICs) by using laser confocal microscopy and flow cytometry to observe the immune adhesion of porcine erythrocytes to fluorescent bacilli and the immune presentation process of transferring fluorescent bacilli to macrophages. Isolated porcine alveolar macrophages (PAMs) had uniform morphology and size, and a survival rate of 97.2%. The phagocytosis rate was 98.8%. After WT E. coli was labeled with Fluorescein Isothiocyanate (FITC), the bacteria showed a bright green fluorescence, and the labeling rate was 92.3%. When laser confocal microscopy was utilized to observe the co-incubation system of porcine erythrocytes, PAM, and fluorescent E. coli, the fluorescence intensity of bacilli decreased with increasing observation time and even disappeared. Flow Cytometry examination showed that the average fluorescence intensity of PAMs co-incubated with porcine erythrocytes adhered to WT-E. coli-FITC, was significantly higher than that of normal PAMs. Furthermore, when porcine erythrocytes adhered to WT E. coli were incubated with PAMs, the surface mean fluorescence intensity of porcine erythrocytes was significantly higher than that of the blank control group. This shows that PAMs can competitively bind to the oposinized E. coli adhered to the surface of porcine erythrocytes, and these oposinized pathogens can enter macrophages by the process of phagocytosis, which promoting the internalization of ICs or pathogens. During this process, the physical morphology of porcine erythrocytes was not damaged, but the levels of its main functional protein CR1-like were reduced.
Highlights
Immune adherence is the most important immune function of human erythrocytes
Ink phagocytosis test result Porcine alveolar macrophages obtained after isolation were allowed to revive and were cultured
WT E. coli were successfully labeled with Fluorescein Isothiocyanate (FITC) After WT E. coli were labeled with FITC dye, they were placed under a direct microscope
Summary
Immune adherence is the most important immune function of human erythrocytes. The molecular basis and mechanism of the erythrocyte immune adherence have been well studied in biomedicine. The results confirmed that changes of erythrocyte immune adherence function are highly correlated with the occurrence, development, outcome, and immune status of the diseases (Khera & Das, 2009). How to cite this article Yin W, Wang C, Fan K, Sun N, Sun Y, Li H. In vitro observation: the GFP-E. coli adhering to porcine erythrocytes can be removed by porcine alveolar macrophages.
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