Phagocytosis by Immune Cells of Protein-Modified Polymer Microparticles

Q4 Biochemistry, Genetics and Molecular Biology

Cell and Tissue Biology Pub Date : 2023-12-11 DOI:10.1134/s1990519x23060123

R. G. Sakhabeev, D. S. Polyakov, N. A. Grudinina, O. I. Antimonova, V. A. Korzhikov-Vlakh, E. R. Alikparova, E. S. Sinitsina, M. M. Shavlovsky

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Abstract

The present work was aimed at studying the ability of three model green proteins to covalently bind to microparticles (MPs) based on poly(D,L-lactic acid) (PLA). Green fluorescent protein (sfGFP), the fusion protein of recombinant human β2-microglobulin (β2M) with sfGFP (β2M–sfGFP) and the fusion protein of recombinant human amylin (IAPP) with sfGFP (IAPP–sfGFP) were isolated using affinity chromatography. MP–PLAs were formed by the double-emulsion method. The modification of MP–PLAs by protein was confirmed by laser scanning microscopy (LSM). In addition, LSM was used to study the phagocytosis of MP–PLA modified by different proteins and free model proteins by macrophages. Recombinant sfGFP was shown to binds to the surface of particles at lower amounts compared to β2M–sfGFP and IAPP–sfGFP. This is probably due to the fact that protein amino groups that could potentially react with activated carboxyl groups on the surface of particles are sterically inaccessible for this reaction because of the sfGFP structure. The β2M and IAPP proteins, being components of the respective recombinant fusion proteins, are spacer structures between the surface of spherical particles and sfGFP. It was established that a threefold increase in the protein/particles ratio did not lead to an increase in the bound protein per unit of particle mass, which may indicate the amount of protein that can be bound per unit of particle mass is limited by the capacity of particles themselves. The study of phagocytosis of protein-modified MP–PLAs has shown that MP–PLAs containing model proteins (β2M–sfGFP and IAPP–sfGFP) on their surface are successfully phagocytized by macrophages and, thereby, can contribute to the activation of cell-mediated immune response, which is important for controlling various, including viral, infections. Phagocytosis of model proteins (β2M–sfGFP, IAPP–sfGFP) has also been shown in the present work. This may be due to the fact that both β2M and IAPP are amyloidogenic and aggregation-prone proteins. In all likelihood, the aggregates of these proteins can be absorbed by macrophages due to the increased size compared to their monomeric forms.

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免疫细胞对蛋白质改性聚合物微粒的吞噬作用

摘要本研究旨在研究三种模型绿色蛋白与基于聚乳酸（PLA）的微颗粒（MPs）共价结合的能力。利用亲和层析法分离了绿色荧光蛋白（sfGFP）、重组人β2-微球蛋白（β2M）与sfGFP的融合蛋白（β2M-sfGFP）和重组人淀粉样蛋白（IAPP）与sfGFP的融合蛋白（IAPP-sfGFP）。采用双乳液法形成了 MP-PLA。激光扫描显微镜（LSM）证实了蛋白质对 MP-PLAs 的修饰。此外，还利用激光扫描显微镜研究了巨噬细胞对经不同蛋白质修饰的 MP-PLA 和游离的模型蛋白质的吞噬作用。与β2M-sfGFP和IAPP-sfGFP相比，重组sfGFP与颗粒表面的结合量较低。这可能是因为由于 sfGFP 的结构，可能与颗粒表面活化的羧基发生反应的蛋白质氨基在这种反应中是立体不可及的。作为各自重组融合蛋白的成分，β2M 和 IAPP 蛋白是球形颗粒表面与 sfGFP 之间的间隔结构。研究发现，蛋白质/颗粒比率增加三倍并不会导致单位颗粒质量结合蛋白质的增加，这可能表明单位颗粒质量可结合的蛋白质量受到颗粒本身容量的限制。对蛋白质修饰的 MP-PLAs 的吞噬作用的研究表明，表面含有模型蛋白质（β2M-sfGFP 和 IAPP-sfGFP）的 MP-PLAs 能被巨噬细胞成功吞噬，从而有助于激活细胞介导的免疫反应，这对控制各种感染（包括病毒感染）非常重要。本研究还显示了模型蛋白（β2M-sfGFP、IAPP-sfGFP）的吞噬作用。这可能是由于 β2M 和 IAPP 都是淀粉样蛋白和易聚集蛋白。与单体形式相比，这些蛋白质的聚集体体积增大，因此很有可能被巨噬细胞吸收。

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来源期刊

Cell and Tissue Biology Biochemistry, Genetics and Molecular Biology-Cell Biology

CiteScore

0.80

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0.00%

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期刊介绍： The journal publishes papers on vast aspects of cell research, including morphology, biochemistry, biophysics, genetics, molecular biology, immunology. The journal accepts original experimental studies, theoretical articles suggesting novel principles and approaches, presentations of new hypotheses, reviews highlighting major developments in cell biology, discussions. The main objective of the journal is to provide a competent representation and integration of research made on cells (animal and plant cells, both in vivo and in cell culture) offering insight into the structure and functions of live cells as a whole. Characteristically, the journal publishes articles on biology of free-living and parasitic protists, which, unlike Metazoa, are eukaryotic organisms at the cellular level of organization.