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用可注射富血小板纤维蛋白生物功能化的异种胶原基质培养的THP-1单核细胞和巨噬细胞中环氧化酶COX-1和COX-2的表达及活性分析

Analysis of the Expression and Activity of Cyclooxygenases COX-1 and COX-2 in THP-1 Monocytes and Macrophages Cultured with Xenogenic Collagen Matrices Biofunctionalized with the Injectable Platelet-Rich Fibrin.

作者信息

Droździk Agnieszka, Barczak Katarzyna, Bosiacki Mateusz, Kupnicka Patrycja, Cenariu Diana, Uriciuc Willi Andrei, Chlubek Dariusz, Lipski Mariusz, Droździk Marek, Baranowska-Bosiacka Irena

机构信息

Laboratory of Preclinical Periodontology, Pomeranian Medical University in Szczecin, Powstańców Wlkp 72, 70-111 Szczecin, Poland.

Department of Conservative Dentistry and Endodontics, Pomeranian Medical University in Szczecin, Powstańców Wlkp 72, 70-111 Szczecin, Poland.

出版信息

Int J Mol Sci. 2025 May 5;26(9):4386. doi: 10.3390/ijms26094386.

Abstract

Xenogenic collagen matrices are used in clinical practice for soft tissue augmentation around teeth and implants, either alone or biofunctionalized with injectable platelet-rich fibrin (iPRF). Their direct interaction with inflammatory cells may influence both healing and destructive inflammation processes. Therefore, expression of cyclooxygenases (COX-1 and COX-2) and prostanoids (PGE2 and TXB2) was studied in THP-1 monocyte/macrophage cultures exposed to porcine collagen matrices (a non-cross-linked monolayer scaffold composed of collagen type I, collagen type III, and elastin (MLCM), a bilayer scaffold made of collagen types I and III (BLCM), and a volume-stable cross-linked monolayer scaffold (VSCM)). The study showed that VSCM and MLCM significantly reduced PGE2 concentrations in THP-1 monocyte cultures. iPRF further reduced PGE2 concentrations when exposed to MLCM. In contrast, incubation of THP-1 monocytes with VSCM and BLCM resulted in a significant increase in TXB2 concentrations compared with control conditions. Incubation of macrophages with MLCM, VSCM, and BLCM increased PGE2 concentrations, with VSCM and BLCM additionally increasing TXB2 concentrations. iPRF in macrophage cultures with VSCM and BLCM also resulted in increased PGE2 and TXB2 concentrations compared with control conditions. Confocal microscopy revealed no visible differences in COX-1 immunoexpression in monocytes and macrophages cultured with collagen matrices, either with or without iPFR. Weak positive COX-2 immunofluorescence was observed in monocytes, while moderate positive immunofluorescence was detected in macrophages. In conclusion, it can be suggested that the studied collagen matrices interact with monocytes/macrophages, with MLCM exhibiting the highest compatibility.

摘要

异种胶原基质在临床实践中用于牙齿和种植体周围的软组织增量,可单独使用,也可与可注射富血小板纤维蛋白(iPRF)进行生物功能化处理。它们与炎症细胞的直接相互作用可能会影响愈合和破坏性炎症过程。因此,在暴露于猪胶原基质(一种由I型胶原、III型胶原和弹性蛋白组成的非交联单层支架(MLCM)、一种由I型和III型胶原制成的双层支架(BLCM)以及一种体积稳定的交联单层支架(VSCM))的THP-1单核细胞/巨噬细胞培养物中,研究了环氧化酶(COX-1和COX-2)和前列腺素(PGE2和TXB2)的表达。研究表明,VSCM和MLCM显著降低了THP-1单核细胞培养物中的PGE2浓度。当暴露于MLCM时,iPRF进一步降低了PGE2浓度。相比之下,与对照条件相比,用VSCM和BLCM孵育THP-1单核细胞导致TXB2浓度显著增加。用MLCM、VSCM和BLCM孵育巨噬细胞会增加PGE2浓度,VSCM和BLCM还会增加TXB2浓度。与对照条件相比,在含有VSCM和BLCM的巨噬细胞培养物中加入iPRF也会导致PGE2和TXB2浓度增加。共聚焦显微镜显示,在用胶原基质培养的单核细胞和巨噬细胞中,无论有无iPFR,COX-1免疫表达均无明显差异。在单核细胞中观察到弱阳性的COX-2免疫荧光,而在巨噬细胞中检测到中度阳性免疫荧光。总之,可以认为所研究的胶原基质与单核细胞/巨噬细胞相互作用,其中MLCM表现出最高的相容性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c0ed/12073069/f02fa8ff4283/ijms-26-04386-g001a.jpg

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