Department of Chemical Engineering, Faculty of Engineering and Applied Sciences, Queen's University, Kingston, ON, Canada.
Centre for Health Innovation, Queen's University and Kingston Health Sciences, Kingston, ON, Canada.
Front Immunol. 2023 Aug 24;14:1232586. doi: 10.3389/fimmu.2023.1232586. eCollection 2023.
The adsorbed protein layer on an implanted biomaterial surface is known to mediate downstream cell-material interactions that drive the host response. While the adsorption of plasma-derived proteins has been studied extensively, the adsorption of damage-associated molecular patterns (DAMPs) derived from damaged cells and matrix surrounding the implant remains poorly understood. Previously, our group developed a DAMP-adsorption model in which 3T3 fibroblast lysates were used as a complex source of cell-derived DAMPs and we demonstrated that biomaterials with adsorbed lysate potently activated RAW-Blue macrophages via Toll-like receptor 2 (TLR2). In the present study, we characterized the response of mouse bone marrow derived macrophages (BMDM) from wildtype (WT), TLR2 and MyD88 mice on Teflon™ AF surfaces pre-adsorbed with 10% plasma or lysate-spiked plasma (10% w/w total protein from 3T3 fibroblast lysate) for 24 hours. WT BMDM cultured on adsorbates derived from 10% lysate in plasma had significantly higher gene and protein expression of IL-1β, IL-6, TNF-α, IL-10, RANTES/CCL5 and CXCL1/KC, compared to 10% plasma-adsorbed surfaces. Furthermore, the upregulation of pro-inflammatory cytokine and chemokine expression in the 10% lysate in plasma condition was attenuated in TLR2 and MyD88 BMDM. Proteomic analysis of the adsorbed protein layers showed that even this relatively small addition of lysate-derived proteins within plasma (10% w/w) caused a significant change to the adsorbed protein profile. The 10% plasma condition had fibrinogen, albumin, apolipoproteins, complement, and fibronectin among the top 25 most abundant proteins. While proteins layers generated from 10% lysate in plasma retained fibrinogen and fibronectin among the top 25 proteins, there was a disproportionate increase in intracellular proteins, including histones, tubulins, actins, and vimentin. Furthermore, we identified 7 DAMPs or DAMP-related proteins enriched in the 10% plasma condition (fibrinogen, apolipoproteins), compared to 39 DAMPs enriched in the 10% lysate in plasma condition, including high mobility group box 1 and histones. Together, these findings indicate that DAMPs and other intracellular proteins readily adsorb to biomaterial surfaces in competition with plasma proteins, and that adsorbed DAMPs induce an inflammatory response in adherent macrophages that is mediated by the MyD88-dependent TLR2 signaling pathway.
植入生物材料表面的吸附蛋白层被认为介导下游细胞与材料相互作用,从而驱动宿主反应。虽然已经广泛研究了血浆衍生蛋白的吸附,但来自受损细胞和植入物周围基质的损伤相关分子模式 (DAMP) 的吸附仍知之甚少。以前,我们的小组开发了一种 DAMP 吸附模型,其中 3T3 成纤维细胞裂解物被用作细胞来源 DAMP 的复杂来源,我们证明了吸附了裂解物的生物材料通过 Toll 样受体 2 (TLR2) 强烈激活 RAW-Blue 巨噬细胞。在本研究中,我们表征了来自野生型 (WT)、TLR2 和 MyD88 小鼠的骨髓来源巨噬细胞 (BMDM) 在预先吸附了 10%血浆或含 10%w/w 3T3 成纤维细胞裂解物总蛋白的裂解物加血浆 (lysate-spiked plasma) 的特氟龙 (Teflon)™ AF 表面上的反应 24 小时。在吸附物上培养的 WT BMDM 来自 10%lysate 的基因和蛋白表达水平血浆中的表达显著高于 10%血浆吸附表面。此外,在 TLR2 和 MyD88 BMDM 中,10%lysate in plasma 条件下促炎细胞因子和趋化因子表达的上调减弱。吸附蛋白层的蛋白质组学分析表明,即使在血浆中添加相对较小量的裂解物衍生蛋白(10%w/w),也会导致吸附蛋白谱发生显著变化。10%血浆条件下,纤维蛋白原、白蛋白、载脂蛋白、补体和纤维连接蛋白是前 25 种最丰富的蛋白质之一。虽然来自 10%lysate 的蛋白质层在血浆中保留了纤维蛋白原和纤维连接蛋白前 25 种蛋白质之一,但细胞内蛋白质,包括组蛋白、微管蛋白、肌动蛋白和波形蛋白的比例显著增加。此外,我们在 10%血浆条件下鉴定了 7 种 DAMPs 或与 DAMP 相关的蛋白质(纤维蛋白原、载脂蛋白),而在 10%lysate 的血浆条件下鉴定了 39 种 DAMPs,包括高迁移率族框 1 和组蛋白。总之,这些发现表明 DAMPs 和其他细胞内蛋白质很容易与血浆蛋白竞争吸附在生物材料表面上,并且吸附的 DAMPs 通过 MyD88 依赖性 TLR2 信号通路诱导粘附巨噬细胞的炎症反应。
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