Purification of Native Dentilisin Complex from Treponema denticola by Preparative Continuous Polyacrylamide Gel Electrophoresis and Functional Analysis by Gelatin Zymography

IF 1 Q3 BIOLOGY

Bio-protocol Pub Date : 2024-04-05 DOI:10.21769/BioProtoc.4970

P. Kamarajan, John C. Timm, M. Goetting-Minesky, Erin Malone, Sean Ganther, A. Radaic, Christian Tafolla, J. Fenno, Yvonne L Kapila

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Abstract

Periodontal disease is characterized by the destruction of the hard and soft tissues comprising the periodontium. This destruction translates to a degradation of the extracellular matrices (ECM), mediated by bacterial proteases, host-derived matrix metalloproteinases (MMPs), and other proteases released by host tissues and immune cells. Bacterial pathogens interact with host tissue, triggering adverse cellular functions, including a heightened immune response, tissue destruction, and tissue migration. The oral spirochete Treponema denticola is highly associated with periodontal disease. Dentilisin, a T. denticola outer membrane protein complex, contributes to the chronic activation of pro-MMP-2 in periodontal ligament (PDL) cells and triggers increased expression levels of activators and effectors of active MMP-2 in PDL cells. Despite these advances, no mechanism for dentilisin-induced MMP-2 activation or PDL cytopathic behaviors leading to disease is known. Here, we describe a method for purification of large amounts of the dentilisin protease complex from T. denticola and demonstrate its ability to activate MMP-2, a key regulator of periodontal tissue homeostasis. The T. denticola dentilisin and MMP-2 activation model presented here may provide new insights into the dentilisin protein and identify potential therapeutic targets for further research. Key features • This protocol builds upon a method described by Cunningham et al. [1] for selective release of Treponema outer membrane proteins. • We adapted the protocol for the purification of biologically active, detergent-stable outer membrane protein complexes from large batch cultures of T. denticola. • The protocol involves large-scale preparative electrophoresis using a Model 491 Prep Cell. • We then use gelatin zymography to demonstrate the activity of the purified dentilisin complex by its ability to activate matrix metalloproteinase 2 (MMP-2).

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用制备型连续聚丙烯酰胺凝胶电泳纯化牙形特雷霉素原生复合物并用明胶酶谱进行功能分析

牙周病的特点是构成牙周的软硬组织遭到破坏。这种破坏转化为细胞外基质（ECM）的降解，由细菌蛋白酶、宿主衍生的基质金属蛋白酶（MMPs）以及宿主组织和免疫细胞释放的其他蛋白酶介导。细菌病原体与宿主组织相互作用，引发不利的细胞功能，包括免疫反应增强、组织破坏和组织迁移。口腔螺旋体齿孢子菌与牙周病密切相关。牙体螺杆菌外膜蛋白复合物--牙体素可促使牙周韧带（PDL）细胞中的原 MMP-2 慢性活化，并引发 PDL 细胞中活性 MMP-2 的活化剂和效应物表达水平升高。尽管取得了这些进展，但目前尚不清楚牙本质素诱导 MMP-2 激活或 PDL 细胞病理行为导致疾病的机制。在这里，我们描述了一种从T.denticola中纯化大量牙质素蛋白酶复合物的方法，并证明了其激活MMP-2的能力，MMP-2是牙周组织稳态的关键调节因子。本文介绍的牙本质蜱牙本质蛋白和MMP-2激活模型可为牙本质蜱牙本质蛋白的研究提供新的视角，并为进一步研究确定潜在的治疗目标。主要特点--本方案基于 Cunningham 等人[1]描述的选择性释放特雷波纳菌外膜蛋白的方法。- 我们对该方案进行了调整，以便从大批量培养的齿孢子菌中纯化具有生物活性、去污剂稳定的外膜蛋白复合物。- 该方案包括使用 491 型预处理池进行大规模制备电泳。- 然后，我们使用明胶酶谱法通过激活基质金属蛋白酶 2（MMP-2）的能力来证明纯化的齿状菌素复合物的活性。

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来源期刊

Bio-protocol

CiteScore

1.50

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0.00%

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