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Identification and characterization of gelatinases/type IV collagenases in jaw cysts.

机译:颌囊肿中明胶酶/型IV胶原酶的鉴定与表征。

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摘要

The molecular mechanisms of jaw cyst expansion probably involve interactions of matrix metalloproteinases (MMPs) and the tissue inhibitors of MMPs (TIMPs). In this study, molecular species of gelatinases present in neutral salt extracts of cyst walls and cyst fluids were characterized by functional activity measurements (type I gelatin and alpha-casein zymography) and immunologically (Western-blotting). The effects of various protein thiol-group or cysteine-switch reactants involved in the activation of collagenases were studied on cyst gelatinases and a gelatinases purified from human gingival fibroblasts (72 kD MMP-2), gingival keratinocytes (92 kD MMP-9) and polymorphonuclear neutrophilic leukocytes (92 kD MMP-9). Western-blotting revealed the presence of both 92 kD (MMP-9) and 72 kD (MMP-2) gelatinases in cyst wall extracts and cyst fluids. Western-blot studies further suggested that jaw cyst gelatinases were only in part complexed with and thus inhibited by TIMP-1 or TIMP-2, suggesting that both MMP-9 and MMP-2 may participate in cyst expansion. MMP-2 was also partially fragmented to a 68 kD form and additional lower molecular weight proteinases (< 60 kD) were detected by alpha-casein zymography and by Western-blotting, suggesting proteolytic fragmentation. MMP-9 was at least partially activated by all protein-thiol group reactants and rather resistant to oxidative inhibition by hypochlorite (NaOCl); in contrast, MMP-2 was activated by APMA but not at all by gold thioglucose (GTG) and was clearly inactivated by hypochlorite (NaOCl).(ABSTRACT TRUNCATED AT 250 WORDS)
机译:颌骨囊肿膨胀的分子机制可能涉及基质金属蛋白酶(MMP)的相互作用和MMPS(TIMPS)的组织抑制剂。在该研究中,通过功能活性测量(I型明胶和α-酪蛋白酶谱)和免疫(Western-Blotting),表征存在于囊壁和囊液中的中性盐提取物中的凝胶酶的分子种。在囊肿凝胶酶上研究各种蛋白质硫醇组或半胱氨酸开关反应物的效果在囊肿凝胶酶上和从人牙龈成纤维细胞(72kd mmp-2)纯化的明胶酶,牙龈角质形成细胞(92kd mmp-9)和凝胶酶多核核细胞白细胞(92kd mmp-9)。 Western-Blotting揭示了92kd(MMP-9)和72kD(MMP-2)明胶酶的存在,囊壁提取物和囊肿流体。蛋白质印迹研究进一步表明颌囊肿凝胶酶仅部分络合,因此抑制了TIMP-1或TIMP-2,表明MMP-9和MMP-2都可以参与囊肿膨胀。 MMP-2还部分地将68kD形式分割成68kd形式,并通过α-酪蛋白酶谱检测额外的较低分子量蛋白酶(<60kd),并通过蛋白质印迹检测蛋白水解碎片。 MMP-9至少部分地由所有蛋白质-Chiol基团反应物激活,并且抗氯酸盐(NaOCl)抵抗氧化抑制;相比之下,MMP-2通过APMA活化,但不受金硫葡聚糖(GTG)并不通过次氯酸盐(NAOCL)灭活。(抽象截断为250字)

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