胶原纤维负载金属离子材料的制备及其吸附水中氟离子的作用机制

利用胶原纤维和几种金属盐制备了胶原纤维负载金属离子(MICF)的新型除氟材料,同时对其吸附水溶液中氟离子进行比较实验。结果表明胶原纤维负载锆(Ⅲ)(ZrCF)对氟的吸附性能较好,在4.0～9.0的pH范围内其吸附效应与离子强度基本无关,常见阴离子(Cl-,NO3-,SO24-)的存在对氟的吸附也未显示出干扰效应。通过扫描电子显微镜(SEM)、表面电荷、红外光谱(IR)对ZrCF的形态、性质和吸附机制进行了表征和探讨。SEM观察到金属离子均匀分散在胶原纤维上;用固相分布法测得ZrCF的等电点升高至9.0;结合吸附前后溶液pH变化和IR表征揭示了氟离子在ZrCF上的吸附以配位交换过程为主,吸附中Zr(Ⅳ)金属氧化物表面羟基与氟离子形成配位络合物,释放出H+。

胶原蛋白肽金属螯合物及其生产制备工艺的研究进展

胶原蛋白肽金属螯合物是胶原蛋白肽与金属离子通过配位共价结合或吸附结合方式形成的螯合物。该螯合物作为金属矿物元素补充剂,具有生物利用率高、安全性高、生物活性高等优点。综述了胶原蛋白肽金属螯合物的螯合机理、稳定性、吸收利用、功能活性和生产制备工艺并展望了其开发应用前景,以期为相关研究提供参考。

祛瘀生肌法对实验性创面肉芽组织中Ⅰ、Ⅲ型胶原和MMP-1 mRNA表达的动态影响

目的探讨祛瘀生肌法在创面修复早、中期对实验性创面新生肉芽组织中Ⅰ、Ⅲ型胶原和胶原金属蛋白酶-1(MMP-1)mRNA表达的影响。方法采用Northem blot杂交法对大鼠创面肉芽组织中MMP- 1和Ⅰ、Ⅲ型胶原mRNA在创面修复早期和中期表达进行检测。结果创面修复初期(3天)和中期(10天)对比,生肌化瘀组MMP-1的mRNA表达明显降低；Ⅰ、Ⅲ型胶原mRNA表达无明显变化。模型组MMP-1的mRNA表达无明显变化；Ⅰ、Ⅲ型胶原mRNA表达明显下降。结论祛瘀生肌法对实验性创面新生肉芽组织中Ⅰ、Ⅲ型胶原和MMP-1 mRNA表达的影响是其促进创面修复的机理之一。

厄贝沙坦对糖尿病大鼠肺脏组织中胶原和基质金属蛋白酶相关因子的影响

目的观察厄贝沙坦是否对抗糖尿病大鼠肺损伤,探讨大鼠肺组织胶原和基质金属蛋白酶(MMPs)通路中相关因子的变化。方法雄性SD大鼠随机分为对照组(NC)、T2DM组、厄贝沙坦+糖尿病组(Ir+T2DM)。8周后测定各组FPG、TG和TC,HE和Masson染色观察肺组织形态、纤维化改变。ELISA测定肺组织MMP-2、MMP-9、TIMP-1和TIMP-2含量,Western blot检测MT1-MMP蛋白的表达。结果与NC组比较,T2DM组FPG、TG和TC水平增高,肺泡结构大部分消失,胶原增生,肺组织MMP-2、MMP-9水平下降,TIMP-1、TIMP-2水平升高,MT1-MMP蛋白表达较NC组增加(P<0.05或P<0.01)。与T2DM组比较,Ir+T2DM组肺组织形态和纤维增生改善,MMP-2、MMP-9水平增加,TIMP-1、TIMP-2水平降低,MT1-MMP蛋白表达降低(P<0.05)。结论 T2DM可诱导肺脏损伤,厄贝沙坦通过调节MMPs信号通路中的相关因子,减轻肺损伤。

Effects of fibril- or fixed-collagen on matrix metalloproteinase-1 and tissue inhibitor of matrix metalloproteinase-1 production in the human hepatocyte cell line HLE

AIM:Matrix metalloproteinase-1 (MMP-1) and tissue inhibitor of matrix metalloproteinase-1 (TIMP-1) are central to the spontaneous resolution of liver fibrosis. The mechanisms involved have been investigated in hepatic stellate cells (HSC), but not in hepatocytes. We investigated the effects of fibril- and fixed-collagen on MMP-1 and TIMP-1 production in hepatocytes, using the HLE cell line. METHODS: Fibril type I and IV collagen were prepared by HCI digestion of type I and IV collagen, respectively. For fixed-collagen, culture dishes were coated with fibril type I or IV collagen and fixed by ultraviolet. Type I collagenase activity was measured using fluorescein isothiocyanate-labeled type I collagen. MMP-1 and TIMP-1 in HLE cells were measured by a one-step sandwich enzyme immunoassay. RESULTS: Both fibril type I and IV collagen significantly increased type I collagenase activity about two-fold compared with no fibril collagen. The effects of the fibril collagen were not affected by the coating condition. There was no significant difference in the effects on collagenase activity between cells cultured in medium containing fibril type I collagen and those cultured in the presence of type IV collagen. Both types of fibril collagen significantly increased MMP-1 production, and showed more than 10-fold higher levels of MMP-1 than the control. The enhanced MMP-1 production by fibril collagens was unaffected by the coating condition. By contrast, TIMP-1 production was not changed by the addition of fibril type I or IV collagen, and neither was it affected by the coating conditions. Coating with type I collagen significantly suppressed MMP-1 production by almost one-tenth compared with no coating. By contrast, TIMP-1 production was not affected by either the absence of a collagen coat or by increasing the concentration of the coating collagen. CONCLUSION: These results indicated that, in HLE cells, fibril- and fixed-collagen have opposite effects on MMP-1 production without affecting TIMP production. Fibril collagen induced collagenase activity by up-regulation of MMP-1 production without affecting TIMP-1 production. By contrast, fixed collagen reduced MMP-1 production. Our results suggest that hepatocytes might also play an important role in the regulation of the hepatic fibrosis alongside HSC.