proenzyme
- n.酶原;前酶
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MMP-3 proenzyme protein expression could be detected in normal rat liver .
在正常大鼠肝组织中有MMP-3的酶原表达。
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Results Preparations of highly purified MBL and proenzyme MASPs were obtained .
结果获得高度纯化的MBL和酶原形式的MASP。
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AIM To investigate the dynamic alteration of gelatinase A ( metalloproteinase-2 , mmp-2 ) proenzyme protein expression in the process of experimental liver fibrosis .
目的研究实验性肝纤维化过程中明胶酶A(mmp-2)酶原蛋白表达的动态变化。
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Caspase-3 proenzyme is composed of one large-subunit and one small-subunit and only after being cut and activated can Caspase-3 perform its function .
该酶原由一个大亚基和一个小亚基组成,只有被切开并激活后Caspase-3才能够行使其功能。
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The carbon tetrachloride-induced hepatic fibrosis rat models were used . MMP-3 proenzyme protein expression in the different stages of liver fibrosis was measured by half quantitative analysis of Western blot .
建立四氯化碳中毒性大鼠肝纤维化模型,采用半定量Western免疫印迹方法,对肝纤维化不同阶段肝内MMP-3的酶原蛋白的表达水平进行了检测。
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Of the system , P0 is one of the important components ; it has two activities , MPO and DPO , and exists as proenzyme PPO in the insect .
其中,PO是PPO系统的关键成分之一,它是以酶原形式PPO存在于昆虫体内,具有MPO和DPO两种酶活性。
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MAIN OUTCOME MEASURE : cellular mitochondrial function , cellular caspase 9 and caspase 3 activity , release of mitochondrial CytC and cleavage of caspase 3 proenzyme .
主要观察指标:细胞线粒体功能、细胞内caspase-9和caspase-3活性、线粒体细胞色素C的释放和caspase-3酶原的降解。
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Splittings of synovial cell of rheumatoid arthritis and asparagic acid specific cysteine protease-3 proenzyme treated with resveratrol in various concentrations for 24 hours were studied with Western-blot method .
采用Western-blot分析不同浓度白藜芦醇处理24h的类风湿关节炎滑膜细胞,天冬氨酸特异性半胱氨酸蛋白酶3酶原的裂解。