Lang John D, Figueroa Mario, Chumley Phillip, Aslan Mutay, Hurt John, Tarpey Margaret M, Alvarez Beatriz, Radi Rafael, Freeman Bruce A
Department of Anesthesiology and Center for Free Radical Biology, The University of Alabama at Birmingham, 35233-6810, USA.
Anesthesiology. 2004 Jan;100(1):51-8. doi: 10.1097/00000542-200401000-00012.
Human serum albumin is used clinically to maintain colloid osmotic pressure and is viewed to serve an antioxidant role in the vascular compartment via binding of redox-active metal complexes, transport of nitric oxide, and the oxidant-scavenging reactions of the single thiol of human serum albumin, cys34. Because of these potentially desirable adjunctive actions, we evaluated the purity and thiol redox state and compared the relative effects of clinically available 25% human serum albumin preparations with a starch-derived colloid, 6% hydroxyethyl starch, in in vitro models of inflammatory vascular injury.
Bovine aortic endothelial cell responses to chemical, enzymatic, and cell-derived reactive inflammatory mediators in the presence of human serum albumin or hydroxyethyl starch were assessed.
The cys34 thiol of fresh human serum albumin preparations was 70-85% oxidized and contained a population of human serum albumin (approximately 25% of total) having the cys34 resistant to reduction by 2-mercaptoethanol and NaBH4. Treatment of bovine aortic endothelial cells with human serum albumin dose-dependently protected from HOCl-mediated 14C-adenine release, with this protective effect of human serum albumin not dependent on protein thiol status. Addition of human serum albumin to cell media provided no protection from the cytotoxic actions of peroxynitrite and xanthine oxidase-derived reactive species. Binding of activated polymorphonuclear leukocytes to bovine aortic endothelial cells was significantly amplified by hydroxyethyl starch and inhibited by human serum albumin administration. The binding of neutrophil-derived myeloperoxidase to bovine aortic endothelial cells, a mediator of multiple oxidative and nitric oxide-consuming reactions, was also inhibited by human serum albumin and enhanced by hydroxyethyl starch.
Clinical human serum albumin preparations show modest intrinsic non-thiol-dependent antiinflammatory properties in vitro, a phenomenon that was not observed with hydroxyethyl starch.
人血清白蛋白在临床上用于维持胶体渗透压,并且被认为通过结合氧化还原活性金属络合物、运输一氧化氮以及人血清白蛋白的单个巯基(半胱氨酸34)的抗氧化清除反应,在血管腔中发挥抗氧化作用。由于这些潜在的有益辅助作用,我们评估了其纯度和巯基氧化还原状态,并在炎症性血管损伤的体外模型中比较了临床上可用的25%人血清白蛋白制剂与淀粉衍生胶体6%羟乙基淀粉的相对作用。
评估在人血清白蛋白或羟乙基淀粉存在的情况下,牛主动脉内皮细胞对化学、酶促和细胞衍生的反应性炎症介质的反应。
新鲜人血清白蛋白制剂的半胱氨酸34巯基有70 - 85%被氧化,并且含有一群半胱氨酸34对2 - 巯基乙醇和硼氢化钠还原具有抗性的人血清白蛋白(约占总量的25%)。用人血清白蛋白处理牛主动脉内皮细胞可剂量依赖性地保护细胞免受次氯酸介导的14C - 腺嘌呤释放,人血清白蛋白的这种保护作用不依赖于蛋白质巯基状态。向细胞培养基中添加人血清白蛋白不能保护细胞免受过氧亚硝酸盐和黄嘌呤氧化酶衍生的反应性物质的细胞毒性作用。羟乙基淀粉显著增强了活化的多形核白细胞与牛主动脉内皮细胞的结合,而人血清白蛋白给药则抑制了这种结合。中性粒细胞衍生的髓过氧化物酶与牛主动脉内皮细胞的结合(多种氧化和消耗一氧化氮反应的介质)也受到人血清白蛋白的抑制,并被羟乙基淀粉增强。
临床人血清白蛋白制剂在体外显示出适度的内在非巯基依赖性抗炎特性,羟乙基淀粉未观察到这种现象。
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