Abedinia M, Pain T, Algar E M, Holmes R S
Division of Science and Technology, Griffith University, Nathan, Brisbane, Australia.
Exp Eye Res. 1990 Oct;51(4):419-26. doi: 10.1016/0014-4835(90)90154-m.
Bovine corneal aldehyde dehydrogenase was purified to homogeneity and characterized with aldehyde substrates at pH 7.4. The enzyme was a dimer with a subunit size of 65 kDa. Using kcat/Km values as an indication of substrate efficacy, aldehyde products of lipid peroxidation were recognized as the likely 'natural' substrates. Protein yields from enzyme purification, as well as electrophoretic analyses of crude and purified enzyme preparations, demonstrated that this enzyme is the major soluble protein in bovine cornea, and constitutes around 0.5% wet weight of tissue. A dual role in protecting the eye against UV-B light is proposed--oxidation of aldehydes generated by light induced lipid peroxidation, and the direct absorption of UV-B light by bovine corneal ALDH.
牛角膜醛脱氢酶被纯化至同质,并在pH 7.4条件下用醛底物进行了特性鉴定。该酶为二聚体,亚基大小为65 kDa。以kcat/Km值作为底物效能的指标,脂质过氧化的醛产物被认为是可能的“天然”底物。酶纯化后的蛋白质产量以及粗酶和纯化酶制剂的电泳分析表明,这种酶是牛角膜中的主要可溶性蛋白质,约占组织湿重的0.5%。有人提出它在保护眼睛免受UV-B光伤害方面具有双重作用——氧化光诱导脂质过氧化产生的醛,以及牛角膜醛脱氢酶直接吸收UV-B光。
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