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Characterization of human lens major intrinsic protein structure.

机译:人类晶状体主要内在蛋白质结构的表征。

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摘要

PURPOSE: To determine the primary covalent structure of human lens major intrinsic protein (MIP) in lenses of varying age. METHODS: MIP was isolated from single human lenses of various ages (7- 86 years) by homogenization of the lenses, followed by centrifugation and urea washes of the membranes. Proteins present in the membrane preparation were reduced, alkylated, and cleaved by CNBr. Peptide fragments were fractionated by reverse-phase high-performance liquid chromatography, and the primary structures of the peptides were determined by tandem mass spectrometry and Edman sequencing. RESULTS: Complete coverage of the human MIP sequence was observed in the form of CNBr fragments. In addition, peptide structures resulting from in vivo heterogeneous N- and C-terminal cleavage were characterized. The amount of intact MIP decreased with lens age; however, the pattern of truncation did not change from 7 to 86 years. The major site of phosphorylation was identified as serine 235. Asparagine residues 246 and 259 were completely deamidated by age 7 years. CONCLUSIONS: The major structural modifications of human lens MIP have been determined. Human MIP is heterogeneously modified in lenses ranging in age from 7 to 86 years of age by N- and C-terminal truncation, phosphorylation, and deamidation, resulting in decreased levels of native intact MIP with age.
机译:目的:确定不同年龄的晶状体中人晶状体主要内在蛋白(MIP)的主要共价结构。方法:通过均质化镜片,然后离心和洗膜尿素,从各个年龄(7-86岁)的单个人类晶状体中分离出MIP。膜制品中存在的蛋白质被CNBr还原,烷基化和裂解。通过反相高效液相色谱法分离肽片段,并通过串联质谱和埃德曼测序确定肽的一级结构。结果:以CNBr片段的形式观察到了人类MIP序列的完全覆盖。另外,表征了由体内异质N-和C-末端裂解产生的肽结构。随着晶状体年龄的增长,完整的MIP数量减少;但是,截断的模式没有从7年更改为86年。磷酸化的主要位点被鉴定为丝氨酸235。到7岁时天冬酰胺残基246和259被完全脱酰胺。结论:已经确定了人类晶状体MIP的主要结构修饰。人类MIP通过N和C末端的截短,磷酸化和脱酰胺作用,在7至86岁年龄段的晶状体中进行了异质修饰,从而导致天然完整MIP的水平随着年龄的增长而降低。

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