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来自年轻人类晶状体的色氨酸代谢产物以及UVA光对维生素C的光氧化作用。

Tryptophan metabolites from young human lenses and the photooxidation of ascorbic acid by UVA light.

作者信息

Ortwerth Beryl J, Bhattacharyya Jaya, Shipova Ekaterina

机构信息

Mason Eye Institute, University of Missouri, Columbia, Missouri 65201, USA.

出版信息

Invest Ophthalmol Vis Sci. 2009 Jul;50(7):3311-9. doi: 10.1167/iovs.08-2927. Epub 2009 Mar 5.

Abstract

PURPOSE

To determine whether there are UVA light-responsive sensitizers in young human lenses capable of initiating the oxidation of ascorbic acid in the absence of oxygen.

METHODS

Lens homogenates were fractionated, and low-molecular-weight (LMW) components were separated from the proteins by filtration through a 3000-MWt cutoff filter. Aliquots of each fraction were assayed for sensitizer activity by UVA irradiation (337-nm cutoff filter) with 0.1 mM ascorbic acid, measuring ascorbate oxidation by loss of absorbance at 265 nm. Two major peaks were isolated from a human lens water-soluble (WS)-LMW fraction on a reversed-phase column and were identified by mass spectrometry.

RESULTS

All human lens fractions oxidized ascorbate when irradiated by UVA light. Most of the sensitizer activity in young human lenses was in the LMW fractions. An action spectrum for the WS-LMW fraction from human lens showed activity throughout the UVA region. Assays with and without oxygen showed little or no difference in ascorbate oxidized, arguing for a direct transfer of an electron in a so-called type 1 reaction. A human lens WS-LMW fraction contained two major peaks of activity. The greater peak was identified as 3-hydroxykynurenine glucoside (3OHKG) by mass spectrometry and its absorption spectrum, whereas the lesser peak was identified as 4-(2-amino-3-hydroxyphenyl)-4-oxobutanoic acid glucoside (AHBG). The activities were 1.1 and 2.8 nmol of ascorbate oxidized in 30 minutes/nmol 3OHKG and AHBG, respectively.

CONCLUSIONS

The filter compounds present in human lenses can absorb UVA light and cause the oxidation of ascorbic acid in the presence and absence of oxygen, possibly initiating the glycation of lens proteins.

摘要

目的

确定在年轻人类晶状体中是否存在能够在无氧条件下引发抗坏血酸氧化的UVA光反应性敏化剂。

方法

对晶状体匀浆进行分级分离,通过截留分子量为3000的滤膜过滤,将低分子量(LMW)成分与蛋白质分离。对每个级分的等分试样进行UVA照射(337nm截止滤光片),加入0.1mM抗坏血酸,通过测量265nm处吸光度的损失来测定抗坏血酸氧化,以此检测敏化剂活性。在反相柱上从人晶状体水溶性(WS)-LMW级分中分离出两个主要峰,并通过质谱进行鉴定。

结果

当受到UVA光照射时,所有人晶状体级分均能氧化抗坏血酸。年轻人类晶状体中的大多数敏化剂活性存在于LMW级分中。人晶状体WS-LMW级分的作用光谱显示在整个UVA区域均有活性。有氧和无氧条件下的测定结果表明,氧化的抗坏血酸几乎没有差异,这表明在所谓的1型反应中电子直接转移。人晶状体WS-LMW级分包含两个主要活性峰。通过质谱及其吸收光谱鉴定,较大的峰为3-羟基犬尿氨酸葡萄糖苷(3OHKG),较小的峰为4-(2-氨基-3-羟苯基)-4-氧代丁酸葡萄糖苷(AHBG)。活性分别为30分钟内氧化1.1和2.8nmol抗坏血酸/ nmol 3OHKG和AHBG。

结论

人类晶状体中存在的滤光化合物可吸收UVA光,并在有氧和无氧条件下导致抗坏血酸氧化,可能引发晶状体蛋白的糖基化。

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