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[猪虹膜脂质过氧化与色素沉着的关系]

[Dependence of lipid peroxidation on pigmentation of the porcine iris].

作者信息

Nau-Staudt K, Nau W M, Haefliger I O, Flammer J

机构信息

Universitäts-Augenklinik, Labor für okuläre Pharmakologie und Physiologie, Mittlere Strasse 91, CH-4056 Basel.

出版信息

Klin Monbl Augenheilkd. 2001 May;218(5):341-4. doi: 10.1055/s-2001-15895.

Abstract

PURPOSE

Melanin has been shown to act as antioxidant in lipid peroxidation studies. We have now investigated lipid peroxidation in dependence on stromal pigmentation in isolated porcine irises.

METHODS

The same number of lightly pigmented and heavily pigmented porcine irises (visual selection) were homogenized in buffer (50 mmol/l Na2HPO4, 50 mmol/l NaH2PO4 and 4 mmol/l sodium azide; 1:20 w/v). 500 microliters homogenate were incubated at 37 degrees C for 5, 10, 20 and 40 min in absence and presence of Fe2+ as inducer of lipid peroxidation. Lipid peroxidation was assayed by the thiobarbituric acid (TBA) test. Results are expressed as nmol of TBA reactive material produced (TBAR) per mg protein. Fe2+ concentration of the supernatant was determined spectrophotometrically with phenanthroline.

RESULTS

70 mumol/l, 180 mumol/l and 360 mumol/l Fe2+ induced lipid peroxidation. A plateau region was reached after 20 min. Lipid peroxidation differed in dependence on stromal pigmentation in porcine irises by a factor of 2.8. 180 mumol/l Fe2+ induced 1.373 +/- 0.138 nmol TBAR/mg protein in lightly pigmented irises compared to 0.491 +/- 0.125 nmol TBAR/mg protein in heavily pigmented irises after 10 min incubation (p < 0.0001, n = 4). On the other hand, the content of Fe2+ in the supernatant was the same within error.

CONCLUSIONS

There was a stronger induction of lipid peroxidation in lightly pigmented porcine irises compared to heavily pigmented porcine irises. This effect may be related to the difference in stromal melanin content and its antioxidant activity.

摘要

目的

在脂质过氧化研究中,黑色素已被证明具有抗氧化作用。我们现在研究了分离的猪虹膜中脂质过氧化与基质色素沉着的关系。

方法

将相同数量的轻度色素沉着和重度色素沉着的猪虹膜(目视选择)在缓冲液(50 mmol/L磷酸氢二钠、50 mmol/L磷酸二氢钠和4 mmol/L叠氮化钠;1:20 w/v)中匀浆。500微升匀浆在37℃下,在不存在和存在作为脂质过氧化诱导剂的Fe2+的情况下分别孵育5、10、20和40分钟。通过硫代巴比妥酸(TBA)试验测定脂质过氧化。结果以每毫克蛋白质产生的TBA反应性物质(TBAR)的纳摩尔数表示。用邻菲罗啉分光光度法测定上清液中Fe2+的浓度。

结果

70 μmol/L、180 μmol/L和360 μmol/L的Fe2+诱导脂质过氧化。20分钟后达到平稳期。猪虹膜中脂质过氧化因基质色素沉着不同而相差2.8倍。孵育10分钟后,180 μmol/L的Fe2+在轻度色素沉着的虹膜中诱导产生1.373±0.138 nmol TBAR/mg蛋白质,而在重度色素沉着的虹膜中为0.491±0.125 nmol TBAR/mg蛋白质(p<0.0001,n = 4)。另一方面,上清液中Fe2+的含量在误差范围内相同。

结论

与重度色素沉着的猪虹膜相比,轻度色素沉着的猪虹膜中脂质过氧化的诱导作用更强。这种效应可能与基质黑色素含量及其抗氧化活性的差异有关。

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