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剑尾鱼皮肤中紫外线辐射诱导的DNA损伤及其光修复

Ultraviolet radiation-induced DNA damage and its photorepair in the skin of the platyfish Xiphophorus.

作者信息

Ahmed F E, Setlow R B

机构信息

Biology Department, Brookhaven National Laboratory, Upton, New York 11973.

出版信息

Cancer Res. 1993 May 15;53(10 Suppl):2249-55.

PMID:8485710
Abstract

Fluence response relationships for the induction of DNA damage in the skin of UV-irradiated Xiphophorus fish were obtained by quantitative gel electrophoresis of unlabeled DNA following extraction and treatment with an enzyme preparation that makes single strand breaks next to cyclobutane pyrimidine dimers. A buffer containing 7 M urea minimized the degradation of DNA during extraction and gave reproducible results. The shapes of fluence response curves for the production of dimers by sun lamp irradiation (lambda > 290 nm) or 302 nm in the dermis of grown fish were similar. Photoreversal of dimers was readily observed by black light exposure or from the longer wavelengths (> 304 nm) from sun lamps. As expected, the number of pyrimidine dimers/incident fluence in young fish skin was considerably higher on the irradiated side of immobilized fish than it was in swimming (randomly moving) fish, and the shape of the fluence response curves was linear for all wavelengths used lambda > 290, 302, and 313 nm. On the other hand, young fish irradiated from above with lambda > 290 nm showed a less than linear relationship between pyrimidine dimers in their skin and radiation fluence because most exposure occurred on the dorsal rim of fish skin; thus, some cells in that skin were exposed to high fluences while others were not, leading to a heterogenous population of cells. Values of dimers produced were also much less than in immobilized fish. The pigment melanin decreased the number of dimers in the epidermis of grown fish exposed to lambda > 290, 302, or 313 nm, or in the dermis of fish following 302 nm, thus conferring protection against this kind of damage. No dimers were detected in the epidermis of fish exposed to 365 nm. The dimers produced at 302 and 313 nm at tumoricidal exposures correspond to 1 dimer in 10(5) base pairs.

摘要

通过对未标记DNA进行定量凝胶电泳来获得紫外线照射的剑尾鱼皮肤中DNA损伤诱导的通量响应关系。提取DNA后,用一种能在环丁烷嘧啶二聚体旁产生单链断裂的酶制剂进行处理。含有7M尿素的缓冲液可最大程度减少提取过程中DNA的降解,并给出可重复的结果。成年鱼真皮经太阳灯照射(波长>290nm)或302nm照射产生二聚体的通量响应曲线形状相似。通过黑光照射或太阳灯较长波长(>304nm)很容易观察到二聚体的光逆转。正如预期的那样,固定鱼受照射一侧幼鱼皮肤中嘧啶二聚体的数量/入射通量比游动(随机移动)鱼的要高得多,并且对于所有使用的波长(波长>290、302和313nm),通量响应曲线的形状都是线性的。另一方面,用波长>290nm从上方照射的幼鱼,其皮肤中嘧啶二聚体与辐射通量之间的关系小于线性关系,因为大多数照射发生在鱼皮肤的背缘;因此,该皮肤中的一些细胞暴露于高通量,而其他细胞则未暴露,导致细胞群体不均一。产生的二聚体值也比固定鱼中的少得多。色素黑色素减少了成年鱼暴露于波长>290、302或313nm时表皮中二聚体的数量,或减少了302nm照射后鱼真皮中二聚体的数量,从而提供了针对这种损伤的保护。在暴露于365nm的鱼表皮中未检测到二聚体。在杀肿瘤剂量下于302和313nm产生的二聚体相当于每10(5)个碱基对中有1个二聚体。

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