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野生醋栗番茄对急性紫外线-C照射的响应:损伤的组织细胞化学及DNA损伤

Responsiveness of Lycopersicon pimpinellifolium to acute UV-C exposure: histo-cytochemistry of the injury and DNA damage.

作者信息

Iriti M, Guarnieri S, Faoro F

机构信息

Istituto di Patologia Vegetale, Università di Milano, Italy.

出版信息

Acta Biochim Pol. 2007;54(2):273-80. Epub 2007 May 23.

Abstract

The in vivo and in vitro effects of UV-C (254 nm) exposure (0.039 watt . m(-2) . s for 2 h) of currant tomato (Lycopersicon pimpinellifolium), indigenous to Peru and Ecuador, were assayed. H(2)O(2) deposits, dead cells and DNA damage were localized, 12/24 h after irradiation, mainly in periveinal parenchyma of the 1st and 2nd order veins of the leaves, and before the appearance of visible symptoms, which occurred 48 h after irradiation. Cell death index was of 43.5 +/- 12% in exposed leaf tissues, 24 h after treatment. In currant tomato protoplasts, the percentage of viable cells dropped 1 h after UV-C irradiation from 97.42 +/- 2.1% to 43.38 +/- 4.2%. Afterwards, the protoplast viability progressively decreased to 40.16 +/- 7.25% at 2 h, to 38.31 +/- 6.9% at 4 h, and to 36.46 +/- 1.84% at 6 h after the exposure. The genotoxic impact of UV-C radiation on protoplasts was assessed with single cell gel electrophoresis (SCGE, or comet assay). UV-C treatment greatly enhanced DNA migration, with 75.37 +/- 3.7% of DNA in the tail versus 7.88 +/- 5.5% in the case of untreated nuclei. Oxidative stress by H(2)O(2) used as a positive control, induced a similar damage on non-irradiated protoplasts, with 71.59 +/- 5.5% of DNA in the tail, whereas oxidative stress imposed on UV-C irradiated protoplasts slightly increased the DNA damage (85.13 +/- 4.1%). According to these results, SCGE of protoplasts could be an alternative to nuclei extraction directly from leaf tissues.

摘要

对原产于秘鲁和厄瓜多尔的醋栗番茄(Lycopersicon pimpinellifolium)进行了紫外线C(254纳米)照射(0.039瓦特·米-2·秒,持续2小时)的体内和体外效应分析。在照射后12/24小时,H2O2沉积物、死亡细胞和DNA损伤主要定位在叶片一级和二级叶脉的脉周薄壁组织中,且在照射48小时后出现可见症状之前。处理后24小时,暴露叶片组织的细胞死亡指数为43.5±12%。在醋栗番茄原生质体中,紫外线C照射1小时后,活细胞百分比从97.42±2.1%降至43.38±4.2%。此后,原生质体活力在照射后2小时逐渐降至40.16±7.25%,4小时降至38.31±6.9%,6小时降至36.46±1.84%。用单细胞凝胶电泳(SCGE,即彗星试验)评估紫外线C辐射对原生质体的遗传毒性影响。紫外线C处理极大地增强了DNA迁移,尾部DNA占75.37±3.7%,而未处理细胞核的这一比例为7.88±5.5%。用作阳性对照的H2O2诱导的氧化应激对未照射的原生质体造成了类似损伤,尾部DNA占71.59±5.5%,而对紫外线C照射的原生质体施加氧化应激则使DNA损伤略有增加(85.13±4.1%)。根据这些结果,原生质体的SCGE可以替代直接从叶片组织中提取细胞核。

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