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二血卟啉醚对人NHIK 3025细胞中细胞分裂的光动力效应。

Photodynamic effects of Photofrin II on cell division in human NHIK 3025 cells.

作者信息

Berg K, Moan J

机构信息

Norwegian Radium Hospital, Department of Biophysics, Montebello, Oslo.

出版信息

Int J Radiat Biol Relat Stud Phys Chem Med. 1988 May;53(5):797-811. doi: 10.1080/09553008814551141.

Abstract

Human cervix carcinoma cells of the line NHIK 3025 were exposed to light after 18 h incubation with Photofrin II. After this photodynamic treatment cells in the interphase were retarded with respect to entry into mitosis for a period which increased with increasing light dose. Following the prolonged interphase, an increase in the mitotic index was observed, giving rise to a 3-fold higher level of mitotic cells compared to the control level. Staining of methanol-fixed cells with the DNA-specific dye mithramycin indicated that the increase in mitotic index was due to a prolongation of the metaphase. For all the light doses studied most of the metaphase cells could be characterized as three-group metaphases or c-metaphase-like structures for the first 8 h after treatment. An approximately 10-fold increase above the control level in the number of tripolar mitoses was also observed. A 2h incubation in a Photofrin II-free medium after the 18 h incubation with Photofrin II and before light exposure reduced the fluorescence of the cells by 30 per cent. However, this wash-out period had no effect on the increase in mitotic index after light exposure. A light dose corresponding to 80 per cent survival (as assayed on asynchronous cells) was given to cells in mitosis after Photofrin II incubation. This treatment delayed more than 90 per cent of the metaphase cells from entering the anaphase for at least 1 h. Cells photodynamically treated in the anaphase and telophase entered the interphase at a similar rate as control cells. These observations indicate a temporary block in the initiation of the anaphase and a prolongation of the metaphase. A microscopic study of cells immunologically stained for beta-tubulin 1 h after photodynamic treatment indicated that the organization of the spindle apparatus was disturbed by the photodynamic treatment. Such perturbations are suggested to be the cause of the observed accumulation of cells in mitosis.

摘要

将人源宫颈癌细胞系NHIK 3025与二血卟啉醚(Photofrin II)孵育18小时后进行光照。这种光动力处理后,处于间期的细胞进入有丝分裂受到延迟,延迟时间随光照剂量增加而延长。在延长的间期之后,观察到有丝分裂指数增加,与对照水平相比,有丝分裂细胞水平高出3倍。用DNA特异性染料光辉霉素对甲醇固定的细胞进行染色表明,有丝分裂指数的增加是由于中期延长所致。对于所研究的所有光照剂量,在处理后的前8小时,大多数中期细胞可被表征为三组中期或类c-中期结构。还观察到三极有丝分裂的数量比对照水平增加了约10倍。在与二血卟啉醚孵育18小时后且光照前,在无二血卟啉醚的培养基中孵育2小时,可使细胞荧光降低30%。然而,这段洗脱期对光照后有丝分裂指数的增加没有影响。在二血卟啉醚孵育后,对处于有丝分裂期的细胞给予相当于80%存活率(在非同步细胞上测定)的光照剂量。这种处理使超过90%的中期细胞延迟至少1小时进入后期。在后期和末期进行光动力处理的细胞进入间期的速率与对照细胞相似。这些观察结果表明后期启动存在暂时阻滞,中期延长。光动力处理1小时后对细胞进行β-微管蛋白免疫染色的显微镜研究表明,光动力处理扰乱了纺锤体装置的组织。这种扰动被认为是观察到的有丝分裂期细胞积累的原因。

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