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Ki-67、拓扑异构酶IIα、增殖细胞核抗原、p53和p21WAF1/Cip1的表达增强,反映了紫外线照射的黑素细胞痣中的增殖和修复活性。

Enhanced expression of Ki-67, topoisomerase IIalpha, PCNA, p53 and p21WAF1/Cip1 reflecting proliferation and repair activity in UV-irradiated melanocytic nevi.

作者信息

Rudolph P, Tronnier M, Menzel R, Möller M, Parwaresch R

机构信息

Department of Pathology and the Lymph Node Registry, German Society of Pathology, at the University of Kiel.

出版信息

Hum Pathol. 1998 Dec;29(12):1480-7. doi: 10.1016/s0046-8177(98)90019-3.

DOI:10.1016/s0046-8177(98)90019-3
PMID:9865836
Abstract

To investigate the effect of ultraviolet (UV) irradiation on the expression of cell cycle-associated proteins, melanocytic nevi from healthy volunteers were partially covered, irradiated with a defined UV dose, and excised 1 week thereafter. The irradiated and the protected parts were examined separately by conventional microscopy and immunohistochemistry using the antibodies Ki-S11 (Ki-67), Ki-S7 (topoisomerase IIalpha), PC10 (proliferating cell nuclear antigen [PCNA]), DO-7 (p53), 6B6 (p21WAF1/Cip1), and the melanocytic marker HMB-45. DNA nick-end labeling was used as a marker of apoptosis. Irradiation resulted in morphological changes and increased HMB-45 reactivity. Proliferation, as assessed by Ki-67 and topoisomerase IIalpha expression, was also clearly enhanced in the UV-exposed areas. This was confirmed by the appearance of occasional mitotic figures. PCNA expression levels markedly exceeded those of the proliferation markers and did not correlate with the latter in most cases. p21 immunolabeling indices were also consistently augmented after UV exposure; hence it is likely that growth-inhibitory mechanisms partly compensate for the proliferative impulse, and the disproportional rise in PCNA expression probably reflects DNA repair activity. Enhanced p53 immunostaining in four cases suggests that the induction of p21 after irradiation may be p53 mediated, whereas no concomitant apoptotic events were observed. We conclude that UV light can stimulate the proliferative activity of melanocytes in melanocytic nevi, but that simultaneously cell cycle inhibitors are activated to permit DNA repair.

摘要

为研究紫外线(UV)照射对细胞周期相关蛋白表达的影响,对来自健康志愿者的黑素细胞痣进行部分遮盖,给予特定紫外线剂量照射,1周后切除。使用抗体Ki-S11(Ki-67)、Ki-S7(拓扑异构酶IIα)、PC10(增殖细胞核抗原[PCNA])、DO-7(p53)、6B6(p21WAF1/Cip1)以及黑素细胞标志物HMB-45,通过传统显微镜检查和免疫组织化学分别检测照射部位和受保护部位。DNA缺口末端标记用作细胞凋亡的标志物。照射导致形态学改变并增加HMB-45反应性。通过Ki-67和拓扑异构酶IIα表达评估的增殖在紫外线暴露区域也明显增强。偶尔出现的有丝分裂象证实了这一点。PCNA表达水平明显超过增殖标志物,且在大多数情况下与后者不相关。紫外线暴露后p21免疫标记指数也持续增加;因此,生长抑制机制可能部分补偿了增殖冲动,PCNA表达的不成比例升高可能反映了DNA修复活性。4例中p53免疫染色增强表明照射后p21的诱导可能是p53介导的,而未观察到伴随的细胞凋亡事件。我们得出结论,紫外线可刺激黑素细胞痣中黑素细胞的增殖活性,但同时细胞周期抑制剂被激活以允许DNA修复。

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