Turesson Ingela, Simonsson Martin, Hermansson Ingegerd, Book Majlis, Sigurdadottir Sunna, Thunberg Ulf, Qvarnström Fredrik, Johansson Karl-Axel, Fessé Per, Nyman Jan
Department of Immunology, Genetics and Pathology, Experimental and Clinical Oncology, Uppsala University, Uppsala, Sweden.
Department of Oncology.
Radiat Res. 2020 May;193(5):481-496. doi: 10.1667/RR15417.1. Epub 2020 Mar 20.
During fractionated radiotherapy, epithelial cell populations are thought to decrease initially, followed by accelerated repopulation to compensate cell loss. However, previous findings in skin with daily 1.1 Gy dose fractions indicate continued and increasing cell depletion. Here we investigated epidermal keratinocyte response with daily 2 Gy fractions as well as accelerated and hypofractionation. Epidermal interfollicular melanocytes were also assessed. Skin-punch biopsies were collected from breast cancer patients before, during and after mastectomy radiotherapy to the thoracic wall with daily 2 Gy fractions for 5 weeks. In addition, 2.4 Gy radiotherapy four times per week and 4 Gy fractions twice per week for 5 weeks, and two times 2 Gy daily for 2.5 weeks, were used. Basal keratinocyte density of the interfollicular epidermis was determined and immunostainings of keratinocytes for DNA double-strand break (DSB) foci, growth arrest, apoptosis and mitosis were quantified. In addition, interfollicular melanocytes were counted. Initially minimal keratinocyte loss was observed followed by pronounced depletion during the second half of treatment and full recovery at 2 weeks post treatment. DSB foci per cell peaked towards the end of treatment. p21-stained cell counts increased during radiotherapy, especially the second half. Apoptotic frequency was low throughout radiotherapy but increased at treatment end. Mitotic cell count was significantly suppressed throughout radiotherapy and did not recover during weekend treatment gaps, but increased more than threefold compared to unexposed skin 2 weeks post-radiotherapy. The number of melanocytes remained constant over the study period. Germinal keratinocyte loss rate increased gradually during daily 2 Gy fractions for 5 weeks, and similarly for hypofractionation. DSB foci number after 2 Gy irradiation revealed an initial radioresistance followed by increasing radiosensitivity. Growth arrest mediated by p21 strongly suggests that cells within or recruited into the cell cycle during treatment are at high risk of loss and do not contribute significantly to repopulation. It is possible that quiescent (G) cells at treatment completion accounted for the accelerated post-treatment repopulation. Recent knowledge of epidermal tissue regeneration and cell cycle progression during genotoxic and mitogen stress allows for a credible explanation of the current finding. Melanocytes were radioresistant regarding cell depletion.
在分割放疗期间,上皮细胞群体起初被认为会减少,随后会加速再增殖以补偿细胞损失。然而,先前在每日剂量分割为1.1 Gy的皮肤研究结果显示细胞持续且不断增加地耗竭。在此,我们研究了每日剂量分割为2 Gy以及加速分割和大分割放疗时表皮角质形成细胞的反应。还评估了表皮非毛囊性黑素细胞。在乳腺癌患者胸壁进行乳房切除术后放疗期间及前后,采集皮肤打孔活检样本,放疗采用每日2 Gy剂量分割,持续5周。此外,还采用了每周4次2.4 Gy放疗、每周2次4 Gy剂量分割,持续5周,以及每日2次2 Gy,持续2.5周的方案。测定非毛囊性表皮基底角质形成细胞密度,并对角质形成细胞进行免疫染色,以量化DNA双链断裂(DSB)灶、生长停滞、凋亡和有丝分裂情况。此外,对非毛囊性黑素细胞进行计数。起初观察到角质形成细胞损失最小,随后在治疗后半期出现明显耗竭,治疗后2周完全恢复。每个细胞的DSB灶在治疗末期达到峰值。放疗期间p21染色细胞计数增加,尤其是在后半期。整个放疗期间凋亡频率较低,但在治疗结束时增加。有丝分裂细胞计数在整个放疗期间显著受到抑制,在周末治疗间隙未恢复,但在放疗后2周与未照射皮肤相比增加了三倍多。在研究期间黑素细胞数量保持恒定。在每日2 Gy剂量分割持续5周以及大分割放疗时,生发层角质形成细胞损失率逐渐增加。2 Gy照射后的DSB灶数量显示出最初的放射抗性,随后放射敏感性增加。由p21介导的生长停滞强烈表明,在治疗期间进入或被招募进入细胞周期的细胞有很高的损失风险,并且对再增殖没有显著贡献。有可能治疗结束时的静止(G)细胞促成了治疗后的加速再增殖。目前关于表皮组织再生以及遗传毒性和有丝分裂原应激期间细胞周期进展的知识为当前发现提供了可信的解释。黑素细胞在细胞耗竭方面具有放射抗性。
