Coppes R P, Roffel A F, Zeilstra L J, Vissink A, Konings A W
Department of Radiobiology University of Groningen, Groningen, The Netherlands.
Radiat Res. 2000 Mar;153(3):339-46. doi: 10.1667/0033-7587(2000)153[0339:ereomr]2.0.co;2.
Although the salivary glands have a low rate of cell turnover, they are relatively radiosensitive. To study the possible mechanism behind this inherent radiosensitivity, a rat model was developed in which saliva can be collected after local irradiation of the parotid gland without the use of anesthetics or stressful handling. Saliva secretion was induced by the partial muscarinic receptor agonist pilocarpine (0.03-3 mg/kg) with or without pretreatment with the beta-adrenoceptor antagonist propranolol (2.5 mg/kg), or the full muscarinic receptor agonist methacholine (0.16-16 mg/min), and measured during 5 min per drug dose before and 1, 3, 6 and 10 days after irradiation. The maximal secretory response induced by pilocarpine plus propranolol was increased compared to that with pilocarpine alone but did not reach the level of methacholine-induced secretion, which was about five times higher. One day after irradiation a decrease in maximal pilocarpine-induced secretion was observed (-22%) using the same dose of pilocarpine that induces 50% of the maximal response (ED(50)), in both the absence and presence of propranolol, indicating that the receptor-drug interaction was not affected by the radiation at this time. The secretory response to methacholine 1 day after irradiation, however, was normal. At day 3 after irradiation, the maximal methacholine-induced secretion was also affected, whereas pilocarpine (+/-propranolol)-induced maximal secretion decreased further. At day 6 after irradiation, maximal secretory responses had declined to approximately 50% regardless of the agonist used, whereas ED(50) values were still unaffected. No net acinar cell loss was observed within the first 10 days after irradiation, and this therefore could not account for the loss in function. The results indicate that radiation does not affect cell number or receptor-drug interaction, but rather signal transduction, which eventually leads to the impaired response. We hypothesize that the early radiation effect, within 3 days, may be membrane damage affecting the receptor-G-protein signaltransfer. Later critical damage, however, is probably of a different nature and may be located in the second-messenger signal transduction pathway downstream from the G protein, not necessarily involving cellular membranes.
尽管唾液腺的细胞更新率较低,但它们对辐射相对敏感。为了研究这种固有辐射敏感性背后的可能机制,建立了一种大鼠模型,在该模型中,在不使用麻醉剂或进行应激处理的情况下,对腮腺进行局部照射后可以收集唾液。通过部分毒蕈碱受体激动剂毛果芸香碱(0.03 - 3mg/kg)诱导唾液分泌,同时使用或不使用β-肾上腺素能受体拮抗剂普萘洛尔(2.5mg/kg)进行预处理,或者使用完全毒蕈碱受体激动剂乙酰甲胆碱(0.16 - 16mg/min)进行诱导,并在给药前以及照射后1、3、6和10天期间,每剂药物持续5分钟测量唾液分泌量。与单独使用毛果芸香碱相比,毛果芸香碱加普萘洛尔诱导的最大分泌反应有所增加,但未达到乙酰甲胆碱诱导分泌水平的约五倍。照射后一天,在使用诱导50%最大反应(ED(50))的相同剂量毛果芸香碱时,无论是否存在普萘洛尔,最大毛果芸香碱诱导的分泌均出现下降(-22%),这表明此时受体-药物相互作用未受辐射影响。然而,照射后一天对乙酰甲胆碱的分泌反应正常。照射后第3天,最大乙酰甲胆碱诱导的分泌也受到影响,而毛果芸香碱(±普萘洛尔)诱导的最大分泌进一步下降。照射后第6天,无论使用何种激动剂,最大分泌反应均下降至约50%,而ED(50)值仍未受影响。照射后前10天未观察到腺泡细胞净损失,因此这不能解释功能丧失的原因。结果表明,辐射不影响细胞数量或受体-药物相互作用,而是影响信号转导,最终导致反应受损。我们推测,3天内的早期辐射效应可能是膜损伤影响受体-G蛋白信号转导。然而,后期的关键损伤可能性质不同,可能位于G蛋白下游的第二信使信号转导途径中,不一定涉及细胞膜。
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