国家毒理学控制项目关于转基因(FVB Tg)中阿斯巴甜毒理学研究的报告(CAS No. 22839-47-0)。AC半合子和B6.129-Cdkn2atm1Rdp (N2)缺乏小鼠以及阿斯巴甜在转基因[B6.129-Trp53tm1Brd (N5)单倍不足]小鼠中的致癌性研究(饲料研究)。

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引用次数: 0

摘要

未标明:阿斯巴甜是一种人造甜味剂,在世界各地的食品和饮料中都有使用。传统的2年啮齿类动物阿斯巴甜癌症研究被认为是阴性的,尽管在一项大鼠研究中观察到少量脑肿瘤(联邦登记册)。, 1981 a, b)。国家毒理学计划探索了使用转基因小鼠模型作为2年啮齿动物癌症试验的辅助手段。这些模型可能被证明更快速,使用更少的动物,并提供一些关于肿瘤反应的机制见解。作为评估新的小鼠癌症筛选模型的一部分,阿斯巴甜在两种研究相对较充分的模型中进行了潜在毒性和致癌性测试。AC半合子菌株和p53单倍缺陷菌株,以及一个未表征的模型,Cdkn2a缺陷菌株。男、女Tg。AC半合子、p53单倍体不足和Cdkn2a缺陷小鼠给予含有阿斯巴甜(纯度大于98%)的饲料9个月。对鼠伤寒沙门菌、大鼠骨髓细胞和小鼠外周血红细胞进行了遗传毒理学研究。9个月的Tg研究。AC半合子小鼠:雄性15只,雌性15只。给AC半合子小鼠喂食含有0、3,125、6,250、12,500、25,000或50,000 ppm阿斯巴甜的饲料(相当于雄性阿斯巴甜的平均日剂量约为490、980、1,960、3,960或7,660 mg/kg体重,雌性为550、1,100、2,260、4,420或8,180 mg/kg体重),持续40周。接触阿斯巴甜对存活没有影响。从第15周到研究结束,50,000 ppm女性的平均体重大于对照组。在整个研究过程中,暴露组的饲料消耗量与对照组相似。没有肿瘤或非肿瘤性病变可归因于暴露于阿斯巴甜。为期9个月的p53单倍体缺失小鼠研究:每组15只雄性和15只雌性p53单倍体缺失小鼠被喂食含有0、3,125、6,250、12,500、25,000或50,000 ppm阿斯巴甜的饲料(相当于雄性的平均日剂量约为490、970、1,860、3,800或7,280 mg/kg,雌性为630、1,210、2,490、5,020或9,620 mg/kg),持续40周。接触阿斯巴甜对存活和平均体重没有影响。在整个研究过程中,暴露组的饲料消耗量与对照组相似。没有肿瘤或非肿瘤性病变归因于接触阿斯巴甜。对Cdkn2a缺陷小鼠进行为期9个月的研究:每组15只雄性和15只雌性Cdkn2a缺陷小鼠喂食含有0、3,125、6,250、12,500、25,000或50,000 ppm阿斯巴甜的饮食,持续40周(相当于雄性的平均日剂量约为约490、960、1,900、3,700和7,400 mg/kg,雌性为610、1,200、2,390、4,850和9,560 mg/kg)。所有暴露组的存活率与对照组相似。在29周和16周后,3125 ppm和6250 ppm的男性的平均体重分别低于对照组。在整个研究过程中,雌性小鼠的平均体重与对照组相似。暴露于6250、25,000或50,000 ppm阿斯巴甜的男性门静脉周围肝细胞出现轻微到轻度细胞质空泡的发生率明显高于对照组。遗传毒理学:阿斯巴甜对鼠伤寒沙门菌基因突变的诱导进行了测试。菌株TA98、TA100和TA1535在有无外源代谢激活的情况下均未检测到致突变性(S9)。此外,TA1537与30%大鼠肝脏S9的单次试验结果为阴性。然而,在含有30%大鼠肝脏S9的TA97中,观察到突变菌落的可重复的小幅度增加,这种反应被认为是模棱两可的。TA97不含S9或含仓鼠肝S9均无致突变性。用阿斯巴甜灌胃F344/N雄性大鼠进行急性骨髓微核试验。在任何剂量水平均未观察到微核多染红细胞的增加。Tg暴露9个月后进行外周血微核试验。AC半合子,p53单倍体不足和Cdkn2a缺陷小鼠对阿斯巴甜的剂量饲料。男女Tg均为阴性。AC半合子和Cdkn2a缺陷小鼠。雄性p53单倍体不足小鼠也得到阴性结果。在雌性p53单倍体不足小鼠中,根据显著的趋势检验和50,000 ppm组微核红细胞频率虽小但有统计学意义的增加,判断微核试验结果为阳性。结论:在这项为期9个月的饲料研究条件下,暴露于3,125,6,250,12,500,25,000或50,000 ppm的雄性或雌性p53单倍体不足小鼠中,没有证据表明阿斯巴甜具有致癌活性。由于这是一种新模型,因此尚不确定该研究是否具有足够的灵敏度来检测致癌效应。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
NTP report on the toxicology studies of aspartame (CAS No. 22839-47-0) in genetically modified (FVB Tg.AC hemizygous) and B6.129-Cdkn2atm1Rdp (N2) deficient mice and carcinogenicity studies of aspartame in genetically modified [B6.129-Trp53tm1Brd (N5) haploinsufficient] mice (feed studies).

Unlabelled: Aspartame is an artificial sweetener used throughout the world in food and beverages. Conventional 2-year rodent cancer studies of aspartame are considered negative, although a small number of neoplasms of the brain were observed in a rat study (Fed. Regist., 1981a,b). The NTP has explored the use of genetically altered mouse models as adjuncts to the 2-year rodent cancer assay. These models may prove to be more rapid, use fewer animals, and provide some mechanistic insights into neoplastic responses. As part of the evaluation of new mouse cancer screening models, aspartame was tested for potential toxicity and carcinogenicity in two relatively well-studied models, the Tg.AC hemizygous strain and the p53 haploinsufficient strain, and an uncharacterized model, the Cdkn2a deficient strain. Male and female Tg.AC hemizygous, p53 haploinsufficient, and Cdkn2a deficient mice were given feed containing aspartame (greater than 98% pure) for 9 months. Genetic toxicology studies were conducted in Salmonella typhimurium, rat bone marrow cells, and mouse peripheral blood erythrocytes. 9-MONTH STUDY IN Tg.AC HEMIZYGOUS MICE: Groups of 15 male and 15 female Tg.AC hemizygous mice were fed diets containing 0, 3,125, 6,250, 12,500, 25,000, or 50,000 ppm aspartame (equivalent to average daily doses of approximately 490, 980, 1,960, 3,960, or 7,660 mg aspartame/kg body weight to males and 550, 1,100, 2,260, 4,420, or 8,180 mg/kg to females) for 40 weeks. Exposure to aspartame had no effect on survival. The mean body weights of 50,000 ppm females were greater than those of the controls from week 15 until the end of the study. Feed consumption by the exposed groups was similar to that by the control groups throughout the study. There were no neoplasms or nonneoplastic lesions that were attributed to exposure to aspartame. 9-MONTH STUDY IN p53 HAPLOINSUFFICIENT MICE: Groups of 15 male and 15 female p53 haploinsufficient mice were fed diets containing 0, 3,125, 6,250, 12,500, 25,000, or 50,000 ppm aspartame (equivalent to average daily doses of approximately 490, 970, 1,860, 3,800, or 7,280 mg/kg to males and 630, 1,210, 2,490, 5,020, or 9,620 mg/kg to females) for 40 weeks. Exposure to aspartame had no effect on survival or mean body weights. Feed consumption by the exposed groups was similar to that by the control groups throughout the study. No neoplasms or nonneoplastic lesions were attributed to exposure to aspartame. 9-MONTH STUDY IN Cdkn2a DEFICIENT MICE: Groups of 15 male and 15 female Cdkn2a deficient mice were fed diets containing 0, 3,125, 6,250, 12,500, 25,000, or 50,000 ppm aspartame for 40 weeks (equivalent to average daily doses of approximately of approximately 490, 960, 1,900, 3,700, and 7,400 mg/kg to males and 610, 1,200, 2,390, 4,850, and 9,560 mg/kg to females). Survival of all exposed groups was similar to that of the control groups. Mean body weights of 3,125 and 6,250 ppm males were less than those of the controls after weeks 29 and 16, respectively. Mean body weights of female mice were similar to those of the controls throughout the study. The incidences of minimal to mild cytoplasmic vacuolization of periportal hepatocytes were significantly greater than controls in males exposed to 6,250, 25,000, or 50,000 ppm aspartame.

Genetic toxicology: Aspartame was tested for induction of gene mutations in Salmonella typhimurium. No mutagenicity was detected in strains TA98, TA100, or TA1535 with or without exogenous metabolic activation (S9). In addition, a single test in TA1537 with 30% rat liver S9 gave negative results. In TA97 with 30% rat liver S9, however, a reproducible small increase in mutant colonies was observed, and this response was judged to be equivocal. No mutagenicity was detected in TA97 without S9 or with hamster liver S9. An acute bone marrow micronucleus test was conducted with aspartame administered by gavage to male F344/N rats. No increase in micronucleated polychromatic erythrocytes was observed at any dose level. Peripheral blood micronucleus tests were conducted after 9 months exposure of Tg.AC hemizygous, p53 haploinsufficient, and Cdkn2a deficient mice to aspartame in dosed feed. Negative results were obtained in male and female Tg.AC hemizygous and Cdkn2a deficient mice. Negative results were also obtained with male p53 haploinsufficient mice. In female p53 haploinsufficient mice, the results of the micronucleus test were judged to be positive, based on a significant trend test and a small but statistically significant increased frequency of micronucleated erythrocytes in the 50,000 ppm group.

Conclusions: Under the conditions of this 9-month feed study, there was no evidence of carcinogenic activity of aspartame in male or female p53 haploinsufficient mice exposed to 3,125, 6,250, 12,500, 25,000, or 50,000 ppm. Because this is a new model, there is uncertainty whether the study possessed sufficient sensitivity to detect a carcinogenic effect.

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