Spiegelstein Ofer, Gould Amy, Wlodarczyk Bogdan, Tsie Marlene, Lu Xiufen, Le Chris, Troen Aron, Selhub Jacob, Piedrahita Jorge A, Salbaum J Michael, Kappen Claudia, Melnyk Stepan, James Jill, Finnell Richard H
Center for Environmental and Genetic Medicine, Institute of Biosciences and Technology, Texas A&M University System Health Science Center, Houston, TX 77030, USA.
Toxicol Appl Pharmacol. 2005 Feb 15;203(1):18-26. doi: 10.1016/j.taap.2004.07.006.
Previous studies have demonstrated that mice lacking a functional folate binding protein 2 gene (Folbp2-/-) were significantly more sensitive to in utero arsenic exposure than were the wild-type mice similarly exposed. When these mice were fed a folate-deficient diet, the embryotoxic effect of arsenate was further exacerbated. Contrary to expectations, studies on 24-h urinary speciation of sodium arsenate did not demonstrate any significant difference in arsenic biotransformation between Folbp2-/- and Folbp2+/+ mice. To better understand the influence of folate pathway genes on arsenic embryotoxicity, the present investigation utilized transgenic mice with disrupted folate binding protein 1 (Folbp1) and reduced folate carrier (RFC) genes. Because complete inactivation of Folbp1 and RFC genes results in embryonic lethality, we used heterozygous animals. Overall, no RFC genotype-related differences in embryonic susceptibility to arsenic exposure were observed. Embryonic lethality and neural tube defect (NTD) frequency in Folbp1 mice was dose-dependent and differed from the RFC mice; however, no genotype-related differences were observed. The RFC heterozygotes tended to have higher plasma levels of S-adenosylhomocysteine (SAH) than did the wild-type controls, although this effect was not robust. It is concluded that genetic modifications at the Folbp1 and RFC loci confers no particular sensitivity to arsenic toxicity compared to wild-type controls, thus disproving the working hypothesis that decreased methylating capacity of the genetically modified mice would put them at increased risk for arsenic-induced reproductive toxicity.
先前的研究表明,缺乏功能性叶酸结合蛋白2基因(Folbp2-/-)的小鼠比同样暴露于子宫内砷的野生型小鼠对砷暴露更为敏感。当给这些小鼠喂食叶酸缺乏的饮食时,砷酸盐的胚胎毒性作用会进一步加剧。与预期相反,关于砷酸钠24小时尿形态的研究并未表明Folbp2-/-和Folbp2+/+小鼠之间在砷生物转化方面有任何显著差异。为了更好地理解叶酸途径基因对砷胚胎毒性的影响,本研究利用了叶酸结合蛋白1(Folbp1)和叶酸载体(RFC)基因被破坏的转基因小鼠。由于Folbp1和RFC基因的完全失活会导致胚胎致死,我们使用了杂合动物。总体而言,未观察到RFC基因型与胚胎对砷暴露易感性之间的差异。Folbp1小鼠的胚胎致死率和神经管缺陷(NTD)频率呈剂量依赖性,且与RFC小鼠不同;然而,未观察到基因型相关的差异。RFC杂合子的血浆S-腺苷同型半胱氨酸(SAH)水平往往高于野生型对照,尽管这种影响并不显著。得出的结论是,与野生型对照相比,Folbp1和RFC位点的基因修饰对砷毒性没有特别的敏感性,从而推翻了转基因小鼠甲基化能力降低会使其砷诱导的生殖毒性风险增加的工作假设。