Kaderlik K R, Minchin R F, Mulder G J, Ilett K F, Daugaard-Jenson M, Teitel C H, Kadlubar F F
National Center for Toxicological Research (HFT-100), Jefferson, AR 72079.
Carcinogenesis. 1994 Aug;15(8):1703-9. doi: 10.1093/carcin/15.8.1703.
The food-borne mutagen 2-amino-1-methyl-6-phenylimidazo[4,5-b]pyridine (PhIP) induces tumors in colon of male rats and has been implicated in the etiology of human cancers, particularly colorectal cancer. This study was conducted to examine: (1) the biliary and/or circulatory transport of N-hydroxy-PhIP and its N-glucuronides, N-sulfonyloxy-PhIP and N-acetoxy-PhIP; (2) their role as proximate and ultimate carcinogenic metabolites of PhIP; (3) the potential role of glutathione in modulating PhIP-DNA adduct formation. PhIP-DNA adducts, measured by the 32P-postlabeling method, were highest in the pancreas (361 adducts/10(8) nucleotides or 100%), followed by colon (56%), lung (28%), heart (27%) and liver (2%), at 24 h after a single oral dose of PhIP (220 mumol/kg) to male rats. In each tissue examined, we observed two major adducts, each of which accounted for 35-45% of the total, and one minor adduct, which represented about 10-20% of the total. One of the major adducts was identified as N-(deoxyguanosin-8-yl)-2-amino-1-methyl-6-phenylimidazo[4,5- b]pyridine by chromatographic comparisons with an authentic standard. The major urinary metabolites of PhIP in these rats were 4'-hydroxy-PhIP and its glucuronide and sulfate conjugates, followed by N-hydroxy-PhIP N3-glucuronide, N-hydroxy-PhIP N2-glucuronide and unchanged PhIP. In bile duct-ligated rats, the urinary excretion of the N-OH-PhIP N3-glucuronide was increased two-fold, but there was no effect on PhIP-DNA adduct formation in the colon, heart, lung, pancreas or liver. 2,6-Dichloro-4-nitrophenol, which strongly inhibits arylsulfo-transferase-mediated DNA binding in vivo, had no effect on PhIP-DNA adduct levels in liver or in extrahepatic tissues. Pretreatment of rats with buthionine sulfoximine, which results in hepatic glutathione depletion, caused a five-fold increase in adduct formation in the liver. Intravenous administration (10 mumol/kg) of N-hydroxy-PhIP and N-acetoxy-PhIP each led to high levels of PhIP-DNA adducts in each of the extrahepatic tissues examined. Adduct levels ranged from two- to six-fold higher (for N-hydroxy-PhIP) and four- to 28-fold higher (for N-acetoxy-PhIP) as compared to that after an i.v. dose of the parent compound, indicating that these two bioactivated derivatives of PhIP are sufficiently stable to be transported through the circulation to extrahepatic tissues.(ABSTRACT TRUNCATED AT 400 WORDS)
食源性诱变剂2-氨基-1-甲基-6-苯基咪唑并[4,5-b]吡啶(PhIP)可诱发雄性大鼠结肠肿瘤,并且被认为与人类癌症尤其是结直肠癌的病因有关。本研究旨在检测:(1)N-羟基-PhIP及其N-葡萄糖醛酸苷、N-磺酰氧基-PhIP和N-乙酰氧基-PhIP的胆汁和/或循环转运;(2)它们作为PhIP的近端和最终致癌代谢物的作用;(3)谷胱甘肽在调节PhIP-DNA加合物形成中的潜在作用。通过32P后标记法测定,在雄性大鼠单次口服PhIP(220μmol/kg)后24小时,胰腺中的PhIP-DNA加合物含量最高(361个加合物/10^8个核苷酸或100%),其次是结肠(56%)、肺(28%)、心脏(27%)和肝脏(2%)。在每个检测的组织中,我们观察到两种主要加合物,每种占总量的35-45%,以及一种次要加合物,约占总量的10-20%。通过与标准品进行色谱比较,其中一种主要加合物被鉴定为N-(脱氧鸟苷-8-基)-2-氨基-1-甲基-6-苯基咪唑并[4,5-b]吡啶。这些大鼠中PhIP的主要尿液代谢物是4'-羟基-PhIP及其葡萄糖醛酸苷和硫酸盐结合物,其次是N-羟基-PhIP N3-葡萄糖醛酸苷、N-羟基-PhIP N2-葡萄糖醛酸苷和未变化的PhIP。在胆管结扎的大鼠中,N-OH-PhIP N3-葡萄糖醛酸苷的尿液排泄增加了两倍,但对结肠、心脏、肺、胰腺或肝脏中的PhIP-DNA加合物形成没有影响。2,6-二氯-4-硝基苯酚在体内强烈抑制芳基磺基转移酶介导的DNA结合,对肝脏或肝外组织中的PhIP-DNA加合物水平没有影响。用丁硫氨酸亚砜胺预处理大鼠会导致肝脏谷胱甘肽耗竭,使肝脏中的加合物形成增加五倍。静脉注射(10μmol/kg)N-羟基-PhIP和N-乙酰氧基-PhIP均导致每个检测的肝外组织中PhIP-DNA加合物水平升高。与静脉注射母体化合物后的加合物水平相比,加合物水平高出2至6倍(对于N-羟基-PhIP)和4至28倍(对于N-乙酰氧基-PhIP),表明PhIP的这两种生物活化衍生物足够稳定,能够通过循环转运到肝外组织。(摘要截断于400字)
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