Pruess-Schwartz D, Baird W M, Nikbakht A, Merrick B A, Selkirk J K
Cancer Res. 1986 Jun;46(6):2697-702.
The benzo(a)pyrene (BaP):DNA adducts formed in normal human mammary epithelial cell cultures and the human mammary carcinoma T47D cell line were analyzed by chromatography and acid hydrolysis of the BaP:deoxyribonucleoside adducts to BaP:purine adducts and BaP:tetraols. Human mammary epithelial cell cultures and human mammary carcinoma T47D cells were exposed to [3H]BaP for 24 h, and the levels of binding were 81 and 182 pmol BaP/mg DNA in normal and T47D cultures, respectively. Analysis of BaP:deoxyribonucleoside adducts resolved by immobilized boronate chromatography and reversephase high-performance liquid chromatography demonstrated the presence of three BaP:deoxyribonucleoside adducts in both cells: M2, MS1, and MS2 in a ratio of 1.6:1:14. Two adducts (MS1 and MS2) bound to the immobilized boronate column indicating the presence of cis-vicinal hydroxyl groups, a configuration which would result from reaction of 7 beta, 8 alpha-dihydroxy-9 alpha, 10 alpha-epoxy-7,8,9,10-tetrahydroBaP (anti-BaPDE) with DNA. MS2 was identified as (+)-anti-BaPDE:deoxyguanosine (dGuo) for it cochromatographed with a [14C]-(+)-anti-BaPDE:dGuo marker, the BaP:purine hydrolysis product of MS2 cochromatographed with [14C]-(+)-anti-BaPDE:guanine, and the tetraol hydrolysis products cochromatographed with (+/-)-anti-BaPDE:tetraols. MS1 was identified as (-)-anti-BaPDE:dGuo for MS1 eluted in the same relative position as a (-)-anti-BaPDE:dGuo marker, the BaP:purine hydrolysis product of MS1 cochromatographed with [14C]-(+)-anti-BaPDE:guanine, and the tetraol hydrolysis products cochromatographed with (+/-)-anti-BaPDE:tetraols. Thus, both adducts that bound to the immobilized boronate column were formed from (+/-)-anti-BaPDE. One major adduct that did not contain cis-vicinal hydroxy groups, M2, was detected in both cell types. M2 was formed from (+/-)-7 beta, 8 alpha-dihydroxy-9 beta, 10 beta-epoxy-7,8,9,10-tetrahydroBaP (syn-BaPDE) as M2 eluted in the same relative position as a syn-BaPDE:dGuo adduct marker and the tetraol hydrolysis products of M2 cochromatographed with tetraols formed from (+/-)-syn-BaPDE. The isolation of the individual BaP:DNA adducts followed by acid hydrolysis allowed the identification of the BaP:DNA adducts formed in human mammary cell cultures and demonstrated the presence of (-)-anti-BaPDE:dGuo. Thus, this work provides the first evidence, other than cochromatography, that (-)-anti-BaPDE is formed in cell systems and reacts with DNA in cells to form (-)-anti-BaPDE:dGuo.(ABSTRACT TRUNCATED AT 400 WORDS)
通过对苯并(a)芘(BaP):脱氧核糖核苷加合物进行色谱分析,并将BaP:脱氧核糖核苷加合物酸水解为BaP:嘌呤加合物和BaP:四醇,对正常人乳腺上皮细胞培养物和人乳腺癌T47D细胞系中形成的BaP:DNA加合物进行了分析。将人乳腺上皮细胞培养物和人乳腺癌T47D细胞暴露于[3H]BaP 24小时,正常培养物和T47D培养物中的结合水平分别为81和182 pmol BaP/mg DNA。通过固定化硼酸酯色谱法和反相高效液相色谱法对BaP:脱氧核糖核苷加合物进行分析,结果表明两种细胞中均存在三种BaP:脱氧核糖核苷加合物:M2、MS1和MS2,其比例为1.6:1:14。两种加合物(MS1和MS2)与固定化硼酸酯柱结合,表明存在顺式邻位羟基,这种构型是由7β,8α-二羟基-9α,10α-环氧-7,8,9,10-四氢BaP(反式-BaPDE)与DNA反应产生的。MS2被鉴定为(+)-反式-BaPDE:脱氧鸟苷(dGuo),因为它与[14C]-(+)-反式-BaPDE:dGuo标记物共色谱,MS2的BaP:嘌呤水解产物与[14C]-(+)-反式-BaPDE:鸟嘌呤共色谱,四醇水解产物与(+/-)-反式-BaPDE:四醇共色谱。MS1被鉴定为(-)-反式-BaPDE:dGuo,因为MS1在与(-)-反式-BaPDE:dGuo标记物相同的相对位置洗脱,MS1的BaP:嘌呤水解产物与[14C]-(+)-反式-BaPDE:鸟嘌呤共色谱,四醇水解产物与(+/-)-反式-BaPDE:四醇共色谱。因此,与固定化硼酸酯柱结合的两种加合物均由(+/-)-反式-BaPDE形成。在两种细胞类型中均检测到一种不含顺式邻位羟基的主要加合物M2。M2由(+/-)-7β,8α-二羟基-9β,10β-环氧-7,8,9,10-四氢BaP(顺式-BaPDE)形成,因为M2在与顺式-BaPDE:dGuo加合物标记物相同的相对位置洗脱,M2的四醇水解产物与由(+/-)-顺式-BaPDE形成的四醇共色谱。分离出单个BaP:DNA加合物后进行酸水解,从而鉴定出人乳腺细胞培养物中形成的BaP:DNA加合物,并证明了(-)-反式-BaPDE:dGuo的存在。因此,这项工作提供了除共色谱法之外的首个证据,即(-)-反式-BaPDE在细胞系统中形成并与细胞中的DNA反应形成(-)-反式-BaPDE:dGuo。(摘要截断于400字)
