Van Schooten F J, Kriek E, Steenwinkel M J, Noteborn H P, Hillebrand M J, Van Leeuwen F E
Carcinogenesis. 1987 Sep;8(9):1263-9. doi: 10.1093/carcin/8.9.1263.
A number of polyclonal antibodies specific for DNA modified with (+/-)trans-7,8-dihydroxy-anti-9,10-epoxy-7,8,9,10-tetrahydrobenzo[a]pyre ne (BPDE) were obtained from the sera of New Zealand white rabbits immunized with BPDE-DNA, complexed with methylated bovine serum albumin (mBSA). Monoclonal antibodies were developed by fusion of mouse myeloma cells with spleen cells isolated from BALB/c mice immunized with the same complex of BPDE-DNA and mBSA. These antibodies have been characterized for specificity in a highly sensitive, enzyme-linked immunosorbent assay (ELISA). All antibodies showed a very high affinity for single-stranded BPDE-DNA, but had lower affinity towards native BPDE-DNA. The affinity for the free mononucleoside BPDE-dG was at least 100-fold lower than that for BPDE-DNA, and no affinity was detected for BP tetrols or DNA modified with N-acetoxy-N-acetyl-2-aminofluorene. A high cross reactivity was observed with DNA modified with (+/-)-trans-1,2-dihydroxy-anti-3,4-epoxy-1,2,3,4-tetrahydrochrysene++ +. Using five different antibodies, monoclonal or polyclonal, we observed that the antibody affinity for BPDE-DNA was dependent on the level of modification; in the competitive ELISA as little as 4 fmol BPDE-DNA (50 pmol/micrograms) was sufficient for 50% inhibition with our best antisera, but 17 fmol of the adduct was required when [3H]BPDE-DNA of low modification (1-10 fmol/micrograms) was used as inhibitor. When samples of [3H]BP-DNA isolated from the livers of mice, treated i.p. with different doses of [3H]BP were examined by competitive ELISA and calibrated with [3H]BPDE-DNA of low modification (1-10 fmol/micrograms), binding values calculated from the immunoassay were in good agreement with those obtained from radioactivity measurements. In contrast, when this DNA was quantitated in competitive ELISA using highly modified BPDE-DNA as standards, values by ELISA were 20-40% of those obtained by radioactivity. These results indicate that the use of serially diluted BPDE-DNA of high modification as standard competitor in the ELISA will lead to erroneous results in the measurement of adducts in DNAs modified to a low extent (biological samples). The property of antisera specific for BP-DNA, recognizing highly modified DNA more efficiently than DNA modified to a low extent, may be common to all antisera elicited against highly modified DNA immunogens. Therefore we conclude that antibody affinity must be tested also with DNA samples of low modification, obtained either in vitro or in vivo.
用(±)反式-7,8-二羟基-9,10-环氧-7,8,9,10-四氢苯并[a]芘(BPDE)修饰的DNA制备了多种多克隆抗体,这些抗体取自用BPDE-DNA与甲基化牛血清白蛋白(mBSA)复合后免疫的新西兰白兔血清。通过将小鼠骨髓瘤细胞与从用相同的BPDE-DNA和mBSA复合物免疫的BALB/c小鼠中分离的脾细胞融合,制备了单克隆抗体。这些抗体在高灵敏度的酶联免疫吸附测定(ELISA)中进行了特异性鉴定。所有抗体对单链BPDE-DNA表现出非常高的亲和力,但对天然BPDE-DNA的亲和力较低。对游离单核苷BPDE-dG的亲和力比对BPDE-DNA的亲和力至少低100倍,对BP四醇或用N-乙酰氧基-N-乙酰-2-氨基芴修饰的DNA未检测到亲和力。观察到与用(±)-反式-1,2-二羟基-9,10-环氧-1,2,3,4-四氢并四苯修饰的DNA有高交叉反应性。使用五种不同的单克隆或多克隆抗体,我们观察到抗体对BPDE-DNA的亲和力取决于修饰水平;在竞争ELISA中,对于我们最好的抗血清,低至4 fmol BPDE-DNA(50 pmol/μg)就足以产生50%的抑制,但当使用低修饰(1 - 10 fmol/μg)的[3H]BPDE-DNA作为抑制剂时,需要17 fmol的加合物。当通过竞争ELISA检测从经腹腔注射不同剂量[3H]BP处理的小鼠肝脏中分离的[3H]BP-DNA样品,并用低修饰(1 - 10 fmol/μg)的[3H]BPDE-DNA进行校准时,免疫测定计算得到的结合值与放射性测量得到的值非常一致。相反,当使用高度修饰的BPDE-DNA作为标准在竞争ELISA中对该DNA进行定量时,ELISA得到的值是放射性测量值的20 - 40%。这些结果表明,在ELISA中使用系列稀释的高度修饰的BPDE-DNA作为标准竞争者会导致对低程度修饰的DNA(生物样品)中加合物测量的错误结果。对BP-DNA具有特异性的抗血清,比低程度修饰的DNA更有效地识别高度修饰的DNA,这一特性可能是所有针对高度修饰的DNA免疫原产生的抗血清所共有的。因此我们得出结论,还必须用体外或体内获得的低修饰DNA样品测试抗体亲和力。
