Smith C A
Department of Biological Sciences, Stanford University, CA 94305-5020.
J Cell Sci Suppl. 1987;6:225-41. doi: 10.1242/jcs.1984.supplement_6.16.
To investigate the influence of function or activity of a DNA sequence on its repair, we have studied excision repair of a number of adducts in the non-transcribed, heterochromatic alpha DNA of monkey cells (by physically isolating the DNA) and also the removal of pyrimidine dimers in a number of genes in rodent and human cells (by an indirect assay using a dimer-specific endonuclease). In confluent cells, psoralen and aflatoxin B1 (AFB1) adducts are produced in similar frequencies in alpha and in the rest of the DNA, but removal from alpha is severely deficient. Adducts of N-acetoxyacetylaminofluorene (NA-AAF) are formed in slightly higher frequencies in alpha, and removal is slightly deficient. The removal of thymine glycols from alpha DNA in gamma-irradiated cells is proficient, as is repair synthesis elicited by exposure to methyl methane sulphonate, dimethyl sulphate, or 254 nm ultraviolet light (u.v.). Removal of AFB1 and NA-AAF adducts from alpha is enhanced by small doses of u.v. but not by X-rays or DMS. The quantum efficiency of conversion of psoralen monoadducts to crosslinks is much lower in alpha DNA. Taken together, these results suggest that the highly condensed chromatin structure of alpha hinders access of the repair system that acts on bulky adducts but not of systems for repair of specific base damage, u.v. damage may alter this chromatin structure directly or facilitate the action of some system that changes accessibility of chromatin to repair. The repair deficiencies are not observed in actively growing cells, in which chromatin structure may be less condensed due to DNA replication. We have also demonstrated preferential excision repair of pyrimidine dimers in active genes. Dimers are efficiently removed from the essential dihydrofolate reductase (DHFR) and hydroxymethylglutaryl CoA reductase genes in Chinese hamster ovary (CHO) cells and from the transcribed c-ab1 proto-oncogene in the mouse cells. Both cell types remove few dimers from their overall genomes or from sequences distal to the DHFR gene; dimers are also removed poorly from the non-transcribed mouse c-mos gene. In human cells, dimers are removed more rapidly from the DHFR gene than from the genome as a whole. However, repair is as deficient in this gene in XP-C cells as it is in the entire genome. These results suggest that resistance to DNA damage correlates better with repair of vital or active sequences than with overall repair levels and that mutagenic efficiency may vary according to the activity of the gene under study.
为了研究DNA序列的功能或活性对其修复的影响,我们研究了猴细胞非转录异染色质α-DNA中多种加合物的切除修复(通过物理分离DNA),以及啮齿动物和人类细胞中多个基因中嘧啶二聚体的去除(通过使用二聚体特异性内切酶的间接检测法)。在汇合细胞中,补骨脂素和黄曲霉毒素B1(AFB1)加合物在α-DNA和其余DNA中的产生频率相似,但从α-DNA中的去除严重不足。N-乙酰氧基乙酰氨基芴(NA-AAF)的加合物在α-DNA中的形成频率略高,去除也略有不足。γ射线照射细胞中α-DNA上胸腺嘧啶乙二醇的去除是正常的,暴露于甲基磺酸甲酯、硫酸二甲酯或254nm紫外线(uv)引发的修复合成也是正常的。小剂量uv可增强α-DNA中AFB1和NA-AAF加合物的去除,但X射线或硫酸二甲酯(DMS)则不能。补骨脂素单加合物转化为交联物的量子效率在α-DNA中要低得多。综合这些结果表明,α-DNA高度浓缩的染色质结构阻碍了作用于大分子加合物的修复系统的进入,但不阻碍特定碱基损伤修复系统的进入,uv损伤可能直接改变这种染色质结构,或促进某些改变染色质可及性以进行修复的系统的作用。在活跃生长的细胞中未观察到修复缺陷,在这些细胞中,由于DNA复制,染色质结构可能不那么浓缩。我们还证明了活性基因中嘧啶二聚体的优先切除修复。二聚体在中国仓鼠卵巢(CHO)细胞的必需二氢叶酸还原酶(DHFR)和羟甲基戊二酰辅酶A还原酶基因以及小鼠细胞中转录的c-ab1原癌基因中被有效去除。两种细胞类型从其整个基因组或DHFR基因远端序列中去除的二聚体很少;二聚体从非转录的小鼠c-mos基因中也去除得很差。在人类细胞中,二聚体从DHFR基因中的去除比从整个基因组中更快。然而,在XP-C细胞中,该基因的修复与整个基因组一样不足。这些结果表明,对DNA损伤的抗性与重要或活性序列的修复相关性更好,而不是与总体修复水平相关,并且诱变效率可能根据所研究基因的活性而有所不同。
