Wei D, Maher V M, McCormick J J
Department of Microbiology, Michigan State University, East Lansing 48824.
Proc Natl Acad Sci U S A. 1995 Mar 14;92(6):2204-8. doi: 10.1073/pnas.92.6.2204.
When populations of repair-proficient diploid human fibroblasts were treated with (+/-)-7 beta, 8 alpha-dihydroxy-9 alpha, 10 alpha-epoxy-7,8,9,10-tetrahydrobenzo[a]pyrene (BPDE) during early S phase, just as the hypoxanthine phosphoribosyltransferase gene (HPRT) was being replicated, 5% of the induced base substitutions were found at nt 212, and 5% of the substitutions were found at nt 229 in exon 3. However, when the population was treated in early G1 phase to allow at least 12 hr for repair before the onset of S phase, 21% of the substitutions were found at nt 212, and 10% were found at nt 229. No such cell-cycle-dependent difference in distribution of base substitutions occurred in excision-repair-deficient cells. To test whether the increase in the relative frequency of mutations resulted from inefficient repair at these sites, we adapted ligation-mediated PCR to measure the rates of removal of BPDE adducts from individual sites in exon 3 of the HPRT gene. Cells were treated with 0.5 microM BPDE in early G1 phase and harvested immediately or after 10, 20, and 30 hr for repair. the nontranscribed strand of exon 3 was analyzed for the original distribution of adducts and those remaining after repair, using Escherichia coli UvrABC excinuclease to excise the adducts and annealing a 5' biotinylated gene-specific primer to the DNA and extending it with Sequenase 2.0 to generate a blunt end at the site of each cut. A linker was ligated to the blunt end, and the desired fragments were isolated from the rest of the genomic DNA by using magnetic beads, amplified by PCR, and analyzed on a sequencing gel. The distribution of fragments of particular lengths indicated the relative number of BPDE adducts initially formed or remaining at specific sites. The rates of repair at individual sites varied widely along exon 3 of the HPRT gene and were very slow at nt 212 and 229, strongly supporting the hypothesis that inefficient DNA repair plays an important role in the formation of mutation hotspots.
当具有修复能力的二倍体人成纤维细胞群体在S期早期,即次黄嘌呤磷酸核糖基转移酶基因(HPRT)正在复制时,用(±)-7β,8α-二羟基-9α,10α-环氧-7,8,9,10-四氢苯并[a]芘(BPDE)处理,发现诱导的碱基置换中有5%位于第212位核苷酸,外显子3中5%的置换位于第229位核苷酸。然而,当群体在G1期早期进行处理,以便在S期开始前至少有12小时进行修复时,发现21%的置换位于第212位核苷酸,10%位于第229位核苷酸。在切除修复缺陷的细胞中未出现这种碱基置换分布的细胞周期依赖性差异。为了测试突变相对频率的增加是否源于这些位点的修复效率低下,我们采用连接介导的PCR来测量HPRT基因外显子3中各个位点BPDE加合物的去除率。细胞在G1期早期用0.5 microM BPDE处理,并立即收获或在10、20和30小时后收获以进行修复。使用大肠杆菌UvrABC核酸内切酶切除加合物,并用5'生物素化的基因特异性引物与DNA退火,并用Sequenase 2.0将其延伸,以在每个切割位点产生平端,分析外显子3的非转录链中加合物的原始分布和修复后剩余的加合物。将接头连接到平端,使用磁珠从基因组DNA的其余部分中分离出所需片段,通过PCR扩增,并在测序凝胶上进行分析。特定长度片段的分布表明最初形成或留在特定位点的BPDE加合物的相对数量。沿着HPRT基因外显子3,各个位点的修复速率差异很大,在第212位和229位核苷酸处非常缓慢,这有力地支持了DNA修复效率低下在突变热点形成中起重要作用的假设。
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