Simonian M H, Goldstein R V, Mosteller R D
J Bacteriol. 1978 Feb;133(2):650-60. doi: 10.1128/jb.133.2.650-660.1978.
Genetic and segregation analysis of Escherichia coli strains containing a partial duplication of the trp operon reveal that the 2.5-min-long region trpD-purB is duplicated in tandem in the chromosome. The adjacent loci cysB and fabD are not duplicated. Although one copy of the duplicated region is longer than the maximum size of bacteriophage P1kc transducing fragments, the frequency at which the duplicated segment trpDCBA is transferred by transduction to tonB-trp deletion strains is equal to that observed for transfer of the normal trp operon. This suggests that three-point recombination events believed to account for transduction of long duplications occur as frequently as two-point recombination events believed to account for normal transduction. Cotransduction frequencies of trpDCBA with the duplicated loci tonB, galU, tyrT, and hemA are very similar to those for the trp operon with the same loci. This indicates that normal genetic linkage is maintained during the three-point recombination event. However, purB, which is normally unlinked to trp by transduction, is closely linked to trpDCBA and thus must be near the repeat point of the duplication. Transduction tests with point mutations in the trp operon indicated that the repeat point occurs near the normal boundary between trpE and trpD. Segregation analysis of heterogenotes constructed from tonB-trp deletion strains shows that the frequency at which a marker is lost is approximately proportional to its distance from the repeat point. This finding is consistent with a random, singlesite crossover event during segregation. Several observations indicate that non-reciprocal genetic exchange also occurs between copies of the duplication. Analysis of heterogenotes containing dadR1 and dadR(+) demonstrate that the mutant allele is transdominant.
对含有色氨酸操纵子部分重复的大肠杆菌菌株进行遗传和分离分析表明,染色体中2.5分钟长的trpD - purB区域串联重复。相邻的基因座cysB和fabD没有重复。尽管重复区域的一个拷贝长于噬菌体P1kc转导片段的最大大小,但重复片段trpDCBA通过转导转移到tonB - trp缺失菌株的频率与正常色氨酸操纵子转移时观察到的频率相同。这表明,被认为是长重复序列转导原因的三点重组事件发生的频率与被认为是正常转导原因的两点重组事件相同。trpDCBA与重复基因座tonB、galU、tyrT和hemA的共转导频率与色氨酸操纵子与相同基因座的共转导频率非常相似。这表明在三点重组事件中维持了正常的遗传连锁。然而,通常通过转导与色氨酸不连锁的purB与trpDCBA紧密连锁,因此一定靠近重复点。对色氨酸操纵子中的点突变进行转导测试表明,重复点出现在trpE和trpD的正常边界附近。对由tonB - trp缺失菌株构建的异源二倍体进行分离分析表明,一个标记丢失的频率与其距重复点的距离大致成比例。这一发现与分离过程中随机的单位点交叉事件一致。几项观察结果表明,重复序列的拷贝之间也发生了非互惠遗传交换。对含有dadR1和dadR(+)的异源二倍体的分析表明,突变等位基因是反式显性的。