Macrina F L, Weatherly G G, Curtiss R
J Bacteriol. 1974 Dec;120(3):1387-400. doi: 10.1128/jb.120.3.1387-1400.1974.
Alkaline sucrose velocity sedimentation and cesium chloride-ethidium bromide equilibrium centrifugation have been used to determine the number of copies per chromosomal equivalent of the relaxedly replicating R6K plasmid (a conjugative plasmid conferring ampicillin and streptomycin resistance) in two minicell-producing strains of Escherichia coli K-12. In one strain, the average number of covalently closed circular R6K molecules per chromosomal equivalent is 13 in log-phase and 35 in stationary-phase cells. In the other strain, there is an average of six covalently closed circular R6K molecules per chromosomal equivalent in both log- and stationary-phase cells. Selection from this strain of spontaneously occurring mutants resistant to high concentrations of ampicillin has been accomplished and such mutants show a two- to threefold increase in the number of R6K copies per chromosomal equivalent. Relative to the parental strain, mutants display the following properties: (i) elevated streptomycin resistance, (ii) a 10-fold increase in R6K conjugal transfer, (iii) a 10-fold increase in the amount of R6K plasmid deoxyribonucleic acid segregated into minicells, and (iv) a two- to threefold increase in R6K-specified beta-lactamase. The mutation(s) responsible for the increase in the number of R6K molecules per chromosomal equivalent is located on the bacterial chromosome. No R6K-linked mutations conferring the above phenotypes have been obtained. The mutations are presumed to be in chromosomal genes which play a role in the regulation of R6K replication in this strain.
碱性蔗糖速率沉降法和氯化铯-溴化乙锭平衡离心法已用于测定两株产微小细胞的大肠杆菌K-12中松弛复制型R6K质粒(一种赋予氨苄青霉素和链霉素抗性的接合质粒)每个染色体当量的拷贝数。在一个菌株中,对数期细胞每个染色体当量共价闭合环状R6K分子的平均数为13,稳定期细胞为35。在另一菌株中,对数期和稳定期细胞每个染色体当量平均有6个共价闭合环状R6K分子。已从该菌株中筛选出对高浓度氨苄青霉素具有抗性的自发突变体,这些突变体每个染色体当量的R6K拷贝数增加了两到三倍。相对于亲代菌株,突变体表现出以下特性:(i)链霉素抗性增强,(ii)R6K接合转移增加10倍,(iii)分配到微小细胞中的R6K质粒脱氧核糖核酸量增加10倍,以及(iv)R6K编码的β-内酰胺酶增加两到三倍。导致每个染色体当量R6K分子数量增加的突变位于细菌染色体上。未获得赋予上述表型的R6K连锁突变。推测这些突变存在于该菌株中对R6K复制调控起作用的染色体基因中。