Koch A L, Higgins M L
J Gen Microbiol. 1984 Apr;130(4):735-45. doi: 10.1099/00221287-130-4-735.
Computer reconstructions of 659 and 1325 whole mounted, shadowed cells, randomly chosen from cultures of Streptococcus faecalis undergoing balanced growth and doubling in mass every 83 min and 30 min, respectively, were used to analyse the cell cycle. The size limits and duration of phases of the cell cycle were estimated by applying a method previously described by the authors, details of which are given here to allow others to use the method. Deeply constricted cells whose primary septal radius, Rs, was less than or equal to 0.18 micron were considered as belonging to an E-phase ending the cell cycle. The statistical parameters of these E-phase cells were used to calculate the mean and coefficient of variation of dividing cells. These latter values, in turn, predicted the moments of the total population well enough so that the method's assumptions were judged adequately satisfied. Therefore, the method was considered applicable to other phases and sub-phases of the cell cycle of these two cultures. The E-phase cells were further classified as having either 0, 1 or 2 secondary growth zones, allowing us to calculate the percentage of newborn cells without growth zones. In the slow-growing cells, 69% of the cells arose with no growth zone. On the other hand, in more rapidly growing cells 16% of the cells or less arose with no growth zone. Our calculations showed that they could exist without a growth zone for only 2 and 0.1 min, respectively. We also classified cells as possessing a 'birth site' if the volume between the two daughter bands was greater than 0, but less than 0.06 micron3. From the statistical properties of such cells with new growth zones, the mean pole time, W, was estimated. We also estimated W from the size of cells in E-phase. The major conclusion is that the pole time is only slightly greater than the mass doubling time at both growth rates. Since DNA synthesis in S. faecalis takes longer (C = 50 to 52 min) than the mass doubling time in rich medium (30 min), a new round of chromosome replication must be initiated before the old round of synthesis is completed (dichotomous replication). Consequently, wall band splitting and initiation of chromosome replication do not occur simultaneously. It was also concluded that the cell initiates wall band splitting, resulting in pole formation and cell division, when the growth zones cannot function rapidly enough to allow the increase of surface area required to accommodate continuing production of cytoplasm.
从粪链球菌培养物中随机选取659个和1325个整装、带阴影的细胞进行计算机重建,这些培养物分别处于平衡生长阶段,质量每83分钟和30分钟翻倍一次,用于分析细胞周期。细胞周期各阶段的大小界限和持续时间是通过应用作者先前描述的一种方法来估计的,此处给出该方法的详细信息以便其他人使用。初级隔膜半径Rs小于或等于0.18微米的深度收缩细胞被认为属于结束细胞周期的E期。这些E期细胞的统计参数用于计算分裂细胞的平均值和变异系数。后者的值又能很好地预测整个群体的时刻,从而判断该方法的假设得到了充分满足。因此,该方法被认为适用于这两种培养物细胞周期的其他阶段和亚阶段。E期细胞进一步被分类为具有0、1或2个次生生长区,这使我们能够计算没有生长区的新生细胞的百分比。在生长缓慢的细胞中,69%的细胞产生时没有生长区。另一方面,在生长较快的细胞中,16%或更少的细胞产生时没有生长区。我们的计算表明,它们分别只能在没有生长区的情况下存在2分钟和0.1分钟。如果两个子带之间的体积大于0但小于0.06立方微米,我们也将细胞分类为具有“出生位点”。根据具有新生长区的此类细胞的统计特性,估计了平均极期W。我们还从E期细胞的大小估计了W。主要结论是,在两种生长速率下,极期仅略大于质量翻倍时间。由于粪链球菌中的DNA合成时间(C = 50至52分钟)比丰富培养基中的质量翻倍时间(30分钟)长,因此必须在新一轮染色体复制完成之前启动新一轮染色体复制(二分复制)。因此,壁带分裂和染色体复制的起始不会同时发生。还得出结论,当生长区不能足够快地发挥作用以允许增加表面积以适应细胞质的持续产生时,细胞启动壁带分裂,导致极形成和细胞分裂。
