Mychajlonka M, McDowell T D, Shockman G D
Infect Immun. 1980 Apr;28(1):65-73. doi: 10.1128/iai.28.1.65-73.1980.
Turnover of the cell wall peptidoglycan fraction of six different strains of Streptococcus mutans and eight different strains of Streptococcus sanguis was examined. Cells were grown in the presence of [3H]lysine and [14C]leucine for at least eight generations and then chased in growth medium lacking the two labels. At intervals during the chase, samples of cultures were removed, and the amounts of the two labeled precursors remaining in the peptidoglycan and protein fractions were quantitated. Similar experiments were done in which the pulse-labeling technique was used. In addition, cells were labeled in the presence of tetracycline or penicillin, chased with growth medium containing no inhibitor, and assayed at intervals during the chase for the amount of [3H]lysine present in peptidoglycan fractions. Studies of cultures of S. mutans strains FA-1, OMZ-61, OMZ-176, 6715, GS-5, and Ingbritt and of S. sanguis strains 10558, M-5, Wicky, DL-101, DL-1, 71X26, and 71X48 maintained in the exponential phase of growth in a chemically defined medium failed to show evidence of loss of insoluble peptidoglycan via turnover. Similarly, for the strains of S. mutans, insoluble peptidoglycan assembled during 2 h of benzylpenicillin or tetracycline treatment was also conserved during recovery from growth inhibition.
对六种不同变形链球菌菌株和八种不同血链球菌菌株的细胞壁肽聚糖部分的周转情况进行了检测。细胞在含有[³H]赖氨酸和[¹⁴C]亮氨酸的条件下生长至少八代,然后在不含这两种标记物的生长培养基中进行追踪培养。在追踪培养期间的不同时间间隔,取出培养物样本,对肽聚糖和蛋白质部分中剩余的两种标记前体的量进行定量。采用脉冲标记技术进行了类似的实验。此外,细胞在四环素或青霉素存在的情况下进行标记,然后用不含抑制剂的生长培养基进行追踪培养,并在追踪培养期间的不同时间间隔对肽聚糖部分中存在的[³H]赖氨酸量进行测定。对在化学限定培养基中处于指数生长期的变形链球菌菌株FA - 1、OMZ - 61、OMZ - 176、6715、GS - 5和Ingbritt以及血链球菌菌株10558、M - 5、Wicky、DL - 101、DL - 1、71X26和71X48的培养物研究未能显示出通过周转导致不溶性肽聚糖损失的证据。同样,对于变形链球菌菌株,在苄青霉素或四环素处理2小时期间组装的不溶性肽聚糖在从生长抑制中恢复的过程中也得以保留。
