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粪链球菌的自溶酶系统。3. 自溶素在细胞壁合成位点的定位。

Autolytic enzyme system of Streptococcus faecalis. 3. Localization of the autolysin at the sites of cell wall synthesis.

作者信息

Shockman G D, Pooley H M, Thompson J S

出版信息

J Bacteriol. 1967 Nov;94(5):1525-30. doi: 10.1128/jb.94.5.1525-1530.1967.

Abstract

Cell walls from exponential-phase cultures of Streptococcus faecalis ATCC 9790 autolyzed in dilute buffers. Walls were isolated from cultures grown in the presence of (14)C-lysine for about 10 generations and then on (12)C-lysine for 0.1 to 0.8 of a generation (prelabeled). These walls released (14)C to the soluble fraction more slowly than they lost turbidity during the initial stages of autolysis. Walls isolated from cultures grown in the presence of (14)C-lysine for only the last 0.1 to 0.4 of a generation (postlabeled) released (14)C to the supernatant fluid more rapidly than they lost turbidity. Autolysin in both pre- and postlabeled walls was inactivated, and such walls were then incubated in the presence of unlabeled walls containing active autolysin. The inactivated walls lost their (14)C label only very slowly until autolysis of the unlabeled walls was virtually complete and release of soluble autolysin was expected. When this experiment was done in the presence of trypsin, a fourfold increase in the autolysis rate resulted, but the same pattern of (14)C release was observed. A parallel release of (14)C and loss of turbidity from pre- or postlabeled walls was observed upon trypsin "activation" and by addition of isolated soluble autolysin to inactivated walls. We conclude that the wall-bound autolysin acts first on the more recently synthesized portion of the wall. Trypsin appears to speed wall autolysis by activating additional latent autolysin in situ at sites in the older portion of the wall.

摘要

粪肠球菌ATCC 9790指数生长期培养物的细胞壁在稀缓冲液中自溶。细胞壁是从在含(14)C - 赖氨酸的培养基中生长约10代,然后在含(12)C - 赖氨酸的培养基中生长0.1至0.8代(预标记)的培养物中分离得到的。在自溶初始阶段,这些细胞壁向可溶部分释放(14)C的速度比其浊度降低的速度慢。从仅在最后0.1至0.4代在含(14)C - 赖氨酸的培养基中生长的培养物中分离得到的细胞壁(后标记)向超滤液中释放(14)C的速度比其浊度降低的速度快。预标记和后标记细胞壁中的自溶素均失活,然后将这些细胞壁在含有活性自溶素的未标记细胞壁存在下孵育。失活的细胞壁仅非常缓慢地失去其(14)C标记,直到未标记细胞壁的自溶几乎完成且预期可溶自溶素释放。当在胰蛋白酶存在下进行该实验时,自溶速率提高了四倍,但观察到相同的(14)C释放模式。在胰蛋白酶“激活”以及向失活细胞壁中添加分离的可溶自溶素时,观察到预标记或后标记细胞壁中(14)C的平行释放和浊度降低。我们得出结论,壁结合自溶素首先作用于细胞壁中最新合成的部分。胰蛋白酶似乎通过在细胞壁较老部分的位点原位激活额外的潜在自溶素来加速细胞壁自溶。

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