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枯草芽孢杆菌中的膜能量化与细胞自溶

The energized membrane and cellular autolysis in Bacillus subtilis.

作者信息

Jolliffe L K, Doyle R J, Streips U N

出版信息

Cell. 1981 Sep;25(3):753-63. doi: 10.1016/0092-8674(81)90183-5.

Abstract

Lysis of exponential cultures of B. subtilis follows the addition of reagents that dissipate either the electrical or pH gradients of cellular membranes. Stationary-phase cells or cultures that have been inhibited in division by macromolecular-synthesis inhibitors also lyse when uncoupling agents or ionophores are added to the growth medium. Autolysis occurs after brief starvation for a carbon source. Protoplasts are unaffected by azide or other lysis-inducing agents. Electron-donating agents, such as phenazine methosulfate and ascorbate, are effective in retarding autolysis. The addition of an oxidizable carbon source to starved and lysing cultures prevents their autolysis. These results suggest that cellular lysis in B. subtilis and energized membrane are tightly coupled. The fluorescence intensity and the wavelength of maximal fluorescence of 8-anilino-1-naphthalene sulfonic acid, when added to bacterial suspensions, appear to be qualitatively related to the rate of cell lysis. Analyses show that ATP limitations are probably not involved in the elicitation of lysis by ionophores, uncoupling agents or starvation. Measurements of protonmotive forces in the lysis-prone cells suggest that a threshold force of more than 85 mV may be required to maintain cellular integrity. Lipoteichoic acids, polyelectrolytes such as dextran sulfate or phospholipids do not modify the rate of cellular lysis when added to suspensions containing azide or other reagents that eliminate transmembrane protonmotive forces. We interpret the results to suggest that the in vivo control of autolysin activity in B. subtilis is related to the energized membrane

摘要

枯草芽孢杆菌指数生长期培养物在添加能消除细胞膜电势或pH梯度的试剂后会发生裂解。处于稳定期的细胞或因大分子合成抑制剂而抑制分裂的培养物,在向生长培养基中添加解偶联剂或离子载体时也会裂解。在短暂缺乏碳源饥饿后会发生自溶。原生质体不受叠氮化物或其他诱导裂解剂的影响。电子供体试剂,如硫酸吩嗪甲酯和抗坏血酸盐,可有效延缓自溶。向饥饿和正在裂解的培养物中添加可氧化碳源可防止其自溶。这些结果表明,枯草芽孢杆菌中的细胞裂解与活跃的细胞膜紧密相关。当将8-苯胺基-1-萘磺酸添加到细菌悬液中时,其荧光强度和最大荧光波长似乎与细胞裂解速率在质量上相关。分析表明,离子载体、解偶联剂或饥饿诱导裂解可能与ATP限制无关。对易于裂解的细胞中质子动力的测量表明,可能需要超过85 mV的阈值力来维持细胞完整性。当将脂磷壁酸、聚电解质如硫酸葡聚糖或磷脂添加到含有叠氮化物或其他消除跨膜质子动力的试剂的悬液中时,它们不会改变细胞裂解速率。我们对结果的解释是,枯草芽孢杆菌中自溶素活性的体内控制与活跃的细胞膜有关

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