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噬菌体φX174的吸附与隐蔽机制。II. 与分离的大肠杆菌细胞壁脂多糖的附着及隐蔽

Mechanism of adsorption and eclipse of bacteriophage phi X174. II. Attachment and eclipse with isolated Escherichia coli cell wall lipopolysaccharide.

作者信息

Incardona N L, Selvidge L

出版信息

J Virol. 1973 May;11(5):775-82. doi: 10.1128/JVI.11.5.775-782.1973.

Abstract

A mixture of aqueous phenol, choloroform, and ether extracts the lipopolysaccharides (LPS) from the phiX174-sensitive strain, Escherichia coli C/1, and resistant strains, C/phiX and K12. Interaction of the C/1 LPS with phiX in a starvation buffer containing 10(-3) M CaCl(2) at 37 C, but not at 15 C, results in a first-order inactivation that is specific for C/1 LPS. After interaction for 60 min at 15 C, followed by centrifugation, 37 and 20% of a (14)C-phiX preparation are bound to the C/1 and C/phiX LPS pellets, respectively. The results for intact cells are 75 and 10%. Supporting the conclusion that this represents specific attachment of phiX to its receptor site in the LPS is the fact that EDTA-borate buffer is required to elute 85% of the (14)C-phiX from the C/1 LPS, whereas starvation buffer elutes the same amount from C/phiX LPS. Moreover, 95% of the PFU are found in the C/1 LPS pellets as compared with 50% in the resistant strain LPS pellets. When the products of interaction between phiX and LPS at 37 C are examined by sucrose density gradients in EDTA-borate, a single 60 to 90S peak is observed in the C/1 sample, and the single peak cosediments with the 120S marker phiX in the C/phiX sample. This change in S(20, w) is very similar to that reported for the eclipse of phiX in vivo. If the inactivation at 37 C is carried out on phiX-LPS complexes first formed at 15 C, the first-order kinetics are biphasic and nearly identical to that observed for the eclipse kinetics of phiX attached to intact cells. Thus, the phiX-LPS system is suitable for in vitro studies on the early events in phiX infection.

摘要

苯酚、氯仿和乙醚的混合水溶液可从对φX174敏感的大肠杆菌C/1菌株以及抗性菌株C/φX和K12中提取脂多糖(LPS)。在含有10⁻³M氯化钙的饥饿缓冲液中,C/1 LPS与φX在37℃而非15℃下相互作用,会导致一级失活,且这种失活对C/1 LPS具有特异性。在15℃下相互作用60分钟后进行离心,分别有37%和20%的¹⁴C-φX制剂与C/1和C/φX LPS沉淀结合。完整细胞的结果分别为75%和10%。EDTA-硼酸盐缓冲液需要洗脱C/1 LPS中85%的¹⁴C-φX,而饥饿缓冲液能从C/φX LPS中洗脱相同量的¹⁴C-φX,这一事实支持了这代表φX特异性附着于LPS中其受体位点的结论。此外,在C/1 LPS沉淀中发现95%的噬菌斑形成单位(PFU),而在抗性菌株LPS沉淀中为50%。当在EDTA-硼酸盐中通过蔗糖密度梯度检查37℃下φX与LPS相互作用的产物时,在C/1样品中观察到一个单一的60至90S峰,且该单峰与C/φX样品中的120S标记φX共沉降。这种沉降系数(S(20,w))的变化与体内φX隐蔽期报道的情况非常相似。如果在15℃下首先形成的φX-LPS复合物在37℃下进行失活,一级动力学是双相的,并且与附着于完整细胞的φX隐蔽期动力学观察到的情况几乎相同。因此,φX-LPS系统适用于对φX感染早期事件的体外研究。

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