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实时触发霍林。

Holin triggering in real time.

机构信息

Department of Biology, Texas A&M University, College Station, TX 77843, USA.

出版信息

Proc Natl Acad Sci U S A. 2011 Jan 11;108(2):798-803. doi: 10.1073/pnas.1011921108. Epub 2010 Dec 27.

Abstract

During λ infections, the holin S105 accumulates harmlessly in the membrane until, at an allele-specific time, suddenly triggering to form irregular holes of unprecedented size (>300 nm), releasing the endolysin from the cytoplasm, resulting in lysis within seconds. Here we used a functional S105-GFP chimera and real-time deconvolution fluorescence microscopy to show that the S105-GFP fusion accumulated in a uniformly distributed fashion, until suddenly, within 1 min, it formed aggregates, or rafts, at the time of lethal triggering. Moreover, the isogenic fusion to a nonlethal S105 mutant remained uniformly distributed, whereas a fusion to an early-lysing mutant showed early triggering and early raft formation. Protein accumulation rates of the WT, early, and nonlethal alleles were identical. Fluorescence recovery after photobleaching (FRAP) revealed that the nonlethal mutant and untriggered WT hybrids were highly mobile in the membrane, whereas the WT raft was essentially immobile. Finally, an antiholin allele, S105(ΔTMD1)-mcherryfp, in the product of which the S105 sequence deleted for the first transmembrane domain was fused to mCherryFP. This hybrid retained full antiholin activity, in that it blocked lethal hole formation by the S105-GFP fusion, accumulated uniformly throughout the host membrane and prevented the S105-GFP protein from forming rafts. These findings suggest that phage lysis occurs when the holin reaches a critical concentration and nucleates to form rafts, analogous to the initiation of purple membrane formation after the induction of bacteriorhodopsin in halobacteria. This model for holin function may be relevant for processes in mammalian cells, including the release of nonenveloped viruses and apoptosis.

摘要

在 λ 噬菌体感染过程中,孔蛋白 S105 会无害地在膜中积累,直到在特定等位基因的时间点,突然触发形成前所未有的大不规则孔(>300nm),将内溶素从细胞质中释放出来,导致细胞在几秒钟内裂解。在这里,我们使用功能 S105-GFP 嵌合体和实时反卷积荧光显微镜显示,S105-GFP 融合物均匀分布地积累,直到在致命触发的 1 分钟内突然形成聚集体或筏。此外,与非致死性 S105 突变体的同基因融合保持均匀分布,而与早期裂解突变体的融合则表现出早期触发和早期筏形成。WT、早期和非致死性等位基因的蛋白积累速率相同。光漂白荧光恢复(FRAP)显示,非致死性突变体和未触发的 WT 杂种在膜中具有高度的流动性,而 WT 筏则基本上是不动的。最后,我们构建了一个抗孔蛋白等位基因 S105(ΔTMD1)-mcherryfp,其产物中 S105 序列缺失了第一个跨膜结构域,与 mCherryFP 融合。该杂种保留了完整的抗孔蛋白活性,因为它阻断了 S105-GFP 融合物形成致命孔,在宿主膜中均匀积累,并防止 S105-GFP 蛋白形成筏。这些发现表明,当孔蛋白达到临界浓度并成核形成筏时,噬菌体裂解就会发生,类似于在嗜盐菌中诱导菌视紫红质后紫色膜的形成起始。这种孔蛋白功能模型可能与哺乳动物细胞中的过程有关,包括无包膜病毒的释放和细胞凋亡。

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