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有证据表明局部重折叠事件会触发HK97噬菌体衣壳的成熟。

Evidence that a local refolding event triggers maturation of HK97 bacteriophage capsid.

作者信息

Lee Kelly K, Gan Lu, Tsuruta Hiro, Hendrix Roger W, Duda Robert L, Johnson John E

机构信息

Department of Molecular Biology and Center for Integrative Molecular Biosciences, The Scripps Research Institute, MB-31, 10550 North Torrey Pines Road, La Jolla, CA 92037, USA.

出版信息

J Mol Biol. 2004 Jul 9;340(3):419-33. doi: 10.1016/j.jmb.2004.05.008.

Abstract

Bacteriophage capsids are a striking example of a robust yet dynamic genome delivery vehicle. Like most phages, HK97 undergoes a conformational maturation that converts a metastable Prohead into the mature Head state. In the case of HK97, maturation involves a significant expansion of the capsid and concomitant cross-linking of capsid subunits. The final state, termed Head-II, is a 600 angstroms diameter icosahedral structure with catenated subunit rings. Cryo-EM, small angle X-ray scattering (SAXS), and biochemical assays were used previously to characterize the initial (Prohead-II) and final states (Head-II) as well as four maturation intermediates. Here we extend the characterization of the acid-induced expansion of HK97 in vitro by monitoring changes in intrinsic fluorescence, circular dichroism (CD), and SAXS. We find that the greatest changes in all observables occur at an early stage of maturation. Upon acidification, fluorescence emissions from HK97 exhibit a blueshift and decrease in intensity. These spectral changes reveal two kinetic phases of the expansion reaction. The early phase exhibits sensitivity to pH, increasing in rate nearly 200-fold when acidification pH is lowered from 4.5 to 3.9. The second, slower phase reported by fluorescence is relatively insensitive to pH. Time-resolved SAXS experiments report an increase in overall particle dimension that parallels the fluorescence changes for the early phase. Native agarose gel assays corroborated this finding. By contrast, probes of CD at far-UV indicate that secondary structural changes precede the early expansion phase reported by SAXS and fluorescence. Based on the crystallographic structure of Head-II and the pseudo-atomic model of Prohead-II, we interpret these changes as reflecting the conversion of subunit N-terminal arms (N-arm) from unstructured polypeptide to the mixture of beta-strand and beta-turn observed in the Head-II crystal structure. Refolding of the N-arm may thus represent the conformational trigger that initiates the irreversible expansion of the phage capsid.

摘要

噬菌体衣壳是一种强大而动态的基因组传递载体的显著例子。与大多数噬菌体一样,HK97经历构象成熟,将亚稳态的原头部转化为成熟的头部状态。就HK97而言,成熟涉及衣壳的显著扩张以及衣壳亚基的伴随交联。最终状态,称为头部-II,是一个直径600埃的二十面体结构,带有连环的亚基环。先前使用冷冻电镜、小角X射线散射(SAXS)和生化分析来表征初始(原头部-II)和最终状态(头部-II)以及四个成熟中间体。在这里,我们通过监测内在荧光、圆二色性(CD)和SAXS的变化,扩展了对HK97体外酸诱导扩张的表征。我们发现所有可观测指标的最大变化发生在成熟的早期阶段。酸化后,HK97的荧光发射出现蓝移且强度降低。这些光谱变化揭示了扩张反应的两个动力学阶段。早期阶段对pH敏感,当酸化pH从4.5降至3.9时,速率增加近200倍。荧光报告的第二个较慢阶段对pH相对不敏感。时间分辨SAXS实验报告了整体颗粒尺寸的增加,这与早期阶段的荧光变化平行。天然琼脂糖凝胶分析证实了这一发现。相比之下,远紫外CD探针表明二级结构变化先于SAXS和荧光报告的早期扩张阶段。基于头部-II的晶体结构和原头部-II的伪原子模型,我们将这些变化解释为反映亚基N端臂(N臂)从未结构化多肽转变为在头部-II晶体结构中观察到的β链和β转角的混合物。因此,N臂的重折叠可能代表启动噬菌体衣壳不可逆扩张的构象触发因素。

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