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组蛋白H1的固有酪氨酸荧光。稳态和荧光衰减研究揭示了非均匀发射。

The intrinsic tyrosine fluorescence of histone H1. Steady state and fluorescence decay studies reveal heterogeneous emission.

作者信息

Libertini L J, Small E W

出版信息

Biophys J. 1985 Jun;47(6):765-72. doi: 10.1016/S0006-3495(85)83979-5.

Abstract

In wavelength-resolved steady state spectra we observe three different kinds of emission from histone H1, a class A protein with only a single tyrosine residue. Unfolded H1 emissions that peak at approximately 300 and 340 nm can both be excited maximally at approximately 280 nm. Another, peaking much further to the red at approximately 400 nm, can be excited maximally at approximately 320 nm. The 300-nm fluorescence can be resolved by lifetime measurements into three components with decay times of approximately 1, 2, and 4 ns. On sodium-chloride-induced refolding of H1, simplification of the emission properties occurs. The 340 and 400-nm components disappear while the two shorter lifetime components of the 300-nm band diminish in amplitude and are replaced by the 4-ns decay. We believe that the 340-nm emission is tyrosinate fluorescence resulting from excited-state proton transfer. The origin of the 400-nm emission remains uncertain. We assign the 1 and 2-ns components of the 300-nm emission to two states of tyrosine in denatured H1 and the 4-ns decay to fluorescence of the single tyrosine residue in the globular region of refolded H1. Our results support the contention that salt induced folding of H1 is a cooperative two state process, and permit us to better understand the previously reported increases in fluorescence intensity and anisotropy on salt-induced folding.

摘要

在波长分辨稳态光谱中,我们观察到组蛋白H1(一种仅含单个酪氨酸残基的A类蛋白质)有三种不同类型的发射。未折叠的H1发射在约300和340 nm处达到峰值,二者在约280 nm处均可被最大程度激发。另一种发射在约400 nm处向更长波长方向有更高峰值,在约320 nm处可被最大程度激发。300 nm处的荧光可通过寿命测量解析为三个成分,其衰减时间约为1、2和4 ns。在氯化钠诱导H1重折叠时,发射特性会简化。340和400 nm的成分消失,而300 nm波段中寿命较短的两个成分的幅度减小,并被4 ns的衰减所取代。我们认为340 nm处的发射是激发态质子转移产生的酪氨酸离子荧光。400 nm发射的起源仍不确定。我们将300 nm发射的1和2 ns成分归因于变性H1中酪氨酸的两种状态,将4 ns的衰减归因于重折叠H1球状区域中单个酪氨酸残基的荧光。我们的结果支持了盐诱导H1折叠是一个协同双态过程的论点,并使我们能够更好地理解先前报道的盐诱导折叠时荧光强度和各向异性增加的现象。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4c54/1435174/ac22ccec151b/biophysj00191-0019-a.jpg

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