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首页> 外文期刊>The protein journal >Detection of tryptophan to tryptophan energy transfer in proteins.
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Detection of tryptophan to tryptophan energy transfer in proteins.

机译:检测蛋白质中色氨酸到色氨酸的能量转移。

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摘要

Forster resonance energy transfer (FRET) studies usually involve observation of intensity or lifetime changes in the donor or acceptor molecule and usually these donor and acceptor molecules differ (heterotransfer). The use of polarization to monitor FRET is far less common, although it was one of the first methods utilized. In 1960, Weber demonstrated that homotransfer between tryptophan molecules contributes to depolarization. He also discovered that the efficiency of homotransfer becomes much less effective upon excitation near the red-edge of the absorption. This "red-edge effect" was shown to be a general phenomenon of homotransfer. We have utilized Weber's red-edge effect to study tryptophan homotransfer in proteins. Specifically, we determined the polarization of the tryptophan fluorescence upon excitation at 295 nm and 310 nm (near the red-edge). Rotational diffusion leads to depolarization of the emission excited at either 295 nm or 310 nm, but homotransfer only contributes to depolarization upon excitation at 295 nm. Hence, the 310/295 polarization ratio gives an indication of tryptophan to tryptophan energy transfer. In single tryptophan systems, the 310/295 ratios are generally below 2 whereas in multi-tryptophan systems, the 310/295 ratios can be greater than 3.
机译:Forster共振能量转移(FRET)研究通常涉及观察供体或受体分子的强度或寿命变化,并且通常这些供体和受体分子是不同的(异源转移)。尽管偏振极化是最早使用的方法之一,但使用偏振来监测FRET却很少见。 1960年,韦伯证明色氨酸分子之间的均相转移有助于去极化。他还发现,在吸收的红边附近激发时,均质转移的效率变得低得多。这种“红边效应”被证明是同质转移的普遍现象。我们已经利用韦伯的红边效应来研究蛋白质中色氨酸的同质转移。具体而言,我们确定了在295 nm和310 nm(红边附近)激发后色氨酸荧光的偏振。旋转扩散导致在295 nm或310 nm激发的发射的去极化,但是同质转移仅在295 nm激发时有助于去极化。因此,310/295极化比给出了色氨酸到色氨酸能量转移的指示。在单色氨酸系统中,310/295比率通常低于2,而在多色氨酸系统中,310/295比率可以大于3。

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