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碘化物对哈维氏弧菌荧光素酶氢过氧黄素中间体荧光及活性的影响。

Effects of iodide on the fluorescence and activity of the hydroperoxyflavin intermediate of Vibrio harveyi luciferase.

作者信息

Huang Shouqin, Tu Shiao-Chun

机构信息

Department of Biology and Biochemistry, University of Houston, Houston, TX 77204-5001, USA.

出版信息

Photochem Photobiol. 2005 Mar-Apr;81(2):425-30. doi: 10.1562/2004-10-15-RA-344.

Abstract

The 4a-hydroperoxy-4a,5-dihydroFMN intermediate (II or HFOOH) of Vibrio harveyi luciferase is known to transform from a low quantum yield IIx to a high quantum yield (lambdamax 485 nm, uncorrected) IIy fluorescent species on exposure to excitation light. Similar results were observed with II prepared from the alphaH44A luciferase mutant, which is very weak in bioluminescence activity. Because of the rapid decay of the alphaH44A II, its true fluorescence was obscured by the more intense 520 nm fluorescence (uncorrected) from its decay product oxidized flavin mononucleotide (FMN). Potassium iodide (KI) at 0.2 M was effective in quenching the FMN fluorescence, leaving the 485 nm fluorescence of II from both the wild-type (WT) and alphaH44A luciferase readily detectable. For both II species, the luciferase-bound peroxyflavin was well shielded from KI quenching. KI also enhanced the decay rates of both the WT and alphaH44A II. For alphaH44A, the transformation of IIx to IIy can be induced by KI in the dark, and it is proposed to be a consequence of a luciferase conformational change. The WT II formed a bioluminescence-inactive complex with KI, resulting in two distinct decay time courses based on absorption changes and decreases of bioluminescence activity of II.

摘要

哈维弧菌荧光素酶的4a-氢过氧-4a,5-二氢黄素单核苷酸中间体(II或HFOOH)已知在暴露于激发光时会从低量子产率的IIx转变为高量子产率(未校正的λmax为485 nm)的IIy荧光物种。从生物发光活性非常弱的αH44A荧光素酶突变体制备的II也观察到了类似结果。由于αH44A II的快速衰减,其真实荧光被其衰变产物氧化黄素单核苷酸(FMN)更强的520 nm荧光(未校正)所掩盖。0.2 M的碘化钾(KI)可有效淬灭FMN荧光,使野生型(WT)和αH44A荧光素酶的II的485 nm荧光易于检测。对于这两种II物种,荧光素酶结合的过氧黄素均受到很好的保护,免受KI淬灭。KI还提高了WT和αH44A II的衰减速率。对于αH44A,IIx到IIy的转变可在黑暗中由KI诱导,据推测这是荧光素酶构象变化的结果。WT II与KI形成了生物发光无活性的复合物,基于吸收变化和II的生物发光活性降低,产生了两个不同的衰减时间进程。

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