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用N-(1-芘基)碘乙酰胺标记的马血小板原肌球蛋白的准分子荧光。

Excimer fluorescence of equine platelet tropomyosin labeled with N-(1-pyrenyl)iodoacetamide.

作者信息

Burtnick L D, Stewart D I, Clark I D, Smillie L B

出版信息

Biochemistry. 1986 Jul 1;25(13):3875-80. doi: 10.1021/bi00361a020.

DOI:10.1021/bi00361a020
PMID:3741838
Abstract

Tropomyosin from equine platelets was reacted with N-(1-pyrenyl)iodoacetamide, a sulfhydryl-specific fluorescent reagent, to give an average extent of incorporation of 1.12 pyrene (Py) groups per platelet tropomyosin (P-TM) chain. The predominant site of reaction on P-TM was the penultimate COOH-terminal residue, Cys-246. The high proportion of the total emission that is due to pyrene ecximers and the pretransition observed in thermal denaturation of Py-P-TM point to a rather loose structure for the COOH-terminal amino acid residues of P-TM. The label on Cys-246 also reports on end-to-end overlap interactions that occur between two different tropomyosin molecules. Additions to a Py-P-TM solution at low ionic strength of unlabeled P-TM, rabbit cardiac tropomyosin (C-TM), or a carboxypeptidase A treated, nonpolymerizable derivative of C-TM all reduce the extent of excimer fluorescence from the sample. Addition of salt greatly reduces the effects of the unlabeled TM species on the Py-P-TM emission spectrum. Circular dichroism measurements indicate Py-P-TM still to be greater than 95% helical. However, analysis of excimer fluorescence levels in samples that contained a constant protein concentration but different mole ratios of labeled to unlabeled P-TM suggests that the bulky pyrene group may diminish the tendency of Py-P-TM to polymerize in an end-to-end manner.

摘要

将马血小板中的原肌球蛋白与N-(1-芘基)碘乙酰胺(一种巯基特异性荧光试剂)反应,使得每个血小板原肌球蛋白(P-TM)链平均掺入1.12个芘(Py)基团。P-TM上的主要反应位点是倒数第二个COOH末端残基,即半胱氨酸-246。芘激基缔合物导致的总发射比例较高,以及在Py-P-TM热变性过程中观察到的预转变,表明P-TM的COOH末端氨基酸残基结构相当松散。半胱氨酸-246上的标记还反映了两个不同原肌球蛋白分子之间发生的端对端重叠相互作用。在低离子强度下,向Py-P-TM溶液中添加未标记的P-TM、兔心肌原肌球蛋白(C-TM)或经羧肽酶A处理的、不可聚合的C-TM衍生物,都会降低样品中激基缔合物荧光的程度。添加盐会大大降低未标记的TM物种对Py-P-TM发射光谱的影响。圆二色性测量表明Py-P-TM的螺旋结构仍大于95%。然而,对含有恒定蛋白质浓度但标记与未标记P-TM摩尔比不同的样品中的激基缔合物荧光水平进行分析表明,庞大的芘基团可能会降低Py-P-TM以端对端方式聚合的倾向。

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