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关于白蛋白结合胆红素的光致荧光增强和构象稳定性的调节:ε-NH₂基团封闭和氯仿结合的影响

On the modulation of photoinduced fluorescence enhancement and conformational stability of albumin-bound bilirubin: effect of epsilon-NH(2) groups blocking and chloroform binding.

作者信息

Khan M M, Tayyab S

机构信息

Interdisciplinary Biotechnology Unit, Aligarh Muslim University, 202002, Aligarh, India.

出版信息

Biochim Biophys Acta. 2000 Oct 18;1523(2-3):147-53. doi: 10.1016/s0304-4165(00)00114-8.

DOI:10.1016/s0304-4165(00)00114-8
PMID:11042378
Abstract

Photoinduced fluorescence enhancement of bilirubin bound to primary binding site on human serum albumin (HSA) was completely ceased when epsilon-NH(2) groups of its internal lysine residues were covalently blocked by acetylation or succinylation though the pigment bound to these derivatives in a folded conformation akin to that bound to HSA. These photoinduced fluorescence modulations cannot be ascribed to the binding of bilirubin to secondary low affinity sites as the CD spectrum of bilirubin bound to these derivatives showed complete inversion upon addition of chloroform which binds to subdomain IIA in HSA where high affinity bilirubin binding site is located. Presence of chloroform reconciled the photoinduced alterations in the CD spectrum observed in its absence, suggesting that chloroform stabilized the bound ligand against light but the fluorescence properties of bilirubin complexed with acetylated or succinylated derivatives remained unchanged. Guanidination of internal epsilon-NH(2) groups in HSA by O-methylisourea did not alter the spectral properties of the bound ligand. These results suggest that salt linkage(s) existing between epsilon-NH(2) groups of lysine residues in HSA and carboxyl groups of bilirubin, act(s) as a potential barrier during conformational rotation of the bound ligand assisted by photoactivation and their abolishment can alter its dynamics and stereoselectivity, a hitherto unnoticed implication of salt linkage(s) in BR-HSA complex.

摘要

当人血清白蛋白(HSA)内部赖氨酸残基的ε-NH₂基团通过乙酰化或琥珀酰化被共价阻断时,与HSA上主要结合位点结合的胆红素的光诱导荧光增强完全停止,尽管该色素以类似于与HSA结合的折叠构象与这些衍生物结合。这些光诱导荧光调制不能归因于胆红素与二级低亲和力位点的结合,因为与这些衍生物结合的胆红素的圆二色光谱在加入氯仿后显示出完全反转,氯仿与HSA中高亲和力胆红素结合位点所在的亚结构域IIA结合。氯仿的存在使在其不存在时观察到的圆二色光谱中的光诱导变化得到调和,表明氯仿使结合的配体对光稳定,但与乙酰化或琥珀酰化衍生物复合的胆红素的荧光特性保持不变。用O-甲基异脲对HSA内部的ε-NH₂基团进行胍基化不会改变结合配体的光谱特性。这些结果表明,HSA中赖氨酸残基的ε-NH₂基团与胆红素羧基之间存在的盐键在光激活辅助的结合配体构象旋转过程中起到潜在屏障的作用,其消除可以改变其动力学和立体选择性,这是胆红素-HSA复合物中盐键迄今未被注意到的影响。

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