血管紧张素i转换酶的光谱研究。

Enzyme & protein Pub Date : 1994-01-01 DOI:10.1159/000474999
B Baudin, N Mario, S Gaba, J Giboudeau
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引用次数: 6

摘要

利用近紫外和远紫外分光光度法重新测定了肺血管紧张素转换酶(ACE)在280 nm处的摩尔消光系数(epsilon 280),测定了其色氨酸和酪氨酸含量,并对胍变性进行了随访。在变性条件下,通过SDS-PAGE和毛细管电泳检测ACE的纯度。纯化后的ACE溶解于pH 6.5的磷酸盐缓冲液中,其近紫外光谱最大值在279 nm处;估计M(r)为160 kD,天然ACE的epsilon 280为1.5 +/- 0.05 × 10(5) (mol/l)-1 × cm-1。6mol /l盐酸胍使ACE变性,在280 nm处产生23%的失色效应,蓝移3.5 nm。在胍溶液中,在288 nm和280 nm处的吸光度测量预测酪氨酸和色氨酸的比值为1,而在283 nm和292 nm处的近紫外光谱二阶导数波段的振幅测量表明,酪氨酸和色氨酸的比值为1.8。在6 mol/l胍中肽链的展开也被远紫外光谱的二阶导数很好地表征,与酶活性完全丧失平行,尽管在SDS-PAGE上判断蛋白质保持完整。我们用原子吸收光谱法重新测定了ACE的锌含量,发现ACE分子中明显含有两个锌原子。
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Spectroscopic studies on angiotensin I-converting enzyme.

We used near and far UV spectrophotometry for the re-evaluation of the molar extinction coefficient at 280 nm (epsilon 280) of pulmonary angiotensin-converting enzyme (ACE), for the determination of its tryptophan and tyrosine contents and to follow-up guanidine denaturation. ACE purity was assessed by both SDS-PAGE and capillary electrophoresis performed in denaturing conditions. The maxima of the near UV spectrum of purified ACE, dissolved in phosphate buffer pH 6.5, was at 279 nm; with an estimated M(r) of 160 kD, epsilon 280 of native ACE was 1.5 +/- 0.05 x 10(5) (mol/l)-1 x cm-1. Denaturation of ACE by 6 mol/l guanidine hydrochloride produced a hypochromic effect of 23% at 280 nm and led to a blue shift of 3.5 nm. In guanidine solution, absorbance measurements at 288 and 280 nm predicted a ratio of 1 between tyrosine and tryptophan, whereas it was 1.8 with the measure of the amplitude of the spectral bands at 283 and 292 nm of the second derivative of the near UV spectrum. Unfolding of the peptide chain in 6 mol/l guanidine was also well characterized by the second derivative of the far UV spectrum, in parallel with the complete loss of enzymatic activity although the protein remained whole as judged on SDS-PAGE. We also re-evaluated ACE zinc content by atomic absorption spectroscopy and demonstrated that ACE molecule obviously contains two zinc atoms.

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