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木质素前体的酶促合成。对大豆细胞悬浮培养物中肉桂醇脱氢酶的进一步研究。

Enzymic synthesis of lignin precursors. Further studies on cinnamyl-alcohol dehydrogenase from soybean-cell-suspension cultures.

作者信息

Wyrambik D, Grisebach H

出版信息

Eur J Biochem. 1979 Jul;97(2):503-9. doi: 10.1111/j.1432-1033.1979.tb13138.x.

Abstract

Isoenzyme 2 of cinnamyl-alcohol dehydrogenase from soybean suspension cultures was purified about 3800-fold to apparent homogeneity by an improved purification procedure involving biospecific elution of the enzyme from a NADP+-agarose column. On sodium dodecylsulfate gels the dehydrogenase showed only one protein band with Mr 40 000 +/- 500. The enzyme is strongly inhibited by thiol reagents. Various metal chelators as well as the nonchelating 7,8-benzoquinoline also inhibited enzyme activity. Inhibition by 10 mM 1,10-phenanthroline could be partially reversed by addition of Zn2+. 1,10-Phenanthroline and 7,8-benzoquinoline are non-competitive inhibitors with respect to NADP+. The presence of zinc in the dehydrogenase was proved by atomic absorption spectroscopy and by specific incorporation of 65Zn into the enzyme. In steady-state kinetics inhibition patterns were obtained which are consistent with an ordered bi-bi mechanism in which NADP(H) is the first substrate to bind and the last product released. The cinnamyl-alcohol dehydrogenase belongs to the A-specific dehydrogenases and removes the pro-R hydrogen from coniferyl alcohol. The enzyme shows many similarities with alcohol dehydrogenases from horse and rat liver and from yeast.

摘要

通过一种改进的纯化方法,利用从NADP⁺-琼脂糖柱上对该酶进行生物特异性洗脱,将大豆悬浮培养物中的肉桂醇脱氢酶同工酶2纯化了约3800倍,达到表观均一性。在十二烷基硫酸钠凝胶上,该脱氢酶仅显示一条分子量为40000±500的蛋白带。该酶受到硫醇试剂的强烈抑制。各种金属螯合剂以及非螯合的7,8-苯并喹啉也抑制酶活性。10 mM 1,10-菲咯啉的抑制作用可通过添加Zn²⁺部分逆转。1,10-菲咯啉和7,8-苯并喹啉对NADP⁺而言是非竞争性抑制剂。通过原子吸收光谱法以及将⁶⁵Zn特异性掺入该酶中,证明了脱氢酶中锌的存在。在稳态动力学中获得的抑制模式与有序的双底物双产物机制一致,其中NADP(H)是第一个结合的底物,也是最后一个释放的产物。肉桂醇脱氢酶属于A特异性脱氢酶,从松柏醇中去除前手性R氢。该酶与马、大鼠肝脏以及酵母中的醇脱氢酶有许多相似之处。

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