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通过分析亲和色谱法表征辅酶、调节核苷酸和汽巴克隆蓝与酶的核苷酸结合结构域的特异性相互作用。

Characterization of specific interactions of coenzymes, regulatory nucleotides and cibacron blue with nucleotide binding domains of enzymes by analytical affinity chromatography.

作者信息

Thresher W C, Swaisgood H E

机构信息

Department of Food Science and Biochemistry, North Carolina State University, Raleigh 27695-7624.

出版信息

J Mol Recognit. 1990 Oct-Dec;3(5-6):220-8. doi: 10.1002/jmr.300030509.

DOI:10.1002/jmr.300030509
PMID:2096889
Abstract

The dissociation constant for the complex of rhodanese and Cibacron Blue, determined by analytical affinity chromatography using rhodanese immobilized on controlled-pore glass (CPG) beads (200 nm pore diameter) and aminohexyl-Cibacron Blue, was 44 microM which agreed well with the kinetic inhibition constant, suggesting that the dye binds at or near the active site of this enzyme. Formation of a binary complex of the dye and lactate dehydrogenase (LDH) was also characterized by direct chromatography of LDH on CPG/immobilized Cibacron Blue (KD = 0.29 microM). The binary complex formed between LDH and NADH was characterized by analytical affinity chromatography using both CPG/immobilized LDH and immobilized Cibacron Blue. Since the dye competes with NADH in binding to the active site of LDH, competitive elution chromatography using the immobilized dye allows determination of the dissociation constant of the soluble LDH.NADH complex. Agreement between the dissociation constants determined by direct chromatography of NADH on immobilized LDH (KD = 1.4 microM) and that determined for the soluble complex (KD = 2.4 microM) indicates that immobilization of LDH did not affect the interaction. Formation of various binary, ternary and quaternary complexes of bovine liver glutamate dehydrogenase (GDH) with glutamate, NADPH, NADH, and ADP was also investigated using immobilized GDH. This approach allows characterization of the enzyme/ligand interactions without the complicating effect of enzyme self-association. The affinity for NADPH is considerably greater in the ternary complex (including glutamate) as compared to the binary complex (0.38 microM vs 22 microM); however, occupancy of the regulatory site by ADP greatly reduces the affinity in both complexes (6.4 microM and 43 microM, respectively).(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过使用固定在可控孔径玻璃(CPG)珠(孔径200纳米)上的硫氰酸酶和氨基己基-汽巴克隆蓝进行分析亲和色谱法,测定了硫氰酸酶与汽巴克隆蓝复合物的解离常数为44微摩尔,这与动力学抑制常数非常吻合,表明该染料在该酶的活性位点或其附近结合。染料与乳酸脱氢酶(LDH)二元复合物的形成也通过LDH在CPG/固定化汽巴克隆蓝上的直接色谱法进行了表征(KD = 0.29微摩尔)。LDH与NADH之间形成的二元复合物通过使用CPG/固定化LDH和固定化汽巴克隆蓝的分析亲和色谱法进行了表征。由于该染料在与LDH的活性位点结合时与NADH竞争,使用固定化染料的竞争洗脱色谱法可测定可溶性LDH·NADH复合物的解离常数。通过NADH在固定化LDH上的直接色谱法测定的解离常数(KD = 1.4微摩尔)与可溶性复合物的解离常数(KD = 2.4微摩尔)之间的一致性表明,LDH的固定化并未影响其相互作用。还使用固定化的谷氨酸脱氢酶(GDH)研究了牛肝谷氨酸脱氢酶(GDH)与谷氨酸、NADPH、NADH和ADP形成的各种二元、三元和四元复合物。这种方法能够在没有酶自缔合复杂影响的情况下表征酶/配体相互作用。与二元复合物相比,三元复合物(包括谷氨酸)中对NADPH的亲和力要大得多(分别为0.38微摩尔和22微摩尔);然而,ADP占据调节位点会大大降低两种复合物中的亲和力(分别为6.4微摩尔和43微摩尔)。(摘要截取自250字)

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