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人碳酸酐酶IV的催化与抑制作用

Catalysis and inhibition of human carbonic anhydrase IV.

作者信息

Baird T T, Waheed A, Okuyama T, Sly W S, Fierke C A

机构信息

Department of Biochemistry, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

Biochemistry. 1997 Mar 4;36(9):2669-78. doi: 10.1021/bi962663s.

DOI:10.1021/bi962663s
PMID:9054574
Abstract

Carbonic anhydrase IV (CA IV) is a membrane-bound form of carbonic anhydrase. We have characterized the catalytic activity and inhibition of recombinant human CA IV. CA IV is a high-activity isozyme in CO2 hydration with a pH-independent kcat value (1.1 x 10(6) s(-1)) comparable to that of CA II (8 x 10(5) s(-1)). Furthermore, CA IV is more active in HCO3- dehydration than is CA II as illustrated by the nearly 3-fold increase in kcat/K(M) to 3 x 10(7) M(-1) s(-1). However, the esterase activity of CA IV is decreased 150-fold compared to CA II. The catalytic mechanisms of CA II and CA IV are nearly identical. Both isozymes show similar dependence on buffer concentration with the rate-limiting step at high buffer concentration being intramolecular proton transfer, although the intramolecular proton transfer for CA IV is 3 times faster than that observed with CA II. Additional positive charges in the active site of CA IV stabilize anions as indicated by a decreased pKa for the Zn-bound water compared to CA II (6.2 vs 6.9), as well as lower inhibition constants for a variety of anions, including halides, sulfate, formate, acetate, and bicarbonate. CA IV is also activated by low concentrations (<20 mM) of chloride, bromide, and phosphate. Activation by phosphate suggests that the phospholipid anchor may be acting both as an extracellular tether and as a protein activator. Finally, the affinity of CA IV for sulfonamide inhibitors is decreased up to 65-fold compared to CA II as demonstrated by fluorescence titration. The increased bicarbonate activity and altered pH profile are consistent with the proposed physiological role of CA IV in renal bicarbonate reabsorption.

摘要

碳酸酐酶IV(CA IV)是碳酸酐酶的一种膜结合形式。我们已经对重组人CA IV的催化活性和抑制作用进行了表征。CA IV是CO2水合作用中的一种高活性同工酶,其pH无关的催化常数(kcat)值(1.1×10^6 s^(-1))与CA II(8×10^5 s^(-1))相当。此外,CA IV在HCO3-脱水方面比CA II更具活性,kcat/K(M)增加近3倍,达到3×10^7 M^(-1) s^(-1)。然而,与CA II相比,CA IV的酯酶活性降低了150倍。CA II和CA IV的催化机制几乎相同。两种同工酶对缓冲液浓度的依赖性相似,在高缓冲液浓度下的限速步骤是分子内质子转移,尽管CA IV的分子内质子转移速度比CA II快3倍。CA IV活性位点中的额外正电荷使阴离子稳定,这表现为与CA II相比,锌结合水的pKa降低(6.2对6.9),以及对包括卤化物、硫酸盐、甲酸盐、乙酸盐和碳酸氢盐在内的多种阴离子的抑制常数更低。CA IV还可被低浓度(<20 mM)的氯离子、溴离子和磷酸盐激活。磷酸盐的激活表明磷脂锚可能既作为细胞外栓系又作为蛋白质激活剂。最后,通过荧光滴定证明,与CA II相比,CA IV对磺胺类抑制剂的亲和力降低了65倍。碳酸氢盐活性的增加和pH曲线的改变与CA IV在肾脏碳酸氢盐重吸收中所提出的生理作用一致。

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