Cooper B F, Sideraki V, Wilson D K, Dominguez D Y, Clark S W, Quiocho F A, Rudolph F B
Department of Biochemistry and Cell Biology, Rice University, Houston, Texas 77251, USA.
Protein Sci. 1997 May;6(5):1031-7. doi: 10.1002/pro.5560060509.
For murine adenosine deaminase, we have determined that a single zinc or cobalt cofactor bound in a high affinity site is required for catalytic function while metal ions bound at an additional site(s) inhibit the enzyme. A catalytically inactive apoenzyme of murine adenosine deaminase was produced by dialysis in the presence of specific zinc chelators in an acidic buffer. This represents the first production of the apoenzyme and demonstrates a rigorous method for removing the occult cofactor. Restoration to the holoenzyme is achieved with stoichiometric amounts of either Zn2+ or Co2+ yielding at least 95% of initial activity. Far UV CD and fluorescence spectra are the same for both the apo- and holoenzyme, providing evidence that removal of the cofactor does not alter secondary or tertiary structure. The substrate binding site remains functional as determined by similar quenching measured by tryptophan fluorescence of apo- or holoenzyme upon mixing with the transition state analog, deoxycoformycin. Excess levels of adenosine or N6- methyladenosine incubated with the apoenzyme prior to the addition of metal prevent restoration, suggesting that the cofactor adds through the substrate binding cleft. The cations Ca2+, Cd2+, Cr2+, Cu+, Cu2+, Mn2+, Fe2+, Fe3+, Pb2+, or Mg2+ did not restore adenosine deaminase activity to the apoenzyme. Mn2+, Cu2+, and Zn2+ were found to be competitive inhibitors of the holoenzyme with respect to substrate and Cd2+ and Co2+ were noncompetitive inhibitors. Weak inhibition (Ki > or = 1000 microM) was noted for Ca2+, Fe2+, and Fe3+.
对于小鼠腺苷脱氨酶,我们已经确定,催化功能需要在高亲和力位点结合单个锌或钴辅因子,而在其他位点结合的金属离子会抑制该酶。在酸性缓冲液中,通过在特定锌螯合剂存在下透析产生了无催化活性的小鼠腺苷脱氨酶脱辅基酶。这是首次产生脱辅基酶,并证明了一种去除隐匿辅因子的严格方法。用化学计量的Zn2+或Co2+可将其恢复为全酶,产生至少95%的初始活性。脱辅基酶和全酶的远紫外圆二色光谱和荧光光谱相同,这表明去除辅因子不会改变二级或三级结构。通过与过渡态类似物脱氧助间型霉素混合后,用脱辅基酶或全酶的色氨酸荧光测量的类似猝灭来确定,底物结合位点仍然具有功能。在添加金属之前,用腺苷或N6-甲基腺苷的过量水平与脱辅基酶孵育可阻止恢复,这表明辅因子是通过底物结合裂隙添加的。阳离子Ca2+、Cd2+、Cr2+、Cu+、Cu2+、Mn2+、Fe2+、Fe3+、Pb2+或Mg2+不能将腺苷脱氨酶活性恢复到脱辅基酶。发现Mn2+、Cu2+和Zn2+是全酶相对于底物的竞争性抑制剂,而Cd2+和Co2+是非竞争性抑制剂。注意到Ca2+、Fe2+和Fe3+有弱抑制作用(Ki≥1000 microM)。