Eisenstein E, Yu H D, Fisher K E, Iacuzio D A, Ducote K R, Schwarz F P
Center for Advanced Research in Biotechnology, University of Maryland Biotechnology Institute, Rockville 20850, USA.
Biochemistry. 1995 Jul 25;34(29):9403-12. doi: 10.1021/bi00029a016.
The linkage between substrate and regulatory effector binding to separate sites on allosteric enzymes results in shifts in their sigmoidal kinetics to regulate metabolism. Control of branched chain amino acid biosynthesis in Escherichia coli occurs in part through shifts in the sigmoidal dependence of alpha-ketobutyrate production promoted by isoleucine and valine binding to biosynthetic threonine deaminase. The structural similarity of threonine, valine, and isoleucine have given rise to suggestions that there may be competition among different ligands for the same sites on this tetrameric enzyme, resulting in a complex pattern of regulation. In an effort to provide a coherent interpretation of the cooperative association of ligands to the active sites and to the effector sites of threonine deaminase, binding studies using single amino acid variants were undertaken. A previously-isolated, feedback-resistant mutant identified in Salmonella typhimurium, ilvA219, has been cloned and sequenced. The phenotype is attributable to a single amino acid substitution in the regulatory domain of the enzyme in which leucine at position 447 is substituted with phenylalanine. The mutant exhibits hyperbolic saturation curves in both ligand binding and steady-state kinetics. These results, in addition to calorimetric and spectroscopic measurements of isoleucine and valine binding, indicate that the low affinity (T) state is destabilized in the mutant and that it exists predominantly in the high affinity (R) conformation in the absence of ligands, providing an explanation for its resistance to isoleucine. Chemical and spectroscopic analyses of another mutant, in which alanine has replaced an essential lysine at position 62 that forms a Schiff base with pyridoxal phosphate, indicate that the cofactor is complexed to exogenous threonine and is therefore unable to bind additional amino acids at the active sites. Isoleucine and valine binding to this inactive, active site-saturated enzyme revealed that it too was stabilized in the R state, yielding binding constants in excellent agreement with the leucine to phenylalanine mutant. The lysine to alanine mutant was further utilized to demonstrate that both threonine and 2-aminobutyrate bind with stronger affinity to the regulatory sites than to the active sites. A direct consequence of these results is that substrates and analogs have a synergistic effect on the allosteric transition since, in effect, they act as both homotropic and heterotropic effectors.(ABSTRACT TRUNCATED AT 250 WORDS)
底物与调节效应物结合到别构酶的不同位点之间的联系,导致其S形动力学发生变化,从而调节新陈代谢。大肠杆菌中支链氨基酸生物合成的控制部分是通过异亮氨酸和缬氨酸与生物合成苏氨酸脱氨酶结合,促使α-酮丁酸产生的S形依赖性发生变化来实现的。苏氨酸、缬氨酸和异亮氨酸的结构相似性,引发了一种观点,即不同配体可能会竞争这种四聚体酶上的相同位点,从而产生复杂的调节模式。为了对配体与苏氨酸脱氨酶活性位点和效应物位点的协同结合提供连贯的解释,开展了使用单个氨基酸变体的结合研究。在鼠伤寒沙门氏菌中先前分离出的一种反馈抗性突变体ilvA219,已被克隆和测序。该表型归因于该酶调节结构域中的单个氨基酸取代,其中第447位的亮氨酸被苯丙氨酸取代。该突变体在配体结合和稳态动力学方面均表现出双曲线饱和曲线。这些结果,除了对异亮氨酸和缬氨酸结合的量热法和光谱法测量外,还表明该突变体中低亲和力(T)状态不稳定,并且在没有配体的情况下它主要以高亲和力(R)构象存在,这为其对异亮氨酸的抗性提供了解释。对另一个突变体的化学和光谱分析表明,在该突变体中丙氨酸取代了与磷酸吡哆醛形成席夫碱的第62位的必需赖氨酸,辅因子与外源苏氨酸络合,因此无法在活性位点结合额外的氨基酸。异亮氨酸和缬氨酸与这种无活性的、活性位点饱和的酶结合表明,它也稳定在R状态,产生的结合常数与亮氨酸到苯丙氨酸突变体的结果非常一致。赖氨酸到丙氨酸突变体进一步被用于证明苏氨酸和2-氨基丁酸与调节位点的结合亲和力都强于与活性位点的结合亲和力。这些结果的一个直接后果是,底物和类似物对别构转变具有协同作用,因为实际上它们既作为同促效应物又作为异促效应物。(摘要截断于250字)
