Kozlov A G, Lohman T M
Department of Biochemistry and Molecular Biophysics, Washington University School of Medicine, St. Louis, Missouri.
Proteins. 2000;Suppl 4:8-22. doi: 10.1002/1097-0134(2000)41:4+<8::aid-prot20>3.0.co;2-h.
Many macromolecular interactions, including protein-nucleic acid interactions, are accompanied by a substantial negative heat capacity change, the molecular origins of which have generated substantial interest. We have shown previously that temperature-dependent unstacking of the bases within oligo(dA) upon binding to the Escherichia coli SSB tetramer dominates the binding enthalpy, DeltaH(obs), and accounts for as much as a half of the observed heat capacity change, DeltaC(p). However, there is still a substantial DeltaC(p) associated with SSB binding to ssDNA, such as oligo(dT), that does not undergo substantial base stacking. In an attempt to determine the origins of this heat capacity change, we have examined by isothermal titration calorimetry (ITC) the equilibrium binding of dT(pT)(34) to SSB over a broad pH range (pH 5. 0-10.0) at 0.02 M, 0.2 M NaCl and 1 M NaCl (25 degrees C), and as a function of temperature at pH 8.1. A net protonation of the SSB protein occurs upon dT(pT)(34) binding over this entire pH range, with contributions from at least three sets of protonation sites (pK(a1) = 5.9-6.6, pK(a2) = 8.2-8.4, and pK(a3) = 10.2-10.3) and these protonation equilibria contribute substantially to the observed DeltaH and DeltaC(p) for the SSB-dT(pT)(34) interaction. The contribution of this coupled protonation ( approximately -260 to -320 cal mol(-1) K(-1)) accounts for as much as half of the total DeltaC(p). The values of the "intrinsic" DeltaC(p,0) range from -210 +/- 33 cal mol(-1) degrees K(-1) to -237 +/- 36 cal mol(-1)K(-1), independent of [NaCl]. These results indicate that the coupling of a temperature-dependent protonation equilibria to a macromolecular interaction can result in a large negative DeltaC(p), and this finding needs to be considered in interpretations of the molecular origins of heat capacity changes associated with ligand-macromolecular interactions, as well as protein folding.
许多大分子相互作用,包括蛋白质 - 核酸相互作用,都伴随着显著的负热容变化,其分子起源引发了广泛关注。我们之前已经表明,寡聚(dA)与大肠杆菌单链结合蛋白(SSB)四聚体结合时,碱基的温度依赖性解堆叠主导了结合焓ΔH(obs),并占观察到的热容变化ΔC(p)的一半之多。然而,SSB与单链DNA(如寡聚(dT))结合时,仍然存在显著的ΔC(p),而寡聚(dT)不会发生大量碱基堆叠。为了确定这种热容变化的起源,我们通过等温滴定量热法(ITC)研究了dT(pT)(34)在0.02 M、0.2 M NaCl和1 M NaCl(25℃)的广泛pH范围(pH 5.0 - 10.0)下与SSB的平衡结合,并研究了在pH 8.1时作为温度函数的结合情况。在整个pH范围内,dT(pT)(34)结合时SSB蛋白发生净质子化,至少有三组质子化位点(pK(a1) = 5.9 - 6.6,pK(a2) = 8.2 - 8.4,pK(a3) = 10.2 - 10.3)对此有贡献,并且这些质子化平衡对观察到的SSB - dT(pT)(34)相互作用的ΔH和ΔC(p)有很大贡献。这种耦合质子化的贡献(约 -260至 -320 cal mol(-1) K(-1))占总ΔC(p)的一半之多。“内在”ΔC(p,0)的值范围为 -210 ± 33 cal mol(-1) K(-1)至 -237 ± 36 cal mol(-1) K(-1),与[NaCl]无关。这些结果表明,温度依赖性质子化平衡与大分子相互作用的耦合可导致很大的负ΔC(p),在解释与配体 - 大分子相互作用以及蛋白质折叠相关的热容变化的分子起源时需要考虑这一发现。
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