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肽与抗原加工相关转运体(TAP)结合的热力学

Thermodynamics of peptide binding to the transporter associated with antigen processing (TAP).

作者信息

Neumann Lars, Abele Rupert, Tampé Robert

机构信息

Institute of Biochemistry, Biocenter, Goethe-University Frankfurt, Marie-Curie-Str. 9, D-60439, Frankfurt, Germany.

出版信息

J Mol Biol. 2002 Dec 13;324(5):965-73. doi: 10.1016/s0022-2836(02)01148-8.

DOI:10.1016/s0022-2836(02)01148-8
PMID:12470952
Abstract

The ATP-binding cassette (ABC) transporter TAP plays an essential role in antigen processing and immune response to infected or malignant cells. TAP translocates proteasomal degradation products from the cytosol into the endoplasmic reticulum, where MHC class I molecules are loaded with these peptides. Kinetically stable peptide-MHC complexes are transported to the cell surface for inspection by cytotoxic T lymphocytes. The transport cycle of TAP is initiated by peptide binding, which is responsible for peptide selection and for stimulation of ATP-hydrolysis and subsequent translocation. Here we have analysed the driving forces for the formation of the peptide-TAP complex by kinetic and thermodynamic methods. First, the apparent peptide association and dissociation rates were determined at various temperatures. Strikingly, very high activation energies for apparent association (E(a)(ass)=106 kJmol(-1)) and dissociation (E(a)(diss)=80 kJmol(-1)) of the peptide-TAP complex were found. Next, the temperature-dependence of the peptide affinity constants was investigated by equilibrium-binding assays. Along with calculations of free enthalpy deltaG, enthalpy deltaH and entropy deltaS, a large positive change in heat capacity was resolved (deltaC degrees =23 kJmol(-1)K(-1)), indicating a fundamental structural reorganization of the TAP complex upon peptide binding. The inspection of the conformational entropy reveals that approximately one-fourth of all TAP residues is rearranged. These thermodynamic studies indicate that at physiological temperature, peptide binding is endothermic and driven by entropy.

摘要

ATP结合盒(ABC)转运蛋白TAP在抗原加工以及对受感染或恶性细胞的免疫反应中起着至关重要的作用。TAP将蛋白酶体降解产物从细胞质转运到内质网,在内质网中MHC I类分子装载这些肽段。动力学稳定的肽-MHC复合物被转运到细胞表面以供细胞毒性T淋巴细胞检查。TAP的转运循环由肽结合启动,肽结合负责肽的选择以及刺激ATP水解和随后的转运。在此,我们通过动力学和热力学方法分析了肽-TAP复合物形成的驱动力。首先,在不同温度下测定了肽的表观缔合和解离速率。令人惊讶的是,发现肽-TAP复合物的表观缔合(E(a)(ass)=106 kJmol(-1))和解离(E(a)(diss)=80 kJmol(-1))具有非常高的活化能。接下来,通过平衡结合试验研究了肽亲和常数的温度依赖性。连同自由焓deltaG、焓deltaH和熵deltaS的计算,解析出热容有很大的正变化(deltaC degrees =23 kJmol(-1)K(-1)),表明肽结合后TAP复合物发生了基本的结构重组。对构象熵的检查表明,所有TAP残基中约四分之一发生了重排。这些热力学研究表明,在生理温度下,肽结合是吸热的且由熵驱动。

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