Department of Chemistry & Biochemistry, California Polytechnic State University, San Luis Obispo, CA, USA.
Department of Chemistry & Biochemistry, California Polytechnic State University, San Luis Obispo, CA, USA.
Biophys Chem. 2020 Sep;264:106410. doi: 10.1016/j.bpc.2020.106410. Epub 2020 Jun 12.
Osmolytes are naturally occurring organic compounds that protect cellular proteins and other macromolecules against various forms of stress including temperature extremes. While biological studies have correlated the accumulation of certain classes of osmolytes with specific forms of stress, including thermal stress, it remains unclear whether or not these observations reflect an intrinsic chemical class hierarchy amongst the osmolytes with respect to effects on protein stability. In addition, very little is known in regards to the molecular elements of the osmolytes themselves that are essential for their functions. In this study, we use differential scanning fluorimetry to quantify the thermal stabilizing effects of members from each of the three main classes of protecting osmolytes on two model protein systems, C-reactive protein and tumor necrosis factor alpha. Our data reveals the absence of a strict chemical class hierarchy amongst the osmolytes with respect to protein thermal stabilization, and indicates differential responses of these proteins to certain osmolytes. In the second part of this investigation we dissected the molecular elements of amino acid osmolytes required for thermal stabilization of myoglobin and C-reactive protein. We show that the complete amino acid zwitterion is required for thermal stabilization of myoglobin, whereas removal of the osmolyte amino group does not diminish stabilizing effects on C-reactive protein. These disparate responses of proteins to osmolytes and other small molecules are consistent with previous observations that osmolyte effects on protein stability are protein-specific. Moreover, the data reported in this study support the view that osmolyte effects cannot be fully explained by considering only the solvent accessibility of the polypeptide backbone in the native and denatured states, and corroborate the need for more complex models that take into account the entire protein fabric.
渗透物是天然存在的有机化合物,可保护细胞蛋白和其他大分子免受各种形式的压力,包括极端温度。虽然生物研究已经将某些类别的渗透物的积累与特定形式的压力(包括热压力)相关联,但尚不清楚这些观察结果是否反映了渗透物在影响蛋白质稳定性方面的固有化学分类层次。此外,对于渗透物本身对于其功能至关重要的分子元素,人们知之甚少。在这项研究中,我们使用差示扫描荧光法来量化三种主要保护渗透物类别中的每个成员对两种模型蛋白系统(C-反应蛋白和肿瘤坏死因子 alpha)的热稳定作用。我们的数据表明,在蛋白质热稳定方面,渗透物之间没有严格的化学分类层次,并且表明这些蛋白质对某些渗透物的反应不同。在这项研究的第二部分中,我们剖析了氨基酸渗透物稳定肌红蛋白和 C-反应蛋白所需的分子元素。我们表明,完整的氨基酸两性离子是肌红蛋白热稳定所必需的,而去除渗透物的氨基则不会降低对 C-反应蛋白的稳定作用。这些蛋白质对渗透物和其他小分子的不同反应与以前的观察结果一致,即渗透物对蛋白质稳定性的影响是蛋白质特异性的。此外,本研究报告的数据支持这样一种观点,即仅考虑天然状态和变性状态下多肽骨架的溶剂可及性,渗透物的影响不能得到充分解释,并证实需要更复杂的模型来考虑整个蛋白质结构。
Zotero 插件