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Individual breathing reactions measured in hemoglobin by hydrogen exchange methods.

机译:通过氢交换方法在血红蛋白中测量的个体呼吸反应。

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摘要

Protein hydrogen exchange is generally believed to register some aspects of internal protein dynamics, but the kind of motion at work is not clear. Experiments are being done to identify the determinants of protein hydrogen exchange and to distinguish between local unfolding and accessibility-penetration mechanisms. Results with small molecules, polynucleotides, and proteins demonstrate that solvent accessibility is by no means sufficient for fast exchange. H-exchange slowing is quite generally connected with intramolecular H-bonding, and the exchange process depends pivotally on transient H-bond cleavage. At least in alpha-helical structures, the cooperative aspect of H-bond cleavage must be expressed in local unfolding reactions. Results obtained by use of a difference hydrogen exchange method appear to provide a direct measurement of transient, cooperative, local unfolding reactions in hemoglobin. The reality of these supposed coherent breathing units is being tested by using the difference H-exchange approach to tritium label the units one at a time and then attempting to locate the tritium by fragmenting the protein, separating the fragments, and testing them for label. Early results demonstrate the feasibility of this approach.
机译:人们普遍认为蛋白质氢交换会记录内部蛋白质动力学的某些方面,但工作中的运动类型尚不清楚。正在进行实验以确定蛋白质氢交换的决定因素,并区分局部展开和可及性-穿透机制。小分子,多核苷酸和蛋白质的结果表明,溶剂的可及性不足以快速交换。 H交换减慢通常与分子内H键有关,而交换过程主要取决于瞬时H键裂解。至少在α-螺旋结构中,氢键裂解的协同作用必须在局部展开反应中表达。通过使用差异氢交换方法获得的结果似乎可以直接测量血红蛋白中的瞬时,协同,局部解折叠反应。通过使用差异H交换方法一次对is单元进行标记,然后通过片段化蛋白质,分离片段并测试其标记性来尝试定位locate,从而测试了这些假设的连贯呼吸单元的真实性。早期结果证明了这种方法的可行性。

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