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通过表面等离子体共振测量确定的HMG蛋白1和2对DNA亲和力的差异。

Difference in affinity for DNA between HMG proteins 1 and 2 determined by surface plasmon resonance measurements.

作者信息

Yamamoto A, Ando Y, Yoshioka K, Saito K, Tanabe T, Shirakawa H, Yoshida M

机构信息

Department of Biological Science and Technology, Science University of Tokyo, Chiba.

出版信息

J Biochem. 1997 Sep;122(3):586-94. doi: 10.1093/oxfordjournals.jbchem.a021793.

Abstract

High mobility group (HMG) proteins 1 and 2 contain two similar but non-identical repeats of DNA-binding domains and an acidic C-terminal. The proposed functions of HMG proteins 1 and 2 imply a probable difference in their DNA-binding abilities. The primary studies by gel retardation assay showed that HMG2 has higher affinity than HMG1 for supercoiled and linear DNA. The DNA-binding of HMG2 appeared strong enough to allow exchange with HMG1 molecule already bound to DNA, while the DNA-binding region of HMG1 showed higher affinity than that of HMG2. In order to compare more quantitatively the affinities, surface plasmon resonance (SPR) measurements using a BIAcore instrument were conducted. The kinetic data indicated that the Kd for the complex of HMG2 with DNA is smaller than that of HMG1, in contrast to the situation for the DNA-binding region of these proteins. The sequence between the second DNA-binding domain and the acidic C-terminal of HMG proteins is required for tight DNA-binding. Also, the acidic C-terminal strongly modulates the DNA-binding ability of each protein. The usefulness of SPR measurement for quantitative analysis of affinity and regions involved in DNA-binding under conditions nearly identical to those in solution is discussed.

摘要

高迁移率族(HMG)蛋白1和2包含两个相似但不完全相同的DNA结合结构域重复序列以及一个酸性C末端。HMG蛋白1和2的推测功能表明它们在DNA结合能力上可能存在差异。凝胶阻滞分析的初步研究表明,HMG2对超螺旋和线性DNA的亲和力高于HMG1。HMG2与DNA的结合似乎足够强,能够与已结合到DNA上的HMG1分子进行交换,而HMG1的DNA结合区域显示出比HMG2更高的亲和力。为了更定量地比较亲和力,使用BIAcore仪器进行了表面等离子体共振(SPR)测量。动力学数据表明,与这些蛋白质的DNA结合区域的情况相反,HMG2与DNA复合物的解离常数(Kd)小于HMG1。紧密结合DNA需要HMG蛋白第二个DNA结合结构域与酸性C末端之间的序列。此外,酸性C末端强烈调节每种蛋白质的DNA结合能力。讨论了SPR测量在几乎与溶液条件相同的情况下对亲和力和参与DNA结合的区域进行定量分析的实用性。

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