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Mechanism of DNA flexibility enhancement by HMGB proteins

机译:HMGB蛋白增强DNA柔韧性的机制

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摘要

The mechanism by which sequence non-specific DNA-binding proteins enhance DNA flexibility is studied by examining complexes of double-stranded DNA with the high mobility group type B proteins HMGB2 (Box A) and HMGB1 (Box A+B) using atomic force microscopy. DNA end-to-end distances and local DNA bend angle distributions are analyzed for protein complexes deposited on a mica surface. For HMGB2 (Box A) binding we find a mean induced DNA bend angle of 78°, with a standard error of 1.3° and a SD of 23°, while HMGB1 (Box A+B) binding gives a mean bend angle of 67°, with a standard error of 1.3° and a SD of 21°. These results are consistent with analysis of the observed global persistence length changes derived from end-to-end distance measurements, and with results of DNA-stretching experiments. The moderately broad distributions of bend angles induced by both proteins are inconsistent with either a static kink model, or a purely flexible hinge model for DNA distortion by protein binding. Therefore, the mechanism by which HMGB proteins enhance the flexibility of DNA must differ from that of the Escherichia coli HU protein, which in previous studies showed a flat angle distribution consistent with a flexible hinge model.
机译:通过使用原子力显微镜检查双链DNA与高迁移率B型蛋白HMGB2(Box A)和HMGB1(Box A + B)的复合物,研究了序列非特异性DNA结合蛋白增强DNA柔性的机制。 。分析DNA的端到端距离和局部DNA弯曲角度分布,以测定云母表面沉积的蛋白质复合物。对于HMGB2(框A)结合,我们发现平均诱导DNA弯曲角为78°,标准误差为1.3°,SD为23°,而HMGB1(框A + B)结合给出的平均弯曲角为67° ,标准误差为1.3°,SD为21°。这些结果与观察到的从端到端距离测量得出的整体持久性长度变化的分析以及DNA拉伸实验的结果一致。两种蛋白质引起的弯曲角度的适度宽广分布与静态扭结模型或用于蛋白质结合引起的DNA畸变的纯柔性铰链模型均不一致。因此,HMGB蛋白增强DNA柔韧性的机制必须与大肠杆菌HU蛋白的机制不同,后者在以前的研究中显示出与柔性铰链模型一致的平坦角度分布。

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