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Single Qdot-labeled glycosylase molecules use a wedge amino acid to probe for lesions while scanning along DNA

机译:单个Qdot标记的糖基化酶分子使用楔形氨基酸在沿着DNA扫描时探测病变

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摘要

Within the base excision repair (BER) pathway, the DNA N-glycosylases are responsible for locating and removing the majority of oxidative base damages. Endonuclease III (Nth), formamidopyrimidine DNA glycosylase (Fpg) and endonuclease VIII (Nei) are members of two glycosylase families: the helix–hairpin–helix (HhH) superfamily and the Fpg/Nei family. The search mechanisms employed by these two families of glycosylases were examined using a single molecule assay to image quantum dot (Qdot)-labeled glycosylases interacting with YOYO-1 stained λ-DNA molecules suspended between 5 µm silica beads. The HhH and Fpg/Nei families were found to have a similar diffusive search mechanism described as a continuum of motion, in keeping with rotational diffusion along the DNA molecule ranging from slow, sub-diffusive to faster, unrestricted diffusion. The search mechanism for an Fpg variant, F111A, lacking a phenylalanine wedge residue no longer displayed slow, sub-diffusive motion compared to wild type, suggesting that Fpg base interrogation may be accomplished by Phe111 insertion.
机译:在碱基切除修复(BER)途径中,DNA N-糖基化酶负责定位和消除大部分氧化性碱基损伤。核酸内切酶III(Nth),甲酰胺基嘧啶DNA糖基化酶(Fpg)和核酸内切酶VIII(Nei)是两个糖基化酶家族的成员:螺旋-发夹-螺旋(HhH)超家族和Fpg / Nei家族。使用单分子测定法检查了这两个糖基化酶家族的搜索机制,以成像量子点(Qdot)标记的糖基化酶与悬浮在5μm二氧化硅微珠之间的YOYO-1染色λ-DNA分子相互作用。发现HhH和Fpg / Nei家族具有类似的扩散搜索机制,称为运动连续体,与沿着DNA分子的旋转扩散(从缓慢,亚扩散到更快,不受限制的扩散)保持一致。与野生型相比,缺少苯丙氨酸楔残基的Fpg变体F111A的搜索机制不再显示缓慢的亚扩散运动,这表明可以通过Phe 111 插入来完成Fpg碱基的询问。

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