Matthew A. Schaich , Tyler M. Weaver , Vera Roginskaya , Bret D. Freudenthal , Bennett Van Houten
{"title":"纯化蛋白质和核提取物的单分子分析:8- 氧代鸟嘌呤糖基化酶 1 的启示","authors":"Matthew A. Schaich , Tyler M. Weaver , Vera Roginskaya , Bret D. Freudenthal , Bennett Van Houten","doi":"10.1016/j.dnarep.2024.103625","DOIUrl":null,"url":null,"abstract":"<div><p><span>By observing one molecule at a time, single-molecule studies can offer detailed insights about biomolecular processes including on rates, off rates, and diffusivity<span><span> of molecules on strands of DNA. A recent technological advance (Single-molecule Analysis of DNA-binding proteins from Nuclear Extracts, SMADNE) has lowered the barrier to entry for single-molecule studies, and single-molecule dynamics can now be determined directly out of nuclear extracts, providing information in an intermediate environment between purified proteins in isolation and the heterogeneity of a nucleus. To compare and contrast the single-molecule </span>DNA binding dynamics in nuclear extracts versus purified proteins, combined </span></span>optical tweezers<span><span> and fluorescence microscopy<span> experiments were performed with purified GFP-tagged 8-oxoguanine glycosylase 1 (OGG1), purified GFP-OGG1 spiked into nuclear extracts, and nuclear extracts from human cells overexpressing GFP-OGG1. We observed differences in undamaged DNA binding during DNA damage search in each of the three conditions. Purified GFP-OGG1 engaged undamaged DNA for a weighted average lifetime of 5.7 s and 21% of these events underwent DNA diffusion after binding. However, unlike other glycosylases studied by SMADNE, OGG1 does not bind non-damaged DNA efficiently in nuclear extracts. In contrast, GFP-OGG1 binding dynamics on DNA substrates containing oxidative damage were relatively similar in all three conditions, with the weighted average binding lifetimes varying from 2.2 s in nuclear extracts to 7.8 s with purified GFP-OGG1 in isolation. Finally, we compared the purified protein and nuclear extract approaches for a catalytically dead OGG1 variant (GFP-OGG1-K249Q). This variant greatly increased the binding lifetime for oxidative DNA damage, with the weighted average lifetime for GFP-OGG1–249Q in nuclear extracts at 15.4 s vs 10.7 s for the purified protein. SMADNE will provide a new window of observation into the behavior of </span></span>nucleic acid binding proteins only accessible by biophysicists trained in protein purification and protein labeling.</span></p></div>","PeriodicalId":300,"journal":{"name":"DNA Repair","volume":"134 ","pages":"Article 103625"},"PeriodicalIF":3.0000,"publicationDate":"2024-01-17","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":"{\"title\":\"Single-molecule analysis of purified proteins and nuclear extracts: Insights from 8-oxoguanine glycosylase 1\",\"authors\":\"Matthew A. Schaich , Tyler M. Weaver , Vera Roginskaya , Bret D. Freudenthal , Bennett Van Houten\",\"doi\":\"10.1016/j.dnarep.2024.103625\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<div><p><span>By observing one molecule at a time, single-molecule studies can offer detailed insights about biomolecular processes including on rates, off rates, and diffusivity<span><span> of molecules on strands of DNA. A recent technological advance (Single-molecule Analysis of DNA-binding proteins from Nuclear Extracts, SMADNE) has lowered the barrier to entry for single-molecule studies, and single-molecule dynamics can now be determined directly out of nuclear extracts, providing information in an intermediate environment between purified proteins in isolation and the heterogeneity of a nucleus. To compare and contrast the single-molecule </span>DNA binding dynamics in nuclear extracts versus purified proteins, combined </span></span>optical tweezers<span><span> and fluorescence microscopy<span> experiments were performed with purified GFP-tagged 8-oxoguanine glycosylase 1 (OGG1), purified GFP-OGG1 spiked into nuclear extracts, and nuclear extracts from human cells overexpressing GFP-OGG1. We observed differences in undamaged DNA binding during DNA damage search in each of the three conditions. Purified GFP-OGG1 engaged undamaged DNA for a weighted average lifetime of 5.7 s and 21% of these events underwent DNA diffusion after binding. However, unlike other glycosylases studied by SMADNE, OGG1 does not bind non-damaged DNA efficiently in nuclear extracts. In contrast, GFP-OGG1 binding dynamics on DNA substrates containing oxidative damage were relatively similar in all three conditions, with the weighted average binding lifetimes varying from 2.2 s in nuclear extracts to 7.8 s with purified GFP-OGG1 in isolation. Finally, we compared the purified protein and nuclear extract approaches for a catalytically dead OGG1 variant (GFP-OGG1-K249Q). This variant greatly increased the binding lifetime for oxidative DNA damage, with the weighted average lifetime for GFP-OGG1–249Q in nuclear extracts at 15.4 s vs 10.7 s for the purified protein. SMADNE will provide a new window of observation into the behavior of </span></span>nucleic acid binding proteins only accessible by biophysicists trained in protein purification and protein labeling.</span></p></div>\",\"PeriodicalId\":300,\"journal\":{\"name\":\"DNA Repair\",\"volume\":\"134 \",\"pages\":\"Article 103625\"},\"PeriodicalIF\":3.0000,\"publicationDate\":\"2024-01-17\",\"publicationTypes\":\"Journal Article\",\"fieldsOfStudy\":null,\"isOpenAccess\":false,\"openAccessPdf\":\"\",\"citationCount\":\"0\",\"resultStr\":null,\"platform\":\"Semanticscholar\",\"paperid\":null,\"PeriodicalName\":\"DNA Repair\",\"FirstCategoryId\":\"3\",\"ListUrlMain\":\"https://www.sciencedirect.com/science/article/pii/S1568786424000016\",\"RegionNum\":3,\"RegionCategory\":\"生物学\",\"ArticlePicture\":[],\"TitleCN\":null,\"AbstractTextCN\":null,\"PMCID\":null,\"EPubDate\":\"\",\"PubModel\":\"\",\"JCR\":\"Q2\",\"JCRName\":\"GENETICS & HEREDITY\",\"Score\":null,\"Total\":0}","platform":"Semanticscholar","paperid":null,"PeriodicalName":"DNA Repair","FirstCategoryId":"3","ListUrlMain":"https://www.sciencedirect.com/science/article/pii/S1568786424000016","RegionNum":3,"RegionCategory":"生物学","ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q2","JCRName":"GENETICS & HEREDITY","Score":null,"Total":0}
引用次数: 0
摘要
通过一次观察一个分子,单分子研究可以详细了解生物分子过程,包括分子在 DNA 链上的开启率、关闭率和扩散率。最近的一项技术进步(核提取物中 DNA 结合蛋白的单分子分析,SMADNE)降低了单分子研究的门槛,现在可以直接从核提取物中测定单分子动力学,提供介于分离纯化蛋白和细胞核异质性之间的信息。为了比较和对比核提取物与纯化蛋白中的单分子 DNA 结合动力学,我们用纯化的 GFP 标记的 8-氧代鸟嘌呤糖基化酶 1 (OGG1)、添加到核提取物中的纯化 GFP-OGG1 以及过表达 GFP-OGG1 的人体细胞的核提取物进行了光学镊子和荧光显微镜联合实验。我们观察到,在这三种条件下,DNA 损伤搜索过程中未损伤 DNA 的结合情况各不相同。纯化的 GFP-OGG1 与未损伤 DNA 结合的加权平均寿命为 5.7 秒,其中 21% 在结合后发生了 DNA 扩散。然而,与 SMADNE 研究的其他糖基化酶不同,OGG1 在核提取物中不能有效地结合未损坏的 DNA。相比之下,GFP-OGG1 在含有氧化损伤的 DNA 底物上的结合动态在所有三种条件下都相对相似,加权平均结合寿命从核提取物中的 2.2 秒到分离纯化的 GFP-OGG1 的 7.8 秒不等。最后,我们对催化死亡的 OGG1 变体(GFP-OGG1-K249Q)的纯化蛋白和核提取物方法进行了比较。这种变体大大提高了氧化 DNA 损伤的结合寿命,核提取物中 GFP-OGG1-249Q 的加权平均寿命为 15.4 秒,而纯化蛋白为 10.7 秒。SMADNE 将为观察核酸结合蛋白的行为提供一个新的窗口,只有受过蛋白质纯化和蛋白质标记训练的生物物理学家才能观察到。
Single-molecule analysis of purified proteins and nuclear extracts: Insights from 8-oxoguanine glycosylase 1
By observing one molecule at a time, single-molecule studies can offer detailed insights about biomolecular processes including on rates, off rates, and diffusivity of molecules on strands of DNA. A recent technological advance (Single-molecule Analysis of DNA-binding proteins from Nuclear Extracts, SMADNE) has lowered the barrier to entry for single-molecule studies, and single-molecule dynamics can now be determined directly out of nuclear extracts, providing information in an intermediate environment between purified proteins in isolation and the heterogeneity of a nucleus. To compare and contrast the single-molecule DNA binding dynamics in nuclear extracts versus purified proteins, combined optical tweezers and fluorescence microscopy experiments were performed with purified GFP-tagged 8-oxoguanine glycosylase 1 (OGG1), purified GFP-OGG1 spiked into nuclear extracts, and nuclear extracts from human cells overexpressing GFP-OGG1. We observed differences in undamaged DNA binding during DNA damage search in each of the three conditions. Purified GFP-OGG1 engaged undamaged DNA for a weighted average lifetime of 5.7 s and 21% of these events underwent DNA diffusion after binding. However, unlike other glycosylases studied by SMADNE, OGG1 does not bind non-damaged DNA efficiently in nuclear extracts. In contrast, GFP-OGG1 binding dynamics on DNA substrates containing oxidative damage were relatively similar in all three conditions, with the weighted average binding lifetimes varying from 2.2 s in nuclear extracts to 7.8 s with purified GFP-OGG1 in isolation. Finally, we compared the purified protein and nuclear extract approaches for a catalytically dead OGG1 variant (GFP-OGG1-K249Q). This variant greatly increased the binding lifetime for oxidative DNA damage, with the weighted average lifetime for GFP-OGG1–249Q in nuclear extracts at 15.4 s vs 10.7 s for the purified protein. SMADNE will provide a new window of observation into the behavior of nucleic acid binding proteins only accessible by biophysicists trained in protein purification and protein labeling.
期刊介绍:
DNA Repair provides a forum for the comprehensive coverage of DNA repair and cellular responses to DNA damage. The journal publishes original observations on genetic, cellular, biochemical, structural and molecular aspects of DNA repair, mutagenesis, cell cycle regulation, apoptosis and other biological responses in cells exposed to genomic insult, as well as their relationship to human disease.
DNA Repair publishes full-length research articles, brief reports on research, and reviews. The journal welcomes articles describing databases, methods and new technologies supporting research on DNA repair and responses to DNA damage. Letters to the Editor, hot topics and classics in DNA repair, historical reflections, book reviews and meeting reports also will be considered for publication.
求助内容:
应助结果提醒方式:
京公网安备 11010802042870号
