Archaeal Chromatin Proteins Cren7 and Sul7d Compact DNA by Bending and Bridging

Archaeal Chromatin Proteins Cren7 and Sul7d Compact DNA by Bending and Bridging

A long-standing question is how chromosomal DNA is packaged in Crenarchaeota, a major group of archaea, which synthesize large amounts of unique small DNA-binding proteins but in general contain no archaeal histones. In the present work, we tested our hypothesis that the two well-studied crenarchaea...

Full description

Bibliographic Details
Main Authors: Zhenfeng Zhang, Zhengyan Zhan, Bing Wang, Yuanyuan Chen, Xiuqiang Chen, Cuihong Wan, Yu Fu, Li Huang
Format: Article
Language:English
Published: American Society for Microbiology 2020-06-01
Series:mBio
Subjects:
archaea
atomic force microscopy
chromatin protein
single-molecule technology
sulfolobus
Online Access:https://doi.org/10.1128/mBio.00804-20
id doaj-12631e7841c045db8fc733fa68b1886b
record_format Article
spelling doaj-12631e7841c045db8fc733fa68b1886b2021-07-02T12:47:18ZengAmerican Society for MicrobiologymBio2150-75112020-06-01113e00804-2010.1128/mBio.00804-20Archaeal Chromatin Proteins Cren7 and Sul7d Compact DNA by Bending and BridgingZhenfeng ZhangZhengyan ZhanBing WangYuanyuan ChenXiuqiang ChenCuihong WanYu FuLi HuangA long-standing question is how chromosomal DNA is packaged in Crenarchaeota, a major group of archaea, which synthesize large amounts of unique small DNA-binding proteins but in general contain no archaeal histones. In the present work, we tested our hypothesis that the two well-studied crenarchaeal chromatin proteins Cren7 and Sul7d compact DNA by both DNA bending and bridging. We show that the two proteins are capable of compacting DNA, albeit with different efficiencies and in different manners, at the single molecule level. We demonstrate for the first time that the two proteins, which have long been regarded as DNA binders and benders, are able to mediate DNA bridging, and this previously unknown property of the proteins allows DNA to be packaged into highly condensed structures. Therefore, our results provide significant insights into the mechanism and kinetics of chromosomal DNA organization in Crenarchaeota.Archaeal chromatin proteins Cren7 and Sul7d from Sulfolobus are DNA benders. To better understand their architectural roles in chromosomal DNA organization, we analyzed DNA compaction by Cren7 and Sis7d, a Sul7d family member, from Sulfolobus islandicus at the single-molecule (SM) level by total single-molecule internal reflection fluorescence microscopy (SM-TIRFM) and atomic force microscopy (AFM). We show that both Cren7 and Sis7d were able to compact singly tethered λ DNA into a highly condensed structure in a three-step process and that Cren7 was over an order of magnitude more efficient than Sis7d in DNA compaction. The two proteins were similar in DNA bending kinetics but different in DNA condensation patterns. At saturating concentrations, Sis7d formed randomly distributed clusters whereas Cren7 generated a single and highly condensed core on plasmid DNA. This observation is consistent with the greater ability of Cren7 than of Sis7d to bridge DNA. Our results offer significant insights into the mechanism and kinetics of chromosomal DNA organization in Crenarchaea.https://doi.org/10.1128/mBio.00804-20archaeaatomic force microscopychromatin proteinsingle-molecule technologysulfolobus
collection DOAJ
language English
format Article
sources DOAJ
author Zhenfeng Zhang
Zhengyan Zhan
Bing Wang
Yuanyuan Chen
Xiuqiang Chen
Cuihong Wan
Yu Fu
Li Huang
spellingShingle Zhenfeng Zhang
Zhengyan Zhan
Bing Wang
Yuanyuan Chen
Xiuqiang Chen
Cuihong Wan
Yu Fu
Li Huang
Archaeal Chromatin Proteins Cren7 and Sul7d Compact DNA by Bending and Bridging
mBio
archaea
atomic force microscopy
chromatin protein
single-molecule technology
sulfolobus
author_facet Zhenfeng Zhang
Zhengyan Zhan
Bing Wang
Yuanyuan Chen
Xiuqiang Chen
Cuihong Wan
Yu Fu
Li Huang
author_sort Zhenfeng Zhang
title Archaeal Chromatin Proteins Cren7 and Sul7d Compact DNA by Bending and Bridging
title_short Archaeal Chromatin Proteins Cren7 and Sul7d Compact DNA by Bending and Bridging
title_full Archaeal Chromatin Proteins Cren7 and Sul7d Compact DNA by Bending and Bridging
title_fullStr Archaeal Chromatin Proteins Cren7 and Sul7d Compact DNA by Bending and Bridging
title_full_unstemmed Archaeal Chromatin Proteins Cren7 and Sul7d Compact DNA by Bending and Bridging
title_sort archaeal chromatin proteins cren7 and sul7d compact dna by bending and bridging
publisher American Society for Microbiology
series mBio
issn 2150-7511
publishDate 2020-06-01
description A long-standing question is how chromosomal DNA is packaged in Crenarchaeota, a major group of archaea, which synthesize large amounts of unique small DNA-binding proteins but in general contain no archaeal histones. In the present work, we tested our hypothesis that the two well-studied crenarchaeal chromatin proteins Cren7 and Sul7d compact DNA by both DNA bending and bridging. We show that the two proteins are capable of compacting DNA, albeit with different efficiencies and in different manners, at the single molecule level. We demonstrate for the first time that the two proteins, which have long been regarded as DNA binders and benders, are able to mediate DNA bridging, and this previously unknown property of the proteins allows DNA to be packaged into highly condensed structures. Therefore, our results provide significant insights into the mechanism and kinetics of chromosomal DNA organization in Crenarchaeota.Archaeal chromatin proteins Cren7 and Sul7d from Sulfolobus are DNA benders. To better understand their architectural roles in chromosomal DNA organization, we analyzed DNA compaction by Cren7 and Sis7d, a Sul7d family member, from Sulfolobus islandicus at the single-molecule (SM) level by total single-molecule internal reflection fluorescence microscopy (SM-TIRFM) and atomic force microscopy (AFM). We show that both Cren7 and Sis7d were able to compact singly tethered λ DNA into a highly condensed structure in a three-step process and that Cren7 was over an order of magnitude more efficient than Sis7d in DNA compaction. The two proteins were similar in DNA bending kinetics but different in DNA condensation patterns. At saturating concentrations, Sis7d formed randomly distributed clusters whereas Cren7 generated a single and highly condensed core on plasmid DNA. This observation is consistent with the greater ability of Cren7 than of Sis7d to bridge DNA. Our results offer significant insights into the mechanism and kinetics of chromosomal DNA organization in Crenarchaea.
topic archaea
atomic force microscopy
chromatin protein
single-molecule technology
sulfolobus
url https://doi.org/10.1128/mBio.00804-20
work_keys_str_mv AT zhenfengzhang archaealchromatinproteinscren7andsul7dcompactdnabybendingandbridging
AT zhengyanzhan archaealchromatinproteinscren7andsul7dcompactdnabybendingandbridging
AT bingwang archaealchromatinproteinscren7andsul7dcompactdnabybendingandbridging
AT yuanyuanchen archaealchromatinproteinscren7andsul7dcompactdnabybendingandbridging
AT xiuqiangchen archaealchromatinproteinscren7andsul7dcompactdnabybendingandbridging
AT cuihongwan archaealchromatinproteinscren7andsul7dcompactdnabybendingandbridging
AT yufu archaealchromatinproteinscren7andsul7dcompactdnabybendingandbridging
AT lihuang archaealchromatinproteinscren7andsul7dcompactdnabybendingandbridging
_version_ 1721329625013944320

Similar Items