Micromechanical Analysis of the Binding of DNA-Bending Proteins HMGB1, NHP6A, and HU Reveals Their Ability To Form Highly Stable DNA−Protein Complexes

Skoko, Dunja; Wong, Ben; Johnson, Reid C.; Marko, John F.

doi:10.1021/bi048428o

Cited by 140 publications

(211 citation statements)

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“…However, the data are consistent with a chromosome composed of highly condensed DNA. This description gives a segment length of order 40 nm, which is more in line with studies of DNA bound to nucleoid-associated proteins (35)(36)(37)(38). A recent study of the positioning of chromosomal loci in E. coli similarly concluded that the chromosome contains a higher-order structure that can be modeled as a condensed DNA fiber (5).…”

Section: Discussionsupporting

confidence: 57%

Membrane protein expression triggers chromosomal locus repositioning in bacteria

Libby¹,

Roggiani

Goulian

2012

Proc. Natl. Acad. Sci. U.S.A.

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It has long been hypothesized that subcellular positioning of chromosomal loci in bacteria may be influenced by gene function and expression state. Here we provide direct evidence that membrane protein expression affects the position of chromosomal loci in Escherichia coli. For two different membrane proteins, we observed a dramatic shift of their genetic loci toward the membrane upon induction. In related systems in which a cytoplasmic protein was produced, or translation was eliminated by mutating the start codon, a shift was not observed. Antibiotics that block transcription and translation similarly prevented locus repositioning toward the membrane. We also found that repositioning is relatively rapid and can be detected at positions that are a considerable distance on the chromosome from the gene encoding the membrane protein (>90 kb). Given that membrane protein-encoding genes are distributed throughout the chromosome, their expression may be an important mechanism for maintaining the bacterial chromosome in an expanded and dynamic state.bacterial nucleoid | chromosome-membrane association | transertion S tudies of several different bacteria have revealed that their chromosomes are organized structures, with genetic loci occupying relatively defined positions along the long axis of the cell (1-7). However, the potential impact of gene function and expression state on chromosome organization and on subcellular positioning of specific loci remains relatively unexplored. Such modulation of the spatial organization of the chromosome may affect numerous cellular processes, including the regulation of gene expression, gross transcriptional control, assembly of macromolecular complexes and domains, and the generation of cellular asymmetry (8)(9)(10)(11)(12)(13)(14).One long-standing hypothesis posits that genes actively expressing membrane proteins are localized to regions proximal to the membrane (8,11,15). To date, however, there is no direct evidence for membrane protein expression affecting the subcellular positions of chromosomal loci. We therefore sought to test directly whether expressing a membrane protein affects the localization of its encoding gene in Escherichia coli. We tested two loci and found that induction of membrane protein expression rapidly results in a dramatic repositioning toward the membrane. We also show that the positions of chromosomal loci as far away as 90 kb from the induced gene are affected. This shift in position is a significant perturbation on the scale of the cell and may therefore be a major determinant of chromosome conformation. ResultsWe first tested the effect of inducing the lac operon on the intracellular position of the chromosomal lac locus. The operon lacZYA encodes the membrane protein lactose permease (LacY), in addition to two cytoplasmic proteins, beta-galactosidase (LacZ) and galactoside acetyltransferase (LacA). To follow the intracellular position of lacZYA, we inserted an array of Tet repressor binding sites (tetO) in the gene cynX, which is adjacent to lacA ...

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Section: Discussionsupporting

confidence: 57%

Membrane protein expression triggers chromosomal locus repositioning in bacteria

Libby¹,

Roggiani

Goulian

2012

Proc. Natl. Acad. Sci. U.S.A.

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“…All single-molecule micromanipulation experiments were performed by using the magnetic tweezers setup described (23,24). Flow-cell preparation, force measurements, and calibration were performed as described (23,24).…”

Section: Methodsmentioning

confidence: 99%

Topoisomerase V relaxes supercoiled DNA by a constrained swiveling mechanism

Taneja

Schnurr

Slesarev

et al. 2007

Proc. Natl. Acad. Sci. U.S.A.

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Topoisomerase V is a type I topoisomerase without structural or sequence similarities to other topoisomerases. Although it belongs to the type I subfamily of topoisomerases, it is unrelated to either type IA or IB enzymes. We used real-time single-molecule micromechanical experiments to show that topoisomerase V relaxes DNA via events that release multiple DNA turns, employing a constrained swiveling mechanism similar to that for type IB enzymes. Relaxation is powered by the torque in the supercoiled DNA and is constrained by friction between the protein and the DNA. Although all type IB enzymes share a common structure and mechanism and type IA and type II enzymes show marked structural and functional similarities, topoisomerase V represents a different type of topoisomerase that relaxes DNA in a similar overall manner as type IB molecules but by using a completely different structural and mechanistic framework.magnetic tweezers ͉ single molecule ͉ archaeon ͉ DNA topology ͉ type IC T opoisomerase V (topo V) of the archaeon Methanopyrus kandleri is a 110-kDa enzyme belonging to the type I family of topoisomerases (1). Type I topoisomerases previously have been subdivided into two subtypes, IA and IB (2), based on whether they form a transient 5Ј or 3Ј covalent bond with the broken DNA strand (reviewed in ref.3). Topo V possesses biochemical properties associated with type IB topoisomerases, namely, cleavage of a single DNA strand, formation of a covalent intermediate with the 3Ј end of the broken strand, and the ability to relax both positive and negative supercoils in a magnesium-and ATP-independent manner (1). Despite these commonalities, topo V shows no sequence similarity to other type IB enzymes (4). Furthermore, the structure of topo V bears no resemblance to any known topoisomerase but instead reveals a unique fold (5). Although the active site of topo V includes a constellation of amino acids similar to that in type IB enzymes, their spatial arrangement is different. All these data suggest that, despite overall similarities, topo V and type IB enzymes use different catalytic mechanisms for DNA cleavage and religation. Furthermore, the mechanism of DNA relaxation used by topo V is unknown.Two mechanisms of DNA relaxation have been discussed for type I topoisomerases: an enzyme-bridged strand passage mechanism and a swiveling or ''controlled rotation'' mechanism. Type IA topoisomerases have a characteristic toroidal shape (6) and use an enzyme-bridged strand passage mechanism where both ends of the broken DNA strand are bound to the enzyme, preventing DNA swiveling. The intact DNA strand is passed through the transient break in the other strand before the topoisomerase religates the broken strand. This mechanism changes the DNA linking number strictly in increments of one (⌬Lk ϭ Ϯ1) (7-9). Type IB enzymes use a radically different mechanism involving swiveling, or rotation of one DNA strand around the other, to release supercoils. The protein embraces the DNA and cleaves one strand, allowing the free cleav...

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“…Controlled forces were applied to the bead by using permanent magnets (Smith et al, 1992;Strick et al, 1996Strick et al, , 1998Strick et al, , 2000, and bead positions were measured using digital videomicroscopy and bead-tracking computer software. We used two setups: in the first "vertical MT," the bead is pulled perpendicular to the focal plane, so DNA extension is determined by autofocusing software ( Figure 2a); details are described in Skoko et al (2004). In the second "transverse MT" system the DNA is extended in the focal plane ( Figure 2b); for details, see Yan et al (2004).…”

Section: Magnetic Tweezer (Mt) Setups Allow Precise Observation and Cmentioning

confidence: 99%

Micromanipulation Studies of Chromatin Fibers in Xenopus Egg Extracts Reveal ATP-dependent Chromatin Assembly Dynamics

Yan

Maresca

Skoko

et al. 2007

MBoC

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We have studied assembly of chromatin using Xenopus egg extracts and single DNA molecules held at constant tension by using magnetic tweezers. In the absence of ATP, interphase extracts were able to assemble chromatin against DNA tensions of up to 3.5 piconewtons (pN). We observed force-induced disassembly and opening-closing fluctuations, indicating our experiments were in mechanochemical equilibrium. Roughly 50-nm (150-base pair) lengthening events dominated force-driven disassembly, suggesting that the assembled fibers are chiefly composed of nucleosomes. The ATP-depleted reaction was able to do mechanical work of 27 kcal/mol per 50 nm step, which provides an estimate of the free energy difference between core histone octamers on and off DNA. Addition of ATP led to highly dynamic behavior with time courses exhibiting processive runs of assembly and disassembly not observed in the ATP-depleted case. With ATP present, application of forces of 2 pN led to nearly complete fiber disassembly. Our study suggests that ATP hydrolysis plays a major role in nucleosome rearrangement and removal and that chromatin in vivo may be subject to highly dynamic assembly and disassembly processes that are modulated by DNA tension. INTRODUCTIONTranscription, replication, and other in vivo DNA processing in eukaryotes take place in the context of chromatin. The processive nature of these activities, and the necessity to disrupt histone-DNA contacts to accomplish them, suggests that chromatin must be dynamic in its structure, with actively transcribing genes perhaps in a continual state of structural rearrangement. The simplest example of chromatin rearrangement that would allow base pair access is displacement or dissociation of part or all of the histone octamer (Felsenfeld, 1996).Chromosome visualization in vivo gives insight into chromatin dynamics at large length scales (Belmont, 2003;Levi et al., 2005) but is as yet unable to reveal events at the scale of individual nucleosome displacements. A complementary approach is to study individual chromatin fibers by using micromanipulation (Cui and Bustamante, 2000;Ladoux et al., 2000;Bennink et al., 2001;Brower-Toland et al., 2002;Leuba et al., 2003;Claudet et al., 2005;Gemmen et al., 2005;Bancaud et al., 2006). A major objective of such experiments has been the study of mechanically triggered changes in protein-DNA contacts, with an emphasis on force-driven opening of nucleosomes.However, biophysical micromanipulation experiments offer possibilities beyond simply disassembling chromatin by force; experiments in "active" solutions containing chromatin-organizing or chromatin-processing enzymes permit direct observation of chromatin dynamics, and they can reveal details of structure and mechanism concerning compaction of DNA into chromatin, chromatin remodeling, gene expression in chromatin, mitotic chromosome condensation, and how such processes are affected by DNA tension. DNA tension is physiologically relevant because pulling of chromatin is likely to occur in vivo, given the larg...

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Micromechanical Analysis of the Binding of DNA-Bending Proteins HMGB1, NHP6A, and HU Reveals Their Ability To Form Highly Stable DNA−Protein Complexes

Cited by 140 publications

References 39 publications

Membrane protein expression triggers chromosomal locus repositioning in bacteria

Membrane protein expression triggers chromosomal locus repositioning in bacteria

Topoisomerase V relaxes supercoiled DNA by a constrained swiveling mechanism

Micromanipulation Studies of Chromatin Fibers in Xenopus Egg Extracts Reveal ATP-dependent Chromatin Assembly Dynamics

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