DNA supercoil
DNA supercoiling refers to the over- or under-winding of a DNA strand, and is an expression of the strain on that strand. Supercoiling is important in a number of biological processes, such as compacting DNA, and by regulating access to the genetic code, DNA supercoiling strongly affects DNA metabolism and possibly gene expression. Additionally, certain enzymes such as topoisomerases are able to change DNA topology to facilitate functions such as DNA replication or transcription.[1] Mathematical expressions are used to describe supercoiling by comparing different coiled states to relaxed B-form DNA.
Overview
In a "relaxed" double-helical segment of B-DNA, the two strands twist around the helical axis once every 10.4–10.5 base pairs of sequence. Adding or subtracting twists, as some enzymes can do, imposes strain. If a DNA segment under twist strain were closed into a circle by joining its two ends and then allowed to move freely, the circular DNA would contort into a new shape, such as a simple figure-eight. Such a contortion is a supercoil. The noun form "supercoil" is often used in the context of DNA topology.
Positively supercoiled (overwound) DNA is transiently generated during DNA replication and transcription, and, if not promptly relaxed, inhibits (regulates) these processes. The simple figure eight is the simplest supercoil, and is the shape a circular DNA assumes to accommodate one too many or one too few helical twists. The two lobes of the figure eight will appear rotated either clockwise or counterclockwise with respect to one another, depending on whether the helix is over- or underwound. For each additional helical twist being accommodated, the lobes will show one more rotation about their axis. As a general rule, the DNA of most organisms is negatively supercoiled.[2]
Lobal contortions of a circular DNA, such as the rotation of the figure-eight lobes above, are referred to as writhe. The above example illustrates that twist and writhe are interconvertible. Supercoiling can be represented mathematically by the sum of twist and writhe. The twist is the number of helical turns in the DNA and the writhe is the number of times the double helix crosses over on itself (these are the supercoils). Extra helical twists are positive and lead to positive supercoiling, while subtractive twisting causes negative supercoiling. Many topoisomerase enzymes sense supercoiling and either generate or dissipate it as they change DNA topology.
In part because chromosomes may be very large, segments in the middle may act as if their ends are anchored. As a result, they may be unable to distribute excess twist to the rest of the chromosome or to absorb twist to recover from underwinding—the segments may become supercoiled, in other words. In response to supercoiling, they will assume an amount of writhe, just as if their ends were joined.
Supercoiled DNA forms two structures; a plectoneme or a toroid, or a combination of both. A negatively supercoiled DNA molecule will produce either a one-start left-handed helix, the toroid, or a two-start right-handed helix with terminal loops, the plectoneme. Plectonemes are typically more common in nature, and this is the shape most bacterial plasmids will take. For larger molecules it is common for hybrid structures to form – a loop on a toroid can extend into a plectoneme. If all the loops on a toroid extend then it becomes a branch point in the plectonemic structure. DNA supercoiling is important for DNA packaging within all cells, and seems to also play a role in gene expression.[3][4]
Intercalation-induced supercoiling of DNA
Based on the properties of intercalating molecules i.e., fluorescing upon binding to DNA and unwinding of DNA base-pairs, recently a single-molecule technique has been introduced to directly visualize individual plectonemes along supercoiled DNA[5] which would further allow to study the interactions of DNA processing proteins with supercoiled DNA. In that study, Sytox Orange (an intercalating dye), has been used to induce supercoiling on surface tethered DNA molecules.
Using this assay, it was found that the DNA sequence encodes for the position of plectonemic supercoils.[6] Furthermore, DNA supercoils were found to be enriched at the transcription start sites in prokaryotes.
Functions
Genome packaging
DNA supercoiling is important for DNA packaging within all cells. Because the length of DNA can be thousands of times that of a cell, packaging this genetic material into the cell or nucleus (in eukaryotes) is a difficult feat. Supercoiling of DNA reduces the space and allows for DNA to be packaged. In prokaryotes, plectonemic supercoils are predominant, because of the circular chromosome and relatively small amount of genetic material. In eukaryotes, DNA supercoiling exists on many levels of both plectonemic and solenoidal supercoils, with the solenoidal supercoiling proving most effective in compacting the DNA. Solenoidal supercoiling is achieved with histones to form a 10 nm fiber. This fiber is further coiled into a 30 nm fiber, and further coiled upon itself numerous times more.
DNA packaging is greatly increased during mitosis when duplicated sister DNAs are segregated into daughter cells. It has been shown that condensin, a large protein complex that plays a central role in mitotic chromosome assembly, induces positive supercoils in an ATP hydrolysis-dependent manner in vitro.[7][8] Supercoiling could also play an important role during interphase in the formation and maintenance of topologically associating domains (TADs).[9]
Supercoiling is also required for DNA/RNA synthesis. Because DNA must be unwound for DNA/RNA polymerase action, supercoils will result. The region ahead of the polymerase complex will be unwound; this stress is compensated with positive supercoils ahead of the complex. Behind the complex, DNA is rewound and there will be compensatory negative supercoils. Topoisomerases such as DNA gyrase (Type II Topoisomerase) play a role in relieving some of the stress during DNA/RNA synthesis.[10]
Gene expression
Specialized proteins can unzip small segments of the DNA molecule when it is replicated or transcribed into RNA. But work published in 2015 illustrates how DNA opens on its own.[3][4]
Simply twisting DNA can expose internal bases to the outside, without the aid of any proteins. Also, transcription itself contorts DNA in living human cells, tightening some parts of the coil and loosening it in others. That stress triggers changes in shape, most notably opening up the helix to be read. Unfortunately, these interactions are very difficult to study because biological molecules morph shapes so easily. In 2008 it was noted that transcription twists DNA, leaving a trail of undercoiled (or negatively supercoiled) DNA in its wake. Moreover, they discovered that the DNA sequence itself affects how the molecule responds to supercoiling.[3][4] For example, the researchers identified a specific sequence of DNA that regulates transcription speed; as the amount of supercoil rises and falls, it slows or speeds the pace at which molecular machinery reads DNA.[3] It is hypothesized that these structural changes might trigger stress elsewhere along its length, which in turn might provide trigger points for replication or gene expression.[3][4] This implies that it is a very dynamic process in which both DNA and proteins each influences how the other acts and reacts.[3]
Mathematical description
In nature, circular DNA is always isolated as a higher-order helix-upon-a-helix, known as a superhelix. In discussions of this subject, the Watson-Crick twist is referred to as a "secondary" winding, and the superhelices as a "tertiary" winding. The sketch at right indicates a "relaxed", or "open circular" Watson-Crick double-helix, and, next to it, a right-handed superhelix. The "relaxed" structure on the left is not found unless the chromosome is nicked; the superhelix is the form usually found in nature.
For purposes of mathematical computations, a right-handed superhelix is defined as having a "negative" number of superhelical turns, and a left-handed superhelix is defined as having a "positive" number of superhelical turns. In the drawing (shown at the right), both the secondary (i.e., "Watson-Crick") winding and the tertiary (i.e., "superhelical") winding are right-handed, hence the supertwists are negative (-3 in this example).
The superhelicity is presumed to be a result of underwinding, meaning that there is a deficiency in the number of secondary Watson-Crick twists. Such a chromosome will be strained, just as a macroscopic metal spring is strained when it is either overwound or unwound. In DNA which is thusly strained, supertwists will appear.
DNA supercoiling can be described numerically by changes in the linking number Lk. The linking number is the most descriptive property of supercoiled DNA. Lko, the number of turns in the relaxed (B type) DNA plasmid/molecule, is determined by dividing the total base pairs of the molecule by the relaxed bp/turn which, depending on reference is 10.4;[11] 10.5;[12][13] 10.6.[14]
Lk is merely the number of crosses a single strand makes across the other. Lk, known as the "linking number", is the number of Watson-Crick twists found in a circular chromosome in a (usually imaginary) planar projection. This number is physically "locked in" at the moment of covalent closure of the chromosome, and cannot be altered without strand breakage.
The topology of the DNA is described by the equation below in which the linking number is equivalent to the sum of TW, which is the number of twists or turns of the double helix, and Wr which is the number of coils or 'writhes'. If there is a closed DNA molecule, the sum of Tw and Wr, or the linking number, does not change. However, there may be complementary changes in TW and Wr without changing their sum.
Tw, called "twist", refers to the number of Watson-Crick twists in the chromosome when it is not constrained to lie in a plane. We have already seen that native DNA is usually found to be superhelical. If one goes around the superhelically twisted chromosome, counting secondary Watson-Crick twists, that number will be different from the number counted when the chromosome is constrained to lie flat. In general, the number of secondary twists in the native, supertwisted chromosome is expected to be the "normal" Watson-Crick winding number, meaning a single 10-base-pair helical twist for every 34 Å of DNA length.
Wr, called "writhe", is the number of superhelical twists. Since biological circular DNA is usually underwound, Lk will generally be less than Tw, which means that Wr will typically be negative.
If DNA is underwound, it will be under strain, exactly as a metal spring is strained when forcefully unwound, and that the appearance of supertwists will allow the chromosome to relieve its strain by taking on negative supertwists, which correct the secondary underwinding in accordance with the topology equation above.
The topology equation shows that there is a one-to-one relationship between changes in Tw and Wr. For example, if a secondary "Watson-Crick" twist is removed, then a right-handed supertwist must have been removed simultaneously (or, if the chromosome is relaxed, with no supertwists, then a left-handed supertwist must be added).
The change in the linking number, ΔLk, is the actual number of turns in the plasmid/molecule, Lk, minus the number of turns in the relaxed plasmid/molecule Lko.
If the DNA is negatively supercoiled ΔLk < 0. The negative supercoiling implies that the DNA is underwound.
A standard expression independent of the molecule size is the "specific linking difference" or "superhelical density" denoted σ, that represents the number of turns added or removed relative to the total number of turns in the relaxed molecule/plasmid, indicating the level of supercoiling.
The Gibbs free energy associated with the coiling is given by the equation below[15]
The difference in Gibbs free energy between the supercoiled circular DNA and uncoiled circular DNA with N > 2000 bp is approximated by:
or, 16 cal/bp.
Since the linking number L of supercoiled DNA is the number of times the two strands are intertwined (and both strands remain covalently intact), L cannot change. The reference state (or parameter) L0 of a circular DNA duplex is its relaxed state. In this state, its writhe W = 0. Since L = T + W, in a relaxed state T = L. Thus, if we have a 400 bp relaxed circular DNA duplex, L ~ 40 (assuming ~10 bp per turn in B-DNA). Then T ~ 40.
- Positively supercoiling:
- T = 0, W = 0, then L = 0
- T = +3, W = 0, then L = +3
- T = +2, W = +1, then L = +3
- Negatively supercoiling:
- T = 0, W = 0, then L = 0
- T = -3, W = 0, then L = -3
- T = -2, W = -1, then L = -3
Negative supercoils favor local unwinding of the DNA, allowing processes such as transcription, DNA replication, and recombination. Negative supercoiling is also thought to favour the transition between B-DNA and Z-DNA, and moderate the interactions of DNA binding proteins involved in gene regulation.[16]
Effects on sedimentation coefficient
The topological properties of circular DNA are complex. In standard texts, these properties are invariably explained in terms of a helical model for DNA, but in 2008 it was noted that each topoisomer, negative or positive, adopts a unique and surprisingly wide distribution of three-dimensional conformations.[4]
When the sedimentation coefficient, s, of circular DNA is ascertained over a large range of pH, the following curves are seen. Three curves are shown here, representing three species of DNA. From top-to-bottom they are: "Form IV" (green), "Form I" (blue) and "Form II" (red).
"Form I" (blue curve) is the traditional nomenclature used for the native form of duplex circular DNA, as recovered from viruses and intracellular plasmids. Form I is covalently closed, and any plectonemic winding which may be present is therefore locked in. If one or more nicks are introduced to Form I, free rotation of one strand with respect to the other becomes possible, and Form II (red curve) is seen.
Form IV (green curve) is the product of alkali denaturation of Form I. Its structure is unknown, except that it is persistently duplex, and extremely dense.
Between pH 7 and pH 11.5, the sedimentation coefficient s, for Form I, is constant. Then it dips, and at a pH just below 12, reaches a minimum. With further increases in pH, s then returns to its former value. It doesn’t stop there, however, but continues to increase relentlessly. By pH 13, the value of s has risen to nearly 50, two to three times its value at pH 7, indicating an extremely compact structure.
If the pH is then lowered, the s value is not restored. Instead, one sees the upper, green curve. The DNA, now in the state known as Form IV, remains extremely dense, even if the pH is restored to the original physiologic range. As stated previously, the structure of Form IV is almost entirely unknown, and there is no currently accepted explanation for its extraordinary density. About all that is known about the tertiary structure is that it is duplex, but has no hydrogen bonding between bases.
These behaviors of Forms I and IV are considered to be due to the peculiar properties of duplex DNA which has been covalently closed into a double-stranded circle. If the covalent integrity is disrupted by even a single nick in one of the strands, all such topological behavior ceases, and one sees the lower Form II curve (Δ). For Form II, alterations in pH have very little effect on s. Its physical properties are, in general, identical to those of linear DNA. At pH 13, the strands of Form II simply separate, just as the strands of linear DNA do. The separated single strands have slightly different s values, but display no significant changes in s with further increases in pH.
A complete explanation for these data is beyond the scope of this article. In brief, the alterations in s come about because of changes in the superhelicity of circular DNA. These changes in superhelicity are schematically illustrated by four little drawings which have been strategically superimposed upon the figure above.
Briefly, the alterations of s seen in the pH titration curve above are widely thought to be due to changes in the superhelical winding of DNA under conditions of increasing pH. Up to pH 11.5, the purported "underwinding" produces a right-handed ("negative") supertwist. But as the pH increases, and the secondary helical structure begins to denature and unwind, the chromosome (if we may speak anthropomorphically) no longer "wants" to have the full Watson-Crick winding, but rather "wants", increasingly, to be "underwound". Since there is less and less strain to be relieved by superhelical winding, the superhelices therefore progressively disappear as the pH increases. At a pH just below 12, all incentive for superhelicity has expired, and the chromosome will appear as a relaxed, open circle.
At higher pH still, the chromosome, which is now denaturing in earnest, tends to unwind entirely, which it cannot do so (because Lk is covalently locked in). Under these conditions, what was once treated as "underwinding" has actually now become "overwinding". Once again there is strain, and once again it is (in part at least) relieved by superhelicity, but this time in the opposite direction (i.e., left-handed or "positive"). Each left-handed tertiary supertwist removes a single, now undesirable right-handed Watson-Crick secondary twist.
The titration ends at pH 13, where Form IV appears.
References
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General references
- Bloomfield, Victor A.; Crothers, Donald M.; Tinoco, Jr., Ignacio (2000). Nucleic acids: structures, properties, and functions. Sausalito, California: University Science Books. pp. 446–453. ISBN 978-0935702491.