How does semi-conservative replication help prevent mutations during DNA replication?

Answer 1

Semi conservative replication prevents mutations during DNA replication because it produces 2 copies that each contained 1 of the original strands and 1 entirely new strand.

Answer 2

DNA replication is a truly amazing biological phenomenon. Consider the countless number of times that your cells divide to make you who you are-not just during development, but even now, as a fully mature adult. Then consider that every time a human cell divides and its DNA replicates, it has to copy and transmit the exact same sequence of 3 billion nucleotides to its daughter cells. Finally, consider the fact that in life (literally), nothing is perfect. While most DNA replicates with fairly high fidelity, mistakes do happen, with polymerase enzymes sometimes inserting the wrong nucleotide or too many or too few nucleotides into a sequence. Fortunately, most of these mistakes are fixed through various DNA repair processes. Repair enzymes recognize structural imperfections between improperly paired nucleotides, cutting out the wrong ones and putting the right ones in their place. But some replication errors make it past these mechanisms, thus becoming permanent mutations. These altered nucleotide sequences can then be passed down from one cellular generation to the next, and if they occur in cells that give rise to gametes, they can even be transmitted to subsequent organismal generations. Moreover, when the genes for the DNA repair enzymes themselves become mutated, mistakes begin accumulating at a much higher rate. In eukaryotes, such mutations can lead to cancer.

Figure 1

After James Watson and Francis Crick published their model of the double-helix structure of DNA in 1953, biologists initially speculated that most replication errors were caused by what are called tautomeric shifts. Both the purine and pyrimidine bases in DNA exist in different chemical forms, or tautomers, in which the protons occupy different positions in the molecule (Figure 1). The Watson-Crick model required that the nucleotide bases be in their more common "keto" form (Watson & Crick, 1953). Scientists believed that if and when a nucleotide base shifted into its rarer tautomeric form (the "imino" or "enol" form), a likely result would be base-pair mismatching. But evidence for these types of tautomeric shifts remains sparse.

Today, scientists suspect that most DNA replication errors are caused by mispairings of a different nature: either between different but nontautomeric chemical forms of bases (e.g., bases with an extra proton, which can still bind but often with a mismatched nucleotide, such as an A with a G instead of a T) or between "normal" bases that nonetheless bond inappropriately (e.g., again, an A with a G instead of a T) because of a slight shift in position of the nucleotides in space (Figure 2). This type of mispairing is known as wobble. It occurs because the DNA double helix is flexible and able to accommodate slightly misshaped pairings (Crick, 1966).

Replication errors can also involve insertions or deletions of nucleotide bases that occur during a process called strand slippage. Sometimes, a newly synthesized strand loops out a bit, resulting in the addition of an extra nucleotide base (Figure 3). Other times, the template strand loops out a bit, resulting in the omission, or deletion, of a nucleotide base in the newly synthesized, or primer, strand. Regions of DNA containing many copies of small repeated sequences are particularly prone to this type of error.

Figure 2: Nonstandard base pairings can occur as a result of the flexibility in DNA structure.

Thymine and guanine can pair through wobble between normal bases. Cytosine and adenine can pair through wobble when adenine is protonated (has an extra hydrogen).

Used with permission. © 2005 by W. H. Freeman and Company. All rights reserved.

DNA polymerase enzymes are amazingly particular with respect to their choice of nucleotides during DNA synthesis, ensuring that the bases added to a growing strand are correctly paired with their complements on the template strand (i.e., A's with T's, and C's with G's). Nonetheless, these enzymes do make mistakes at a rate of about 1 per every 100,000 nucleotides. That might not seem like much, until you consider how much DNA a cell has. In humans, with our 6 billion base pairs in each diploid cell, that would amount to about 120,000 mistakes every time a cell divides!

Fortunately, cells have evolved highly sophisticated means of fixing most, but not all, of those mistakes. Some of the mistakes are corrected immediately during replication through a process known as proofreading, and some are corrected after replication in a process called mismatch repair. When an incorrect nucleotide is added to the growing strand, replication is stalled by the fact that the nucleotide's exposed 3′-OH group is in the "wrong" position. (Recall that new nucleotides are added to the growing strand during replication by means of their 5′-phosphate group binding to the 3′-OH group of the previous nucleotide on the strand.) During proofreading, DNA polymerase enzymes recognize this and replace the incorrectly inserted nucleotide so that replication can continue. Proofreading fixes about 99% of these types of errors, but that's still not good enough for normal cell functioning.

After replication, mismatch repair reduces the final error rate even further. Incorrectly paired nucleotides cause deformities in the secondary structure of the final DNA molecule. During mismatch repair, enzymes recognize and fix these deformities by removing the incorrectly paired nucleotide and replacing it with the correct nucleotide.

Figure 3: Insertions and deletions may result from strand slippage.

Used with permission. © 2005 by W. H. Freeman and Company. All rights reserved.

Incorrectly paired nucleotides that still remain following mismatch repair become permanent mutations after the next cell division. This is because once such mistakes are established, the cell no longer recognizes them as errors. Consider the case of wobble-induced replication errors. When these mistakes are not corrected, the incorrectly sequenced DNA strand serves as a template for future replication events, causing all the base-pairings thereafter to be wrong. For instance, in the lower half of Figure 2, the original strand has a C-G pair; then, during replication, cytosine (C) is incorrectly matched to adenine (A) because of wobble. In this example, wobble occurs because A has an extra hydrogen atom. In the next round of cell division, the double strand with the C-A pairing would separate during replication, each strand serving as a template for synthesis of a new DNA molecule. At that particular spot, C would pair with G, forming a double helix with the same sequence as its original (i.e., before the wobble occurred), but A would pair with T, forming a new DNA molecule with an A-T pair in place of the original C-G pair. This type of mutation is known as a base, or base-pair, substitution. Base substitutions involving replacement of one purine for another or one pyrimidine for another (e.g., a mismatched A-A pair, instead of A-T) are known as transitions; the replacement of a purine by a pyrimidine, or vice versa, is called a transversion.

Likewise, when strand-slippage replication errors are not corrected, they become insertion and deletion mutations. Much of the early research on strand-slippage mutations was conducted by George Streisinger in the 1970s. Streisinger, a professor at the University of Oregon and a fish hobbyist, is known by some as the "founding father of zebrafish research." However, he is also known for his work with phage T4, a bacterial virus. Streisinger used this virus to show that most nucleotide insertion and deletion mutations occur in areas of DNA that contain many repeated sequences (also called tandem repeats), and he formulated the strand-slippage hypothesis to explain why this was the case (Streisinger et al., 1966). (In Figure 3, notice the series of repeat T's on the primer strand where the slippage has occurred.) When slippage takes place, the presence of nearby duplicate bases stabilizes the slippage so that replication can proceed. During the next round of replication, when the two strands separate, the insertion or deletion on either the template or primer strand, respectively, will be perpetuated as a permanent mutation. Scientists have collected enough evidence to confirm Streisinger's strand-slippage hypothesis, and this type of mutagenesis remains an active field of scientific research.

Although most mutations are believed to be caused by replication errors, they can also be caused by various environmentally induced and spontaneous changes to DNA that occur prior to replication but are perpetuated in the same way as unfixed replication errors. As with replication errors, most environmentally induced DNA damage is repaired, resulting in fewer than 1 out of every 1,000 chemically induced lesions actually becoming permanent mutations. The same is true of so-called spontaneous mutations. "Spontaneous" refers to the fact that the changes occur in the absence of chemical, radiation, or other environmental damage. Rather, they are usually caused by normal chemical reactions that go on in cells, such as hydrolysis. These types of errors include depurination, which occurs when the bond connecting a purine to its deoxyribose sugar is broken by a molecule of water, resulting in a purine-free nucleotide that can't act as a template during DNA replication, and deamination, which results in the loss of an amino group from a nucleotide, again by reaction with water. Again, most of these spontaneous errors are corrected by DNA repair processes. But if this does not occur, a nucleotide that is added to the newly synthesized strand can become a permanent mutation.