"De novo mutation" redirects here. For De novo mutation, see
De novo.
In molecular biology and genetics, mutations are changes in a genomic sequence: the DNA sequence of a cell's genome or the DNA or RNA sequence of a virus. These random sequences can be defined as sudden and spontaneous changes in the cell. Mutations are caused by radiation, viruses, transposons and mutagenic chemicals, as well as errors that occur during meiosis or DNA replication.[1][2][3] They can also be induced by the organism itself, by cellular processes such as hypermutation.
Mutation can result in several different types of change in sequences; these can either have no effect, alter the product of a gene, or prevent the gene from functioning properly or completely. One study on genetic variations between different species of Drosophila suggests that if a mutation changes a protein produced by a gene, the result is likely to be harmful, with an estimated 70 percent of amino acid polymorphisms having damaging effects, and the remainder being either neutral or weakly beneficial.[4] Due to the damaging effects that mutations can have on genes, organisms have mechanisms such as DNA repair to prevent mutations.[1]
Mutations can involve large sections of DNA becoming duplicated, usually through genetic recombination.[5] These duplications are a major source of raw material for evolving new genes, with tens to hundreds of genes duplicated in animal genomes every million years.[6] Most genes belong to larger families of genes of shared ancestry.[7] Novel genes are produced by several methods, commonly through the duplication and mutation of an ancestral gene, or by recombining parts of different genes to form new combinations with new functions.[8][9]
Here, domains act as modules, each with a particular and independent function, that can be mixed together to produce genes encoding new proteins with novel properties.[10] For example, the human eye uses four genes to make structures that sense light: three for color vision and one for night vision; all four arose from a single ancestral gene.[11] Another advantage of duplicating a gene (or even an entire genome) is that this increases redundancy; this allows one gene in the pair to acquire a new function while the other copy performs the original function.[12][13] Other types of mutation occasionally create new genes from previously noncoding DNA.[14][15]
Changes in chromosome number may involve even larger mutations, where segments of the DNA within chromosomes break and then rearrange. For example, in the Homininae, two chromosomes fused to produce human chromosome 2; this fusion did not occur in the lineage of the other apes, and they retain these separate chromosomes.[16] In evolution, the most important role of such chromosomal rearrangements may be to accelerate the divergence of a population into new species by making populations less likely to interbreed, and thereby preserving genetic differences between these populations.[17]
Sequences of DNA that can move about the genome, such as transposons, make up a major fraction of the genetic material of plants and animals, and may have been important in the evolution of genomes.[18] For example, more than a million copies of the Alu sequence are present in the human genome, and these sequences have now been recruited to perform functions such as regulating gene expression.[19] Another effect of these mobile DNA sequences is that when they move within a genome, they can mutate or delete existing genes and thereby produce genetic diversity.[2]
Nonlethal mutations accumulate within the gene pool and increase the amount of genetic variation.[20] The abundance of some genetic changes within the gene pool can be reduced by natural selection, while other "more favorable" mutations may accumulate and result in adaptive changes.
For example, a butterfly may produce offspring with new mutations. The majority of these mutations will have no effect; but one might change the color of one of the butterfly's offspring, making it harder (or easier) for predators to see. If this color change is advantageous, the chance of this butterfly surviving and producing its own offspring are a little better, and over time the number of butterflies with this mutation may form a larger percentage of the population.
Neutral mutations are defined as mutations whose effects do not influence the fitness of an individual. These can accumulate over time due to genetic drift. It is believed that the overwhelming majority of mutations have no significant effect on an organism's fitness. Also, DNA repair mechanisms are able to mend most changes before they become permanent mutations, and many organisms have mechanisms for eliminating otherwise permanently mutated somatic cells.
Beneficial mutations can improve reproductive success.
Main article:
Mutagenesis
Two classes of mutations are spontaneous mutations (molecular decay) and induced mutations caused by mutagens.
Spontaneous mutations on the molecular level can be caused by:[21]
- Tautomerism – A base is changed by the repositioning of a hydrogen atom, altering the hydrogen bonding pattern of that base resulting in incorrect base pairing during replication.
- Depurination – Loss of a purine base (A or G) to form an apurinic site (AP site).
- Deamination – Hydrolysis changes a normal base to an atypical base containing a keto group in place of the original amine group. Examples include C → U and A → HX (hypoxanthine), which can be corrected by DNA repair mechanisms; and 5MeC (5-methylcytosine) → T, which is less likely to be detected as a mutation because thymine is a normal DNA base.
- Slipped strand mispairing – Denaturation of the new strand from the template during replication, followed by renaturation in a different spot ("slipping"). This can lead to insertions or deletions.
Induced mutations on the molecular level can be caused by:
- Chemicals
- Hydroxylamine NH2OH
- Base analogs (e.g. BrdU)
- Alkylating agents (e.g. N-ethyl-N-nitrosourea) These agents can mutate both replicating and non-replicating DNA. In contrast, a base analog can only mutate the DNA when the analog is incorporated in replicating the DNA. Each of these classes of chemical mutagens has certain effects that then lead to transitions, transversions, or deletions.
- Agents that form DNA adducts (e.g. ochratoxin A metabolites)[23]
- DNA intercalating agents (e.g. ethidium bromide)
- DNA crosslinkers
- Oxidative damage
- Nitrous acid converts amine groups on A and C to diazo groups, altering their hydrogen bonding patterns which leads to incorrect base pairing during replication.
- Radiation
- Ultraviolet radiation (nonionizing radiation). Two nucleotide bases in DNA – cytosine and thymine – are most vulnerable to radiation that can change their properties. UV light can induce adjacent pyrimidine bases in a DNA strand to become covalently joined as a pyrimidine dimer. UV radiation, particularly longer-wave UVA, can also cause oxidative damage to DNA.[24] Mutation rates also vary across species. Evolutionary biologists[citation needed] have theorized that higher mutation rates are beneficial in some situations, because they allow organisms to evolve and therefore adapt more quickly to their environments. For example, repeated exposure of bacteria to antibiotics, and selection of resistant mutants, can result in the selection of bacteria that have a much higher mutation rate than the original population (mutator strains).
Illustrations of five types of chromosomal mutations.
The sequence of a gene can be altered in a number of ways. Gene mutations have varying effects on health depending on where they occur and whether they alter the function of essential proteins. Mutations in the structure of genes can be classified as:
- Small-scale mutations, such as those affecting a small gene in one or a few nucleotides, including:
- Point mutations, often caused by chemicals or malfunction of DNA replication, exchange a single nucleotide for another.[26] These changes are classified as transitions or transversions.[27] Most common is the transition that exchanges a purine for a purine (A ↔ G) or a pyrimidine for a pyrimidine, (C ↔ T). A transition can be caused by nitrous acid, base mis-pairing, or mutagenic base analogs such as 5-bromo-2-deoxyuridine (BrdU). Less common is a transversion, which exchanges a purine for a pyrimidine or a pyrimidine for a purine (C/T ↔ A/G). An example of a transversion is adenine (A) being converted into a cytosine (C). A point mutation can be reversed by another point mutation, in which the nucleotide is changed back to its original state (true reversion) or by second-site reversion (a complementary mutation elsewhere that results in regained gene functionality). Point mutations that occur within the protein coding region of a gene may be classified into three kinds, depending upon what the erroneous codon codes for:
- Insertions add one or more extra nucleotides into the DNA. They are usually caused by transposable elements, or errors during replication of repeating elements (e.g. AT repeats[citation needed]). Insertions in the coding region of a gene may alter splicing of the mRNA (splice site mutation), or cause a shift in the reading frame (frameshift), both of which can significantly alter the gene product. Insertions can be reverted by excision of the transposable element.
- Deletions remove one or more nucleotides from the DNA. Like insertions, these mutations can alter the reading frame of the gene. They are generally irreversible: though exactly the same sequence might theoretically be restored by an insertion, transposable elements able to revert a very short deletion (say 1–2 bases) in any location are either highly unlikely to exist or do not exist at all. Note that a deletion is not the exact opposite of an insertion: the former is quite random while the latter consists of a specific sequence inserting at locations that are not entirely random or even quite narrowly defined.
- Large-scale mutations in chromosomal structure, including:
- Amplifications (or gene duplications) leading to multiple copies of all chromosomal regions, increasing the dosage of the genes located within them.
- Deletions of large chromosomal regions, leading to loss of the genes within those regions.
- Mutations whose effect is to juxtapose previously separate pieces of DNA, potentially bringing together separate genes to form functionally distinct fusion genes (e.g. bcr-abl). These include:
- Chromosomal translocations: interchange of genetic parts from nonhomologous chromosomes.
- Interstitial deletions: an intra-chromosomal deletion that removes a segment of DNA from a single chromosome, thereby apposing previously distant genes. For example, cells isolated from a human astrocytoma, a type of brain tumor, were found to have a chromosomal deletion removing sequences between the "fused in glioblastoma" (fig) gene and the receptor tyrosine kinase "ros", producing a fusion protein (FIG-ROS). The abnormal FIG-ROS fusion protein has constitutively active kinase activity that causes oncogenic transformation (a transformation from normal cells to cancer cells).
- Chromosomal inversions: reversing the orientation of a chromosomal segment.
- Loss of heterozygosity: loss of one allele, either by a deletion or recombination event, in an organism that previously had two different alleles.
- Loss-of-function mutations are the result of gene product having less or no function. When the allele has a complete loss of function (null allele) it is often called an amorphic mutation. Phenotypes associated with such mutations are most often recessive. Exceptions are when the organism is haploid, or when the reduced dosage of a normal gene product is not enough for a normal phenotype (this is called haploinsufficiency).
- Gain-of-function mutations change the gene product such that it gains a new and abnormal function. These mutations usually have dominant phenotypes. Often called a neomorphic mutation.
- Dominant negative mutations (also called antimorphic mutations) have an altered gene product that acts antagonistically to the wild-type allele. These mutations usually result in an altered molecular function (often inactive) and are characterised by a dominant or semi-dominant phenotype. In humans, Marfan syndrome is an example of a dominant negative mutation occurring in an autosomal dominant disease. In this condition, the defective glycoprotein product of the fibrillin gene (FBN1) antagonizes the product of the normal allele.
- Lethal mutations are mutations that lead to the death of the organisms which carry the mutations.
- A back mutation or reversion is a point mutation that restores the original sequence and hence the original phenotype.[28]
See also Behavior mutation.
In applied genetics it is usual to speak of mutations as either harmful or beneficial.
- A harmful mutation is a mutation that decreases the fitness of the organism.
- A beneficial mutation is a mutation that increases fitness of the organism, or which promotes traits that are desirable.
In theoretical population genetics, it is more usual to speak of such mutations as deleterious or advantageous. In the neutral theory of molecular evolution, genetic drift is the basis for most variation at the molecular level.
- A neutral mutation has no harmful or beneficial effect on the organism. Such mutations occur at a steady rate, forming the basis for the molecular clock.
- A deleterious mutation has a negative effect on the phenotype, and thus decreases the fitness of the organism.
- An advantageous mutation has a positive effect on the phenotype, and thus increases the fitness of the organism.
- A nearly neutral mutation is a mutation that may be slightly deleterious or advantageous, although most nearly neutral mutations are slightly deleterious.
In reality, viewing the fitness effects of mutations in these discrete categories is an oversimplification. Attempts have been made to infer the distribution of fitness effects (DFE) using mutagenesis experiments and theoretical models applied to molecular sequence data. Distribution of fitness effects, as used to determine the relative abundance of different types of mutations (i.e. strongly deleterious, nearly neutral or advantageous), is relevant to many evolutionary questions, such as the maintenance of genetic variation[29] , the rate of genomic decay[30] and the evolution of sex and recombination[31] . In summary, DFE plays an important role in predicting evolutionary dynamics [32] [33] . A variety of approaches have been used to study the distribution of fitness effects, including theoretical, experimental and analytical methods.
- Mutagenesis experiment: The direct method to investigate DFE is to induce mutations and then measure the mutational fitness effects, which has already been done in viruses, bacteria, yeast, and Drosophila. For example, most studies of DFE in viruses used site-directed mutagenesis to create point mutations and measure relative fitness of each mutant [34] [35] [36] [37] . In Escherichia coli, one study used transposon mutagenesis to directly measure the fitness of a random insertion of a derivative of Tn10[38] . In yeast, a combined mutagenesis and deep sequencing approach has been developed to generate high-quality systematic mutant libraries and measure fitness in high throughput [39]. However, given that many mutations have effects too small to be detected[40] and that mutagenesis experiments can only detect mutations of moderately large effect, DNA sequence data analysis can provide valuable information about these mutations.
The distribution of fitness effects of mutations in vesicular stomatitis virus. In this experiment, random mutations were introduced into the virus by site-directed mutagenesis, and the fitness of each mutant was compared with the ancestral type. A fitness of zero, less than one, one, more than one, respectively, indicates that mutations are lethal, deleterious, neutral and advantageous. Data from
[34] .
- Molecular sequence analysis: With rapid development of DNA sequencing technology, an enormous amount of DNA sequence data is available and even more is forthcoming in the future. Various methods have been developed to infer DFE from DNA sequence data[41] [42] [43] [44] . By examining DNA sequence differences within and between species, we are able to infer various characteristics of the DFE for neutral, deleterious and advantageous mutations [45] . Specifically, the DNA sequence analysis approach allows us to estimate the effects of mutations with very small effects, which are hardly detectable through mutagenesis experiments.
One of the earliest theoretical studies of the distribution of fitness effects was done by Motoo Kimura, an influential theoretical population geneticist. His neutral theory of molecular evolution proposes that most novel mutations will be highly deleterious, with a small fraction being neutral[46] [47] . Hiroshi Akashi more recently proposed a bimodal model for DFE, with modes centered around highly deleterious and neutral mutations[48] . Both theories agree that the vast majority of novel mutations are neutral or deleterious and that advantageous mutations are rare, which has been supported by experimental results. One example is a study done on the distribution of fitness effects of random mutations in vesicular stomatitis virus[34] . Out of all mutations, 39.6% were lethal, 31.2% were non-lethal deleterious, and 27.1% were neutral. Another example comes from a high throughput mutagenesis experiment with yeast[39]. In this experiment it was shown that the overall distribution of fitness effects is bimodal, with a cluster of neutral mutations, and a broad distribution of deleterious mutations.
Though relatively few mutations are advantageous, those that are play an important role in evolutionary changes[49]. Like neutral mutations, weakly selected advantageous mutations can be lost due to random genetic drift, but strongly selected advantageous mutations are more likely to be fixed. Knowing the distribution of fitness effects of advantageous mutations may lead to increased ability to predict the evolutionary dynamics. Theoretical work on the DFE for advantageous mutations has been done by John H. Gillespie[50] and H. Allen Orr[51] . They proposed that the distribution for advantageous mutations should be exponential under a wide range of conditions, which has generally been supported by experimental studies, at least for strongly selected advantageous mutations[52] [53] [54] .
In summary, it is generally accepted that the majority of mutations are neutral or deleterious, with rare mutations being advantageous; however, the proportion of types of mutations varies between species. This indicates two important points: first, the proportion of effectively neutral mutations is likely to vary between species, resulting from dependence on effective population size; second, the average effect of deleterious mutations varies dramatically between species[45] . In addition, the DFE also differs between coding regions and non-coding regions, with the DFE of non-coding DNA containing more weakly selected mutations[45] .
- A frameshift mutation is a mutation caused by insertion or deletion of a number of nucleotides that is not evenly divisible by three from a DNA sequence. Due to the triplet nature of gene expression by codons, the insertion or deletion can disrupt the reading frame, or the grouping of the codons, resulting in a completely different translation from the original.[55] The earlier in the sequence the deletion or insertion occurs, the more altered the protein produced is.
- In contrast, any insertion or deletion that is evenly divisible by three is termed an in-frame mutation
- A nonsense mutation is a point mutation in a sequence of DNA that results in a premature stop codon, or a nonsense codon in the transcribed mRNA, and possibly a truncated, and often nonfunctional protein product.
- Missense mutations or nonsynonymous mutations are types of point mutations where a single nucleotide is changed to cause substitution of a different amino acid. This in turn can render the resulting protein nonfunctional. Such mutations are responsible for diseases such as Epidermolysis bullosa, sickle-cell disease, and SOD1 mediated ALS (Boillée 2006, p. 39).
- A neutral mutation is a mutation that occurs in an amino acid codon which results in the use of a different, but chemically similar, amino acid. The similarity between the two is enough that little or no change is often rendered in the protein. For example, a change from AAA to AGA will encode arginine, a chemically similar molecule to the intended lysine.
- Silent mutations are mutations that do not result in a change to the amino acid sequence of a protein. They may occur in a region that does not code for a protein, or they may occur within a codon in a manner that does not alter the final amino acid sequence. The phrase silent mutation is often used interchangeably with the phrase synonymous mutation; however, synonymous mutations are a subcategory of the former, occurring only within exons. The name silent could be a misnomer. For example, a silent mutation in the exon/intron border may lead to alternative splicing by changing the splice site (see Splice site mutation), thereby leading to a changed protein. Silent mutations occur because of the degenerate nature of the genetic code.
A mutation has caused this garden
moss rose to produce flowers of different colors. This is a somatic mutation that may also be passed on in the germ line.
In multicellular organisms with dedicated reproductive cells, mutations can be subdivided into germ line mutations, which can be passed on to descendants through their reproductive cells, and somatic mutations (also called acquired mutations),[56] which involve cells outside the dedicated reproductive group and which are not usually transmitted to descendants.
A germline mutation gives rise to a constitutional mutation in the offspring, that is, a mutation that is present in every cell. A constitutional mutation can also occur very soon after fertilisation, or continue from a previous constitutional mutation in a parent.[57]
The distinction between germline and somatic mutations is important in animals that have a dedicated germ line to produce reproductive cells. However, it is of little value in understanding the effects of mutations in plants, which lack dedicated germ line. The distinction is also blurred in those animals that reproduce asexually through mechanisms such as budding, because the cells that give rise to the daughter organisms also give rise to that organisms germ line. A new mutation that was not inherited from either parent is called a de novo mutation.
Diploid organisms (e.g. human)contain two copies of each gene – a paternal and a maternal allele. Based on the occurrence of mutation on each chromosome, we may classify mutations into three types.
- A heterozygous mutation is a mutation of only one allele.
- A homozygous mutation is an identical mutation of both the paternal and maternal alleles.
- Compound heterozygous mutations or a genetic compound comprises two different mutations in the paternal and maternal alleles.[58]
A wildtype or homozygous non-mutated organism is one in which neither allele is mutated.
- Conditional mutation is a mutation that has wild-type (or less severe) phenotype under certain "permissive" environmental conditions and a mutant phenotype under certain "restrictive" conditions. For example, a temperature-sensitive mutation can cause cell death at high temperature (restrictive condition), but might have no deleterious consequences at a lower temperature (permissive condition).
A committee of the Human Genome Variation Society (HGVS) has developed the standard human sequence variant nomenclature,[59] which should be used by researchers and DNA diagnostic centers to generate unambiguous mutation descriptions. In principle, this nomenclature can also be used to describe mutations in other organisms. The nomenclature specifies the type of mutation and base or amino acid changes.
- Nucleotide substitution (e.g. 76A>T) – The number is the position of the nucleotide from the 5' end, the first letter represents the wild type nucleotide, and the second letter represents the nucleotide which replaced the wild type. In the given example, the adenine at the 76th position was replaced by a thymine.
- If it becomes necessary to differentiate between mutations in genomic DNA, mitochondrial DNA, and RNA, a simple convention is used. For example, if the 100th base of a nucleotide sequence mutated from G to C, then it would be written as g.100G>C if the mutation occurred in genomic DNA, m.100G>C if the mutation occurred in mitochondrial DNA, or r.100g>c if the mutation occurred in RNA. Note that for mutations in RNA, the nucleotide code is written in lower case.
- Amino acid substitution (e.g. D111E) – The first letter is the one letter code of the wild type amino acid, the number is the position of the amino acid from the N-terminus, and the second letter is the one letter code of the amino acid present in the mutation. Nonsense mutations are represented with an X for the second amino acid (e.g. D111X).
- Amino acid deletion (e.g. ΔF508) – The Greek letter Δ (delta) indicates a deletion. The letter refers to the amino acid present in the wild type and the number is the position from the N terminus of the amino acid were it to be present as in the wild type.
Changes in DNA caused by mutation can cause errors in protein sequence, creating partially or completely non-functional proteins. Each cell, in order to function correctly, depends on thousands of proteins to function in the right places at the right times. When a mutation alters a protein that plays a critical role in the body, a medical condition can result. A condition caused by mutations in one or more genes is called a genetic disorder. Some mutations alter a gene's DNA base sequence but do not change the function of the protein made by the gene. One study on the comparison of genes between different species of Drosophila suggests that if a mutation does change a protein, this will probably be harmful, with an estimated 70 percent of amino acid polymorphisms having damaging effects, and the remainder being either neutral or weakly beneficial.[4] However, studies in yeast have shown that only 7% of mutations that are not in genes are harmful.[60]
If a mutation is present in a germ cell, it can give rise to offspring that carries the mutation in all of its cells. This is the case in hereditary diseases. In particular, if there is a mutation in a DNA repair gene within a germ cell, humans carrying such germ-line mutations may have in increased risk of cancer, such as the list on Wikipedia of inherited human DNA repair gene mutations that increase cancer risk. On the other hand, a mutation may occur in a somatic cell of an organism. Such mutations will be present in all descendants of this cell within the same organism, and certain mutations can cause the cell to become malignant, and thus cause cancer.[61]
A DNA damage can cause an error when the the DNA is replicated, and this error of replication can cause a gene mutation that, in turn, could cause a genetic disorder. DNA damages are repaired by the DNA repair system of the cell. Each cell has a number of pathways through which enzymes recognize and repair damages in DNA. Because DNA can be damaged in many ways, the process of DNA repair is an important way in which the body protects itself from disease. Once a DNA damage has given rise to a mutation, the mutation cannot be repaired. DNA repair pathways can only recognize and act on "abnormal" structures in the DNA. Once a mutation occurs in a gene sequence it then has normal DNA structure and cannot be repaired.
Although mutations that change in protein sequences can be harmful to an organism; on occasions, the effect may be positive in a given environment. In this case, the mutation may enable the mutant organism to withstand particular environmental stresses better than wild-type organisms, or reproduce more quickly. In these cases a mutation will tend to become more common in a population through natural selection.
For example, a specific 32 base pair deletion in human CCR5 (CCR5-Δ32) confers HIV resistance to homozygotes and delays AIDS onset in heterozygotes.[62] The CCR5 mutation is more common in those of European descent. One possible explanation of the etiology of the relatively high frequency of CCR5-Δ32 in the European population is that it conferred resistance to the bubonic plague in mid-14th century Europe. People with this mutation were more likely to survive infection; thus its frequency in the population increased.[63] This theory could explain why this mutation is not found in southern Africa, where the bubonic plague never reached. A newer theory suggests that the selective pressure on the CCR5 Delta 32 mutation was caused by smallpox instead of the bubonic plague.[64]
Another example is Sickle cell disease, a blood disorder in which the body produces an abnormal type of the oxygen-carrying substance hemoglobin in the red blood cells. One-third of all indigenous inhabitants of Sub-Saharan Africa carry the gene,[65] because in areas where malaria is common, there is a survival value in carrying only a single sickle-cell gene (sickle cell trait).[66] Those with only one of the two alleles of the sickle-cell disease are more resistant to malaria, since the infestation of the malaria plasmodium is halted by the sickling of the cells which it infests.
Another research from Denmark concludes that blue-eyes are the mutated character of human eyes which were originally brown from around 6,000 to 10,000 years ago. The benign mutation actually effected the OAC2 gene which colorizes our hair and has other functions related to liver e.t.c. So all blue-eyed people share a common ancestor[67]
Prions are proteins and do not contain genetic material. However, prion replication has been shown to be subject to mutation and natural selection just like other forms of replication.[68]
Cells with heterozygous mutations (one good copy of gene and one mutated copy) may function normally with the unmutated copy until the good copy has been spontaneously somatically mutated. This kind of mutation happens all the time in living organisms, but it is difficult to measure the rate. Measuring this rate is important in predicting the rate at which people may develop cancer.[69]
Point mutations may arise from spontaneous mutations that occur during DNA replication. The rate of mutation may be increased by mutagens. Mutagens can be physical, such as radiation from UV rays, X-rays or extreme heat, or chemical (molecules that misplace base pairs or disrupt the helical shape of DNA). Mutagens associated with cancers are often studied to learn about cancer and its prevention.
- ^ a b Bertram J (2000). "The molecular biology of cancer". Mol. Aspects Med. 21 (6): 167–223. DOI:10.1016/S0098-2997(00)00007-8. PMID 11173079.
- ^ a b Aminetzach YT, Macpherson JM, Petrov DA (2005). "Pesticide resistance via transposition-mediated adaptive gene truncation in Drosophila". Science 309 (5735): 764–7. DOI:10.1126/science.1112699. PMID 16051794.
- ^ Burrus V, Waldor M (2004). "Shaping bacterial genomes with integrative and conjugative elements". Res. Microbiol. 155 (5): 376–86. DOI:10.1016/j.resmic.2004.01.012. PMID 15207870.
- ^ a b Sawyer SA, Parsch J, Zhang Z, Hartl DL (2007). "Prevalence of positive selection among nearly neutral amino acid replacements in Drosophila". Proc. Natl. Acad. Sci. U.S.A. 104 (16): 6504–10. DOI:10.1073/pnas.0701572104. PMC 1871816. PMID 17409186. //www.pubmedcentral.nih.gov/articlerender.fcgi?tool=pmcentrez&artid=1871816.
- ^ Hastings, P J; Lupski, JR; Rosenberg, SM; Ira, G (2009). "Mechanisms of change in gene copy number". Nature Reviews. Genetics 10 (8): 551–564. DOI:10.1038/nrg2593. PMC 2864001. PMID 19597530. //www.pubmedcentral.nih.gov/articlerender.fcgi?tool=pmcentrez&artid=2864001.
- ^ Carroll SB, Grenier J, Weatherbee SD (2005). From DNA to Diversity: Molecular Genetics and the Evolution of Animal Design. Second Edition. Oxford: Blackwell Publishing. ISBN 1-4051-1950-0.
- ^ Harrison P, Gerstein M (2002). "Studying genomes through the aeons: protein families, pseudogenes and proteome evolution". J Mol Biol 318 (5): 1155–74. DOI:10.1016/S0022-2836(02)00109-2. PMID 12083509.
- ^ Orengo CA, Thornton JM (2005). "Protein families and their evolution-a structural perspective". Annu. Rev. Biochem. 74: 867–900. DOI:10.1146/annurev.biochem.74.082803.133029. PMID 15954844.
- ^ Long M, Betrán E, Thornton K, Wang W (November 2003). "The origin of new genes: glimpses from the young and old". Nat. Rev. Genet. 4 (11): 865–75. DOI:10.1038/nrg1204. PMID 14634634.
- ^ Wang M, Caetano-Anollés G (2009). "The evolutionary mechanics of domain organization in proteomes and the rise of modularity in the protein world". Structure 17 (1): 66–78. DOI:10.1016/j.str.2008.11.008. PMID 19141283.
- ^ Bowmaker JK (1998). "Evolution of colour vision in vertebrates". Eye (London, England) 12 (Pt 3b): 541–7. DOI:10.1038/eye.1998.143. PMID 9775215.
- ^ Gregory TR, Hebert PD (1999). "The modulation of DNA content: proximate causes and ultimate consequences". Genome Res. 9 (4): 317–24. DOI:10.1101/gr.9.4.317 (inactive 2009-11-14). PMID 10207154. http://genome.cshlp.org/content/9/4/317.full.
- ^ Hurles M (July 2004). "Gene Duplication: The Genomic Trade in Spare Parts". PLoS Biol. 2 (7): E206. DOI:10.1371/journal.pbio.0020206. PMC 449868. PMID 15252449. //www.pubmedcentral.nih.gov/articlerender.fcgi?tool=pmcentrez&artid=449868.
- ^ Liu N, Okamura K, Tyler DM (2008). "The evolution and functional diversification of animal microRNA genes". Cell Res. 18 (10): 985–96. DOI:10.1038/cr.2008.278. PMC 2712117. PMID 18711447. http://www.nature.com/cr/journal/v18/n10/full/cr2008278a.html.
- ^ Siepel A (October 2009). "Darwinian alchemy: Human genes from noncoding DNA". Genome Res. 19 (10): 1693–5. DOI:10.1101/gr.098376.109. PMC 2765273. PMID 19797681. http://genome.cshlp.org/content/19/10/1693.full.
- ^ Zhang J, Wang X, Podlaha O (2004). "Testing the Chromosomal Speciation Hypothesis for Humans and Chimpanzees". Genome Res. 14 (5): 845–51. DOI:10.1101/gr.1891104. PMC 479111. PMID 15123584. //www.pubmedcentral.nih.gov/articlerender.fcgi?tool=pmcentrez&artid=479111.
- ^ Ayala FJ, Coluzzi M (2005). "Chromosome speciation: Humans, Drosophila, and mosquitoes". Proc. Natl. Acad. Sci. U.S.A. 102 (Suppl 1): 6535–42. DOI:10.1073/pnas.0501847102. PMC 1131864. PMID 15851677. http://www.pnas.org/content/102/suppl.1/6535.full.
- ^ Hurst GD, Werren JH (2001). "The role of selfish genetic elements in eukaryotic evolution". Nat. Rev. Genet. 2 (8): 597–606. DOI:10.1038/35084545. PMID 11483984.
- ^ Häsler J, Strub K (2006). "Alu elements as regulators of gene expression". Nucleic Acids Res. 34 (19): 5491–7. DOI:10.1093/nar/gkl706. PMC 1636486. PMID 17020921. //www.pubmedcentral.nih.gov/articlerender.fcgi?tool=pmcentrez&artid=1636486.
- ^ Eyre-Walker A, Keightley PD (August 2007). "The distribution of fitness effects of new mutations". Nature Reviews Genetics 8 (8): 610–8. DOI:10.1038/nrg2146. PMID 17637733. http://www.lifesci.sussex.ac.uk/home/Adam_Eyre-Walker/Website/Publications_files/EWNRG07.pdf.
- ^ "Mutation, Mutagens, and DNA Repair", by Beth A. Montelone, Ph. D., Division of Biology, Kansas State University, 1998
- ^ Created from PDB 1JDG
- ^ Pfohl-Leszkowicz A, Manderville RA (January 2007). "Ochratoxin A: An overview on toxicity and carcinogenicity in animals and humans". Mol Nutr Food Res 51 (1): 61–99. DOI:10.1002/mnfr.200600137. PMID 17195275.
- ^ Kozmin S, Slezak G, Reynaud-Angelin A, Elie C, de Rycke Y, Boiteux S, Sage E (September 2005). "UVA radiation is highly mutagenic in cells that are unable to repair 7,8-dihydro-8-oxoguanine in Saccharomyces cerevisiae". Proc. Natl. Acad. Sci. U.S.A. 102 (38): 13538–43. DOI:10.1073/pnas.0504497102. PMC 1224634. PMID 16157879. http://www.pnas.
- ^ References for the image are found in Wikimedia Commons page at: Commons:File:Notable mutations.svg#References.
- ^ Freese, Ernst (April 1959). "THE DIFFERENCE BETWEEN SPONTANEOUS AND BASE-ANALOGUE INDUCED MUTATIONS OF PHAGE T4". Proc. Natl. Acad. Sci. U.S.A. 45 (4): 622–33. DOI:10.1073/pnas.45.4.622. PMC 222607. PMID 16590424. //www.pubmedcentral.nih.gov/articlerender.fcgi?tool=pmcentrez&artid=222607.
- ^ Freese, Ernst (1959). "The Specific Mutagenic Effect of Base Analogues on Phage T4". J. Mol. Biol. 1 (2): 87–105. DOI:10.1016/S0022-2836(59)80038-3.
- ^ Ellis NA, Ciocci S, German J (2001). "Back mutation can produce phenotype reversion in Bloom syndrome somatic cells". Hum Genet 108 (2): 167–73. DOI:10.1007/s004390000447. PMID 11281456. http://link.springer.de/link/service/journals/00439/bibs/1108002/11080167.htm.
- ^ Charlesworth, D; Charlesworth B, Morgan M T (1995). "The pattern of neutral molecular variation under the background selection model.". Genetics 141 (4): 1619–32. PMC 1206892. PMID 8601499. http://www.genetics.org/content/141/4/1619.long.
- ^ Loewe, L (2006). "Quantifying the genomic decay paradox due to Muller's ratchet in human mitochondrial DNA.". Genet Res 87 (2): 133-59. DOI:10.1017/S0016672306008123. PMID 16709275. http://journals.cambridge.org/action/displayAbstract?fromPage=online&aid=439711.
- ^ Peck, J R; Barreau G, Heath S C (1997). "Imperfect genes, Fisherian mutation and the evolution of sex.". Genetics 145 (4): 1171-99. PMC 1207886. PMID 9093868. http://www.genetics.org/content/145/4/1171.long.
- ^ Keightley, P.D.; Lynch M (2003). "Toward a realistic model of mutations affecting fitness.". Evolution 57 (3): 683-689. PMID 12703958. http://www.jstor.org/discover/10.2307/3094781?uid=3739920&uid=2&uid=4&uid=3739256&sid=56088268663.
- ^ Barton, N.H.; Keightley P.D. (2002). "Understanding quantitative genetic variation.". Nat Rev Genet 3 (1): 11-21. DOI:10.1038/nrg700. PMID 11823787.
- ^ a b c Sanjuan, R; Moya A, Elena S F (2004). "The distribution of fitness effects caused by single-nucleotide substitutions in an RNA virus.". Proc Natl Acad Sci U S A 101 (22): 8396-401. DOI:10.1073/pnas.0400146101. PMID 15159545. http://www.pnas.org/content/101/22/8396.long.
- ^ Carrasco, P; de la Iglesia F, Elena S F (2007). "Distribution of fitness and virulence effects caused by single-nucleotide substitutions in Tobacco Etch virus.". J Virol 81 (23): 12979-84. DOI:10.1128/JVI.00524-07. PMC 2169111. PMID 17898073. //www.pubmedcentral.nih.gov/articlerender.fcgi?tool=pmcentrez&artid=2169111.
- ^ Sanjuan, R (2010). "Mutational fitness effects in RNA and single-stranded DNA viruses: common patterns revealed by site-directed mutagenesis studies.". Philos Trans R Soc Lond B Biol Sci 365 (1548): 1975-82. DOI:10.1098/rstb.2010.0063. PMID 20478892. http://rstb.royalsocietypublishing.org/content/365/1548/1975.long.
- ^ Peris, J.B.; Davis P, Cuevas J M, Nebot M R, Sanjuan R (2010). "Distribution of fitness effects caused by single-nucleotide substitutions in bacteriophage f1.". Genetics 185 (2): 603-9. DOI:10.1534/genetics.110.115162. PMID 20382832. http://www.genetics.org/content/185/2/603.long.
- ^ Elena, S F; Ekunwe L, Hajela N, Oden S A, Lenski R E (1998). "Distribution of fitness effects caused by random insertion mutations in Escherichia coli.". Genetica 102-103 (1-6): 349-58. DOI:10.1023/A:1017031008316. PMID 9720287.
- ^ a b Hietpas, R.T.; Jensen J D, Bolon D N, (2011). "Experimental illumination of a fitness landscape.". Proc Natl Acad Sci U S A 108 (19): 7896-901. DOI:10.1073/pnas.1016024108. PMID 21464309. http://www.pnas.org/content/108/19/7896.long.
- ^ Davies, E K; Peters A D, Keightley P D (1999). "High frequency of cryptic deleterious mutations in Caenorhabditis elegans.". Science 285 (5434): 1748-51. PMID 10481013.
- ^ Loewe, L; Charlesworth B (2006). "Inferring the distribution of mutational effects on fitness in Drosophila.". Biol Lett 2 (3): 426-30. DOI:10.1098/rsbl.2006.0481. PMID 17148422. http://rsbl.royalsocietypublishing.org/content/2/3/426.long.
- ^ Eyre-Walker, A; Woolfit M, Phelps T (2006). "The distribution of fitness effects of new deleterious amino acid mutations in humans.". Genetics 173 (2): 891-900. DOI:10.1534/genetics.106.057570. PMC 1526495. PMID 16547091. http://www.genetics.org/content/173/2/891.long.
- ^ Sawyer, S A; Kulathinal R J, Bustamante C D, Hartl D L (2003). "Bayesian analysis suggests that most amino acid replacements in Drosophila are driven by positive selection.". J Mol Evol 57: S154-64. DOI:10.1007/s00239-003-0022-3. PMID 15008412. http://www.springerlink.com/content/qajqamkgllcqubgm/.
- ^ Piganeau, G; Eyre-Walker A (2003). "Estimating the distribution of fitness effects from DNA sequence data: implications for the molecular clock.". Proc Natl Acad Sci U S A 100 (18): 10335-40. DOI:10.1073/pnas.1833064100. PMID 12925735. http://www.pnas.org/content/100/18/10335.long.
- ^ a b c Eyre-Walker, A; P.D. Keightley (2007). "The distribution of fitness effects of new mutations". Nature Reviews Genetics 8 (8): 610-618. DOI:10.1038/nrg2146. PMID 17637733.
- ^ Kimura, M (1968). "Evolutionary rate at the molecular level.". Nature 217 (5129): 624-6. PMID 5637732.
- ^ Kimura, Motoo (1983). The neutral theory of molecular evolution. Cambridge University Press,. pp. 367. ISBN 82022225.
- ^ Akashi, H (1999). "Within- and between-species DNA sequence variation and the 'footprint' of natural selection.". Gene 238 (1): 39-51. DOI:10.1016/S0378-1119(99)00294-2. PMID 10570982.
- ^ Eyre-Walker, A (2006). "The genomic rate of adaptive evolution.". Trends Ecol Evol 21 (10): 569-75. DOI:10.1016/j.tree.2006.06.015. PMID 16820244.
- ^ Gillespie, J.H. (1984). "Molecular evolution over the mutational landscape.". Evolution 38 (5). DOI:10.2307/2408444.
- ^ Orr, H.A. (2003). "The distribution of fitness effects among beneficial mutations.". Genetics 163 (4): 1519-26. PMC 1462510. PMID 12702694. http://www.genetics.org/content/163/4/1519.long.
- ^ Kassen, R; Bataillon T (2006). "Distribution of fitness effects among beneficial mutations before selection in experimental populations of bacteria.". Nat Genet 38 (4): 484-8. DOI:10.1038/ng1751. PMID 16550173.
- ^ Rokyta, d.R.; Joyce P, Caudle S B, Wichman H A (2005). "An empirical test of the mutational landscape model of adaptation using a single-stranded DNA virus.". Nat Genet 37 (4): 441-4. DOI:10.1038/ng1535. PMID 15778707.
- ^ Imhof, M; Schlotterer C (2001). "Fitness effects of advantageous mutations in evolving Escherichia coli populations.". Proc Natl Acad Sci U S A 98 (3): 1113-7. DOI:10.1073/pnas.98.3.1113. PMC 14717. PMID 11158603. http://www.pnas.org/content/98/3/1113.long.
- ^ C.Michael Hogan. 2010. Mutation. ed. E.Monosson and C.J.Cleveland. Encyclopedia of Earth. National Council for Science and the Environment. Washington DC
- ^ "Genome Dictionary". http://www.theodora.com/genetics/#somaticcellgeneticmutation. Retrieved 2010-06-06. .
- ^ RB1 Genetics at Daisy's Eye Cancer Fund. Retrieved May 2011
- ^ Medterms.com
- ^ Den Dunnen, Johan T.; Antonarakis, Stylianos E. (2000). "Mutation Nomenclature Extensions and Suggestions to Describe Complex Mutations: A Discussion". Human Mutation 15 (1): 7–12. DOI:10.1002/(SICI)1098-1004(200001)15:1<7::AID-HUMU4>3.0.CO;2-N. PMID 10612815.
- ^ Doniger SW, Kim HS, Swain D, et al. (August 2008). Pritchard, Jonathan K.. ed. "A Catalog of Neutral and Deleterious Polymorphism in Yeast". PLoS Genet. 4 (8): e1000183. DOI:10.1371/journal.pgen.1000183. PMC 2515631. PMID 18769710. //www.pubmedcentral.nih.gov/articlerender.fcgi?tool=pmcentrez&artid=2515631.
- ^ Ionov Y, Peinado MA, Malkhosyan S, Shibata D, Perucho M (1993). "Ubiquitous somatic mutations in simple repeated sequences reveal a new mechanism for colonic carcinogenesis". Nature 363 (6429): 558–61. DOI:10.1038/363558a0. PMID 8505985.
- ^ Sullivan, Amy D. et al. (2001). "The coreceptor mutation CCR5Δ32 influences the dynamics of HIV epidemics and is selected for by HIV". PNAS 95 (18): 10214–10219. DOI:10.1073/pnas.181325198. PMC 56941. PMID 11517319. http://www.pnas.org/content/98/18/10214.full.
- ^ "PBS:Secrets of the Dead. Case File: Mystery of the Black Death". http://www.pbs.org/wnet/secrets/previous_seasons/case_plague/clues.html.
- ^ Galvani A, Slatkin M (2003). "Evaluating plague and smallpox as historical selective pressures for the CCR5-Δ32 HIV-resistance allele". Proc Natl Acad Sci USA 100 (25): 15276–9. DOI:10.1073/pnas.2435085100. PMC 299980. PMID 14645720. //www.pubmedcentral.nih.gov/articlerender.fcgi?tool=pmcentrez&artid=299980.
- ^ Sicklecell.md
- ^ Sicklecell.md FAQ: "Why is Sickle Cell Anaemia only found in Black people?
- ^ http://www.areyouamazed.com/all-blue-eyed-people-share-the-same-ancestors
- ^ 'Lifeless' prion proteins are 'capable of evolution'
- ^ "A quantitative measurement of the human somatic mutation rate", by Araten DJ, et al, Cancer Res. 2005 Sep 15;65(18):8111-7.; erratum in Cancer Res. 2005 Nov 15;65(22):10635
Mutation
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Mechanisms of mutation |
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Mutation with respect to structure |
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Mutation with respect to overall fitness |
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