Human mitochondrial genetics
Human mitochondrial genetics is the study of the genetics of human mitochondrial DNA. The human mitochondrial genome is the entirety of hereditary information contained in human mitochondria. Mitochondria are small structures in cells that generate energy for the cell to use, and are hence referred to as the "powerhouses" of the cell.
Mitochondrial DNA is not transmitted through nuclear DNA. In humans, as in most multicellular organisms, mitochondrial DNA is inherited only from the mother's ovum. There are theories, however, that paternal mtDNA transmission in humans can occur under certain circumstances.
Mitochondrial inheritance is therefore non-Mendelian, as Mendelian inheritance presumes that half the genetic material of a fertilized egg derives from each parent.
Eighty percent of mitochondrial DNA codes for mitochondrial RNA, and therefore most mitochondrial DNA mutations lead to functional problems, which may be manifested as muscle disorders.
Because they provide 30 molecules of ATP per glucose molecule in contrast to the 2 ATP molecules produced by glycolysis, mitochondria are essential to all higher organisms for sustaining life. The mitochondrial diseases are genetic disorders carried in mitochondrial DNA, or nuclear DNA coding for mitochondrial components. Slight problems with any one of the numerous enzymes used by the mitochondria can be devastating to the cell, and in turn, to the organism.
Quantity
In humans, mitochondrial DNA forms closed circular molecules that contain 16,569 DNA base pairs, with each such molecule normally containing a full set of the mitochondrial genes. Each human mitochondrion contains, on average, approximately 5 such mtDNA molecules, with the quantity ranging between 1 and 15. Each human cell contains approximately 100 mitochondria, giving a total number of mtDNA molecules per human cell of approximately 500.Inheritance patterns
Because mitochondrial diseases can be inherited both maternally and through chromosomal inheritance, the way in which they are passed on from generation to generation can vary greatly depending on the disease. Mitochondrial genetic mutations that occur in the nuclear DNA can occur in any of the chromosomes. Mutations inherited through the chromosomes can be autosomal dominant or recessive and can also be sex-linked dominant or recessive. Chromosomal inheritance follows normal Mendelian laws, despite the fact that the phenotype of the disease may be masked.Because of the complex ways in which mitochondrial and nuclear DNA "communicate" and interact, even seemingly simple inheritance is hard to diagnose. A mutation in chromosomal DNA may change a protein that regulates the production of another certain protein in the mitochondria or the cytoplasm; this may lead to slight, if any, noticeable symptoms. On the other hand, some devastating mtDNA mutations are easy to diagnose because of their widespread damage to muscular, neural, and/or hepatic tissues and because they are present in the mother and all the offspring.
The number of affected mtDNA molecules inherited by a specific offspring can vary greatly because
- the mitochondria within the fertilized oocyte is what the new life will have to begin with,
- the number of affected mitochondria varies from cell to cell depending both on the number it inherited from its mother cell and environmental factors which may favor mutant or wildtype mitochondrial DNA,
- the number of mtDNA molecules in the mitochondria varies from around two to ten.
Genes
Genes in the human mitochondrial genome are as follows.Electron transport chain, and humanin
It was originally incorrectly believed that the mitochondrial genome contained only 13 protein-coding genes, all of them encoding proteins of the electron transport chain. However, in 2001, a 14th biologically active protein called humanin was discovered, and was found to be encoded by the mitochondrial gene MT-RNR2 which also encodes part of the mitochondrial ribosome :| Complex number | Category | Genes | Positions in the mitogenome | Strand |
| I | NADH dehydrogenase | - | - | - |
| I | NADH dehydrogenase | MT-ND1 | 3,307–4,262 | L |
| I | NADH dehydrogenase | MT-ND2 | 4,470–5,511 | L |
| I | NADH dehydrogenase | MT-ND3 | 10,059–10,404 | L |
| I | NADH dehydrogenase | MT-ND4L | 10,470–10,766 | L |
| I | NADH dehydrogenase | MT-ND4 | 10,760–12,137 | L |
| I | NADH dehydrogenase | MT-ND5 | 12,337–14,148 | L |
| I | NADH dehydrogenase | MT-ND6 | 14,149–14,673 | H |
| III | Coenzyme Q - cytochrome c reductase / Cytochrome b | MT-CYB | 14,747–15,887 | L |
| IV | Cytochrome c oxidase | MT-CO1 | 5,904–7,445 | L |
| IV | Cytochrome c oxidase | MT-CO2 | 7,586–8,269 | L |
| IV | Cytochrome c oxidase | MT-CO3 | 9,207–9,990 | L |
| V | ATP synthase | MT-ATP6 | 8,527–9,207 | L |
| V | ATP synthase | MT-ATP8 | 8,366–8,572 | L |
| — | Humanin | MT-RNR2 | — | — |
Unlike the other proteins, humanin does not remain in the mitochondria, and interacts with the rest of the cell and cellular receptors. Humanin can protect brain cells by inhibiting apoptosis. Despite its name, versions of humanin also exist in other animals, such as rattin in rats.
rRNA
The following genes encode rRNAs:| Subunit | rRNA | Genes | Positions in the mitogenome | Strand |
| Small | 12S | MT-RNR1 | 648–1,601 | L |
| Large | 16S | MT-RNR2 | 1,671–3,229 | L |
tRNA
The following genes encode tRNAs:| Amino Acid | 3-Letter | 1-Letter | MT DNA | Positions | Strand |
| Alanine | Ala | A | MT-TA | 5,587–5,655 | H |
| Arginine | Arg | R | MT-TR | 10,405–10,469 | L |
| Asparagine | Asn | N | MT-TN | 5,657–5,729 | H |
| Aspartic acid | Asp | D | MT-TD | 7,518–7,585 | L |
| Cysteine | Cys | C | MT-TC | 5,761–5,826 | H |
| Glutamic acid | Glu | E | MT-TE | 14,674–14,742 | H |
| Glutamine | Gln | Q | MT-TQ | 4,329–4,400 | H |
| Glycine | Gly | G | MT-TG | 9,991–10,058 | L |
| Histidine | His | H | MT-TH | 12,138–12,206 | L |
| Isoleucine | Ile | I | MT-TI | 4,263–4,331 | L |
| Leucine | Leu | L | MT-TL1 | 3,230–3,304 | L |
| Leucine | Leu | L | MT-TL2 | 12,266–12,336 | L |
| Lysine | Lys | K | MT-TK | 8,295–8,364 | L |
| Methionine | Met | M | MT-TM | 4,402–4,469 | L |
| Phenylalanine | Phe | F | MT-TF | 577–647 | L |
| Proline | Pro | P | MT-TP | 15,956–16,023 | H |
| Serine | Ser | S | MT-TS1 | 7,446–7,514 | H |
| Serine | Ser | S | MT-TS2 | 12,207–12,265 | L |
| Threonine | Thr | T | MT-TT | 15,888–15,953 | L |
| Tryptophan | Trp | W | MT-TW | 5,512–5,579 | L |
| Tyrosine | Tyr | Y | MT-TY | 5,826–5,891 | H |
| Valine | Val | V | MT-TV | 1,602–1,670 | L |
Location of genes
Mitochondrial DNA traditionally had the two strands of DNA designated the heavy and the light strand, due to their buoyant densities during separation in cesium chloride gradients, which was found to be related to the relative G+T nucleotide content of the strand. However, confusion of labeling of this strands is widespread, and appears to originate with an identification of the majority coding strand as the heavy in one influential article in 1999. In humans, the light strand of mtDNA carries 28 genes and the heavy strand of mtDNA carries only 9 genes. Eight of the 9 genes on the heavy strand code for mitochondrial tRNA molecules. Human mtDNA consists of 16,569 nucleotide pairs. The entire molecule is regulated by only one regulatory region which contains the origins of replication of both heavy and light strands. The entire human mitochondrial DNA molecule has been mapped.Genetic code variants
The genetic code is, for the most part, universal, with few exceptions: mitochondrial genetics includes some of these. For most organisms the "stop codons" are "UAA", "UAG", and "UGA". In vertebrate mitochondria "AGA" and "AGG" are also stop codons, but not "UGA", which codes for tryptophan instead. "AUA" codes for isoleucine in most organisms but for methionine in vertebrate mitochondrial mRNA.There are many other variations among the codes used by other mitochondrial m/tRNA, which happened not to be harmful to their organisms, and which can be used as a tool to determine relative proximity of common ancestry of related species. .
Using these techniques, it is estimated that the first mitochondria arose around 1.5 billion years ago. A generally accepted hypothesis is that mitochondria originated as an aerobic prokaryote in a symbiotic relationship within an anaerobic eukaryote.
Replication, repair, transcription, and translation
Mitochondrial replication is controlled by nuclear genes and is specifically suited to make as many mitochondria as that particular cell needs at the time.Mitochondrial transcription in humans is initiated from three promoters, H1, H2, and L. The H2 promoter transcribes almost the entire heavy strand and the L promoter transcribes the entire light strand. The H1 promoter causes the transcription of the two mitochondrial rRNA molecules.
When transcription takes place on the heavy strand a polycistronic transcript is created. The light strand produces either small transcripts, which can be used as primers, or one long transcript. The production of primers occurs by processing of light strand transcripts with the Mitochondrial RNase MRP. The requirement of transcription to produce primers links the process of transcription to mtDNA replication. Full length transcripts are cut into functional tRNA, rRNA, and mRNA molecules.
The process of transcription initiation in mitochondria involves three types of proteins: the mitochondrial RNA polymerase, mitochondrial transcription factor A, and mitochondrial transcription factors B1 and B2. POLRMT, TFAM, and TFB1M or TFB2M assemble at the mitochondrial promoters and begin transcription. The actual molecular events that are involved in initiation are unknown, but these factors make up the basal transcription machinery and have been shown to function in vitro.
Mitochondrial translation is still not very well understood. In vitro translations have still not been successful, probably due to the difficulty of isolating sufficient mt mRNA, functional mt rRNA, and possibly because of the complicated changes that the mRNA undergoes before it is translated.
Mitochondrial DNA polymerase
The Mitochondrial DNA Polymerase is used in the copying of mtDNA during replication. Because the two strands on the circular mtDNA molecule have different origins of replication, it replicates in a D-loop mode. One strand begins to replicate first, displacing the other strand. This continues until replication reaches the origin of replication on the other strand, at which point the other strand begins replicating in the opposite direction. This results in two new mtDNA molecules. Each mitochondrion has several copies of the mtDNA molecule and the number of mtDNA molecules is a limiting factor in mitochondrial fission. After the mitochondrion has enough mtDNA, membrane area, and membrane proteins, it can undergo fission to become two mitochondria. Evidence suggests that mitochondria can also undergo fusion and exchange genetic material among each other. Mitochondria sometimes form large matrices in which fusion, fission, and protein exchanges are constantly occurring. mtDNA shared among mitochondria.Damage and transcription error
Mitochondrial DNA is susceptible to damage from free oxygen radicals from mistakes that occur during the production of ATP through the electron transport chain. These mistakes can be caused by genetic disorders, cancer, and temperature variations. These radicals can damage mtDNA molecules or change them, making it hard for mitochondrial polymerase to replicate them. Both cases can lead to deletions, rearrangements, and other mutations. Recent evidence has suggested that mitochondria have enzymes that proofread mtDNA and fix mutations that may occur due to free radicals. It is believed that a DNA recombinase found in mammalian cells is also involved in a repairing recombination process. Deletions and mutations due to free radicals have been associated with the aging process. It is believed that radicals cause mutations which lead to mutant proteins, which in turn led to more radicals. This process takes many years and is associated with some aging processes involved in oxygen-dependent tissues such as brain, heart, muscle, and kidney. Auto-enhancing processes such as these are possible causes of degenerative diseases including Parkinson's, Alzheimer's, and coronary artery disease.Chromosomally mediated mtDNA replication errors
Because mitochondrial growth and fission are mediated by the nuclear DNA, mutations in nuclear DNA can have a wide array of effects on mtDNA replication. Despite the fact that the loci for some of these mutations have been found on human chromosomes, specific genes and proteins involved have not yet been isolated. Mitochondria need a certain protein to undergo fission. If this protein is not present, the mitochondria grow but they do not divide. This leads to giant, inefficient mitochondria. Mistakes in chromosomal genes or their products can also affect mitochondrial replication more directly by inhibiting mitochondrial polymerase and can even cause mutations in the mtDNA directly and indirectly. Indirect mutations are most often caused by radicals created by defective proteins made from nuclear DNA.Mitochondrial diseases
Contribution of mitochondrial versus nuclear genome
In total, the mitochondrion hosts about 3000 different types of proteins, but only about 13 of them are coded on the mitochondrial DNA. Most of the 3000 types of proteins are involved in a variety of processes other than ATP production, such as porphyrin synthesis. Only about 3% of them code for ATP production proteins. This means most of the genetic information coding for the protein makeup of mitochondria is in chromosomal DNA and is involved in processes other than ATP synthesis. This increases the chances that a mutation that will affect a mitochondrion will occur in chromosomal DNA, which is inherited in a Mendelian pattern. Another result is that a chromosomal mutation will affect a specific tissue due to its specific needs, whether those may be high energy requirements or a need for the catabolism or anabolism of a specific neurotransmitter or nucleic acid. Because several copies of the mitochondrial genome are carried by each mitochondrion, mitochondrial mutations can be inherited maternally by mtDNA mutations which are present in mitochondria inside the oocyte before fertilization, or through mutations in the chromosomes.Presentation
s range in severity from asymptomatic to fatal, and are most commonly due to inherited rather than acquired mutations of mitochondrial DNA. A given mitochondrial mutation can cause various diseases depending on the severity of the problem in the mitochondria and the tissue the affected mitochondria are in. Conversely, several different mutations may present themselves as the same disease. This almost patient-specific characterization of mitochondrial diseases makes them very hard to accurately recognize, diagnose and trace. Some diseases are observable at or even before birth while others do not show themselves until late adulthood. This is because the number of mutant versus wildtype mitochondria varies between cells and tissues, and is continuously changing. Because cells have multiple mitochondria, different mitochondria in the same cell can have different variations of the mtDNA. This condition is referred to as heteroplasmy. When a certain tissue reaches a certain ratio of mutant versus wildtype mitochondria, a disease will present itself. The ratio varies from person to person and tissue to tissue. Mitochondrial diseases are very numerous and different. Apart from diseases caused by abnormalities in mitochondrial DNA, many diseases are suspected to be associated in part by mitochondrial dysfunctions, such as diabetes mellitus, forms of cancer and cardiovascular disease, lactic acidosis, specific forms of myopathy, osteoporosis, Alzheimer's disease, Parkinsons's disease, stroke, male infertility and which are also believed to play a role in the aging process.Use in forensics
Human mtDNA can also be used to help identify individuals. Forensic laboratories occasionally use mtDNA comparison to identify human remains, and especially to identify older unidentified skeletal remains. Although unlike nuclear DNA, mtDNA is not specific to one individual, it can be used in combination with other evidence to establish identification. mtDNA is also used to exclude possible matches between missing persons and unidentified remains. Many researchers believe that mtDNA is better suited to identification of older skeletal remains than nuclear DNA because the greater number of copies of mtDNA per cell increases the chance of obtaining a useful sample, and because a match with a living relative is possible even if numerous maternal generations separate the two.Examples
outlaw Jesse James's remains were identified using a comparison between mtDNA extracted from his remains and the mtDNA of the son of the female-line great-granddaughter of his sister.Similarly, the remains of Alexandra Feodorovna, last Empress of Russia, and her children were identified by comparison of their mitochondrial DNA with that of Prince Philip, Duke of Edinburgh, whose maternal grandmother was Alexandra's sister Victoria of Hesse.
Similarly to identify Emperor Nicholas II remains his mitochondrial DNA was compared with that of James Carnegie, 3rd Duke of Fife, whose maternal great-grandmother Alexandra of Denmark was sister of Nicholas II mother Dagmar of Denmark.
Similarly the remains of king Richard III.