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Friday, September 5, 2014

Gene

Gene

From Wikipedia, the free encyclopedia

A gene is the molecular unit of heredity of a living organism. It is used extensively by the scientific community as a name given to some stretches of deoxyribonucleic acids (DNA) and ribonucleic acids (RNA) that code for a polypeptide or for an RNA chain that has a function in the organism. Living beings depend on genes, as they specify all proteins and functional RNA chains. Genes hold the information to build and maintain an organism's cells and pass genetic traits to offspring. All organisms have genes corresponding to various biological traits, some of which are instantly visible, such as eye color or number of limbs, and some of which are not, such as blood type, increased risk for specific diseases, or the thousands of basic biochemical processes that comprise life. The word gene is derived from the Greek word genesis meaning "birth", or genos meaning "origin" (see pangenesis).
The chemical structure of a four-base fragment of a DNA double helix.

A modern working definition of a gene is "a locatable region of genomic sequence, corresponding to a unit of inheritance, which is associated with regulatory regions, transcribed regions, and or other functional sequence regions ".[1][2] Colloquial usage of the term gene (e.g. "good genes", "hair color gene") may actually refer to an allele: a gene is the basic instruction— a sequence of nucleic acids (DNA or, in the case of certain viruses RNA), while an allele is one variant of that gene. Thus, when the mainstream press refers to "having" a "gene" for a specific trait, this is customarily inaccurate. In most cases, all people would have a gene for the trait in question, although certain people will have a specific allele of that gene, which results in the trait variant. Further, genes code for proteins, which might result in identifiable traits, but it is the gene (genotype), not the trait (phenotype), which is inherited.

Big genes are a class of genes whose nuclear transcript spans 500 kb (1 kb = 1,000 base pairs) or more of chromosomal DNA. The largest of the big genes is the gene for dystrophin, which spans 2.3 Mb. Many big genes have modestly sized mRNAs; the exons encoding these RNAs typically encompass about 1% of the total chromosomal gene region in which they occur.

Physical definitions

RNA genes and genomes in the world

When proteins are manufactured, the gene is first copied into RNA as an intermediate product. In other cases, the RNA molecules are the actual functional products. For example, RNAs known as ribozymes are capable of enzymatic function, and microRNA has a regulatory role. The DNA sequences from which such RNAs are transcribed are known as RNA genes.

Some viruses store their entire genomes in the form of RNA, and contain no DNA at all. Because they use RNA to store genes, their cellular hosts may synthesize their proteins as soon as they are infected and without the delay in waiting for transcription. On the other hand, RNA retroviruses, such as HIV, require the reverse transcription of their genome from RNA into DNA before their proteins can be synthesized. In 2006, French researchers came across a puzzling example of RNA-mediated inheritance in mice. Mice with a loss-of-function mutation in the gene Kit have white tails. Offspring of these mutants can have white tails despite having only normal Kit genes. The research team traced this effect back to mutated Kit RNA.[3] While RNA is common as genetic storage material in viruses, in mammals in particular RNA inheritance has been observed very rarely.

Functional structure of a gene

Diagram of the "typical" eukaryotic protein-coding gene. Promoters and enhancers determine what portions of the DNA will be transcribed into the precursor mRNA (pre-mRNA). The pre-mRNA is then spliced into messenger RNA (mRNA) which is later translated into protein.

The vast majority of living organisms encode their genes in long strands of DNA (deoxyribonucleic acid). DNA consists of a chain made from four types of nucleotide subunits, each composed of: a five-carbon sugar (2'-deoxyribose), a phosphate group, and one of the four bases adenine, cytosine, guanine, and thymine. The most common form of DNA in a cell is in a double helix structure, in which two individual DNA strands twist around each other in a right-handed spiral. In this structure, the base pairing rules specify that guanine pairs with cytosine and adenine pairs with thymine. The base pairing between guanine and cytosine forms three hydrogen bonds, whereas the base pairing between adenine and thymine forms two hydrogen bonds. The two strands in a double helix must therefore be complementary, that is, their bases must align such that the adenines of one strand are paired with the thymines of the other strand, and so on.

Due to the chemical composition of the pentose residues of the bases, DNA strands have directionality. One end of a DNA polymer contains an exposed hydroxyl group on the deoxyribose; this is known as the 3' end of the molecule. The other end contains an exposed phosphate group; this is the 5' end. The directionality of DNA is vitally important to many cellular processes, since double helices are necessarily directional (a strand running 5'-3' pairs with a complementary strand running 3'-5'), and processes such as DNA replication occur in only one direction. All nucleic acid synthesis in a cell occurs in the 5'-3' direction, because new monomers are added via a dehydration reaction that uses the exposed 3' hydroxyl as a nucleophile.

The expression of genes encoded in DNA begins by transcribing the gene into RNA, a second type of nucleic acid that is very similar to DNA, but whose monomers contain the sugar ribose rather than deoxyribose. RNA also contains the base uracil in place of thymine. RNA molecules are less stable than DNA and are typically single-stranded. Genes that encode proteins are composed of a series of three-nucleotide sequences called codons, which serve as the words in the genetic language. The genetic code specifies the correspondence during protein translation between codons and amino acids. The genetic code is nearly the same for all known organisms.

All genes have regulatory regions in addition to regions that explicitly code for a protein or RNA product. A regulatory region shared by almost all genes is known as the promoter, which provides a position that is recognized by the transcription machinery when a gene is about to be transcribed and expressed. A gene can have more than one promoter, resulting in RNAs that differ in how far they extend in the 5' end.[4] Although promoter regions have a consensus sequence that is the most common sequence at this position, some genes have "strong" promoters that bind the transcription machinery well, and others have "weak" promoters that bind poorly. These weak promoters usually permit a lower rate of transcription than the strong promoters, because the transcription machinery binds to them and initiates transcription less frequently. Other possible regulatory regions include enhancers, which can compensate for a weak promoter. Most regulatory regions are "upstream"—that is, before or toward the 5' end of the transcription initiation site. Eukaryotic promoter regions are much more complex and difficult to identify than prokaryotic promoters.

Many prokaryotic genes are organized into operons, or groups of genes whose products have related functions and which are transcribed as a unit. By contrast, eukaryotic genes are transcribed only one at a time, but may include long stretches of DNA called introns which are transcribed but never translated into protein (they are spliced out before translation). Splicing can also occur in prokaryotic genes, but is less common than in eukaryotes.[5]

Chromosomes

The total complement of genes in an organism or cell is known as its genome, which may be stored on one or more chromosomes; the region of the chromosome at which a particular gene is located is called its locus. A chromosome consists of a single, very long DNA helix on which thousands of genes are encoded. Prokaryotesbacteria and archaea—typically store their genomes on a single large,circular chromosome, sometimes supplemented by additional small circles of DNA called plasmids, which usually encode only a few genes and are easily transferable between individuals. For example, the genes for antibiotic resistance are usually encoded on bacterial plasmids and can be passed between individual cells, even those of different species, via horizontal gene transfer.
Although some simple eukaryotes also possess plasmids with small numbers of genes, the majority of eukaryotic genes are stored on multiple linear chromosomes, which are packed within the nucleus in complex with storage proteins called histones. The manner in which DNA is stored on the histone, as well as chemical modifications of the histone itself, are regulatory mechanisms governing whether a particular region of DNA is accessible for gene expression. The ends of eukaryotic chromosomes are capped by long stretches of repetitive sequences called telomeres, which do not code for any gene product but are present to prevent degradation of coding and regulatory regions during DNA replication. The length of the telomeres tends to decrease each time the genome is replicated in preparation for cell division; the loss of telomeres has been proposed as an explanation for cellular senescence, or the loss of the ability to divide, and by extension for the aging process in organisms.[6]

Whereas the chromosomes of prokaryotes are relatively gene-dense, those of eukaryotes often contain so-called "junk DNA", or regions of DNA that serve no obvious function. Simple single-celled eukaryotes have relatively small amounts of such DNA, whereas the genomes of complex multicellular organisms, including humans, contain an absolute majority of DNA without an identified function.[7] However it now appears that, although protein-coding DNA makes up barely 2% of the human genome, about 80% of the bases in the genome may be expressed, so the term "junk DNA" may be a misnomer.[2]

Gene expression

In all organisms, there are two major steps separating a protein-coding gene from its protein: First, the DNA on which the gene resides must be transcribed from DNA to messenger RNA (mRNA); and, second, it must be translated from mRNA to protein. RNA-coding genes must still go through the first step, but are not translated into protein. The process of producing a biologically functional molecule of either RNA or protein is called gene expression, and the resulting molecule itself is called a gene product.

Genetic code

Schematic diagram of a single-stranded RNA molecule illustrating the position of three-base codons.

The genetic code is the set of rules by which information encoded within a gene is translated into a functional protein. Each gene consists of a specific sequence of nucleotides encoded in DNA or RNA. The nucleotide being made up of a sugar, a phosphate molecule and a specific base (adenine, thymine, cytosine, guanine or sometimes uracil [thymine is replaced with uracil in some viruses[8]]); a correspondence between nucleotides, the basic building blocks of genetic material, and amino acids, the basic building blocks of proteins, must be established for genes to be successfully translated into functional proteins. Sets of three nucleotides, known as codons, each correspond to a specific amino acid or to a signal; three codons are known as "stop codons" and, instead of specifying a new amino acid, alert the translation machinery that the end of the gene has been reached, just as a specific set of 3 bases, "AUG", known as the "start codon", signifies the gene to start transcribing. There are 64 possible codons (four possible nucleotides at each of three positions, hence 43 possible codons) and only 20 standard amino acids; hence the code is redundant and multiple codons can specify the same amino acid. The correspondence between codons and amino acids is nearly universal among all known living organisms.

Transcription

The process of genetic transcription produces a single-stranded RNA molecule known as messenger RNA, whose nucleotide sequence is complementary to the DNA from which it was transcribed. The DNA strand whose sequence matches that of the RNA is known as the coding strand and the strand from which the RNA was synthesized is the template strand. Transcription is performed by an enzyme called an RNA polymerase, which reads the template strand in the 3' to 5' direction and synthesizes the RNA from 5' to 3'. To initiate transcription, the polymerase first recognizes and binds a promoter region of the gene. Thus a major mechanism of gene regulation is the blocking or sequestering of the promoter region, either by tight binding by repressor molecules that physically block the polymerase, or by organizing the DNA so that the promoter region is not accessible.

In prokaryotes, transcription occurs in the cytoplasm; for very long transcripts, translation may begin at the 5' end of the RNA while the 3' end is still being transcribed. In eukaryotes, transcription necessarily occurs in the nucleus, where the cell's DNA is sequestered; the RNA molecule produced by the polymerase is known as the primary transcript and must undergo post-transcriptional modifications before being exported to the cytoplasm for translation. The splicing of introns present within the transcribed region is a modification unique to eukaryotes; alternative splicing mechanisms can result in mature transcripts from the same gene having different sequences and thus coding for different proteins. This is a major form of regulation in eukaryotic cells.

Translation

Translation is the process by which a mature mRNA molecule is used as a template for synthesizing a new protein. Translation is carried out by ribosomes, large complexes of RNA and protein responsible for carrying out the chemical reactions to add new amino acids to a growing polypeptide chain by the formation of peptide bonds. The genetic code is read three nucleotides at a time, in units called codons, via interactions with specialized RNA molecules called transfer RNA (tRNA). Each tRNA has three unpaired bases known as the anticodon that are complementary to the codon it reads; the tRNA is also covalently attached to the amino acid specified by the complementary codon. When the tRNA binds to its complementary codon in an mRNA strand, the ribosome ligates its amino acid cargo to the new polypeptide chain, which is synthesized from amino terminus to carboxyl terminus.
During and after its synthesis, the new protein must fold to its active three-dimensional structure before it can carry out its cellular function.

DNA replication and inheritance

The growth, development, and reproduction of organisms relies on cell division, or the process by which a single cell divides into two usually identical daughter cells. This requires first making a duplicate copy of every gene in the genome in a process called DNA replication. The copies are made by specialized enzymes known as DNA polymerases, which "read" one strand of the double-helical DNA, known as the template strand, and synthesize a new complementary strand. Because the DNA double helix is held together by base pairing, the sequence of one strand completely specifies the sequence of its complement; hence only one strand needs to be read by the enzyme to produce a faithful copy. The process of DNA replication is semiconservative; that is, the copy of the genome inherited by each daughter cell contains one original and one newly synthesized strand of DNA.[9]

After DNA replication is complete, the cell must physically separate the two copies of the genome and divide into two distinct membrane-bound cells. In prokaryotes - bacteria and archaea - this usually occurs via a relatively simple process called binary fission, in which each circular genome attaches to the cell membrane and is separated into the daughter cells as the membrane invaginates to split the cytoplasm into two membrane-bound portions. Binary fission is extremely fast compared to the rates of cell division in eukaryotes. Eukaryotic cell division is a more complex process known as the cell cycle; DNA replication occurs during a phase of this cycle known as S phase, whereas the process of segregating chromosomes and splitting the cytoplasm occurs during M phase. In many single-celled eukaryotes such as yeast, reproduction by budding is common, which results in asymmetrical portions of cytoplasm in the two daughter cells.

Molecular inheritance

The duplication and transmission of genetic material from one generation of cells to the next is the basis for molecular inheritance, and the link between the classical and molecular pictures of genes.
Organisms inherit the characteristics of their parents because the cells of the offspring contain copies of the genes in their parents' cells. In asexually reproducing organisms, the offspring will be a genetic copy or clone of the parent organism. In sexually reproducing organisms, a specialized form of cell division called meiosis produces cells called gametes or germ cells that are haploid, or contain only one copy of each gene. The gametes produced by females are called eggs or ova, and those produced by males are called sperm. Two gametes fuse to form a fertilized egg, a single cell that once again has a diploid number of genes—each with one copy from the mother and one copy from the father.

During the process of meiotic cell division, an event called genetic recombination or crossing-over can sometimes occur, in which a length of DNA on one chromatid is swapped with a length of DNA on the corresponding sister chromatid. This has no effect if the alleles on the chromatids are the same, but results in reassortment of otherwise linked alleles if they are different. The Mendelian principle of independent assortment asserts that each of a parent's two genes for each trait will sort independently into gametes; which allele an organism inherits for one trait is unrelated to which allele it inherits for another trait. This is in fact only true for genes that do not reside on the same chromosome, or are located very far from one another on the same chromosome. The closer two genes lie on the same chromosome, the more closely they will be associated in gametes and the more often they will appear together; genes that are very close are essentially never separated because it is extremely unlikely that a crossover point will occur between them. This is known as genetic linkage.

History

Gregor Mendel
Main article: History of genetics

The notion of a gene[10] is evolving with the science of genetics, which began when Gregor Mendel noticed that biological variations are inherited from parent organisms as specific, discrete traits. The biological entity responsible for defining traits was later termed a gene, but the biological basis for inheritance remained unknown until DNA was identified as the genetic material in the 1940s. Prior to Mendel's work, the dominant theory of heredity was one of blending inheritance, which proposes that the traits of the parents blend or mix in a smooth, continuous gradient in the offspring. Although Mendel's work was largely unrecognized after its first publication in 1866, it was rediscovered in 1900 by three European scientists, Hugo de Vries, Carl Correns, and Erich von Tschermak, who had reached similar conclusions from their own research. However, these scientists were not yet aware of the identity of the 'discrete units' on which genetic material resides.

The existence of genes was first suggested by Gregor Mendel (1822–1884), who, in the 1860s, studied inheritance in peaplants (Pisum sativum) and hypothesized a factor that conveys traits from parent to offspring. He spent over 10 years of his life on one experiment. Although he did not use the term gene, he explained his results in terms of inherited characteristics. Mendel was also the first to hypothesize independent assortment, the distinction between dominant and recessive traits, the distinction between a heterozygote and homozygote, and the difference between what would later be described as genotype (the genetic material of an organism) and phenotype (the visible traits of that organism).

Charles Darwin used the term gemmule to describe a microscopic unit of inheritance, and what would later become known as chromosomes had been observed separating out during cell division by Wilhelm Hofmeister as early as 1848. The idea that chromosomes are the carriers of inheritance was expressed in 1883 by Wilhelm Roux. Darwin also coined the word pangenesis by (1868).[11] The word pangenesis is made from the Greek words pan (a prefix meaning "whole", "encompassing") and genesis ("birth") or genos ("origin").

Mendel's concept was given a name by Hugo de Vries in 1889, in his book Intracellular Pangenesis; although probably unaware of Mendel's work at the time, he coined the term "pangen" for "the smallest particle [representing] one hereditary characteristic".[12] Danish botanist Wilhelm Johannsen coined the word "gene" ("gen" in Danish and German) in 1909 to describe the fundamental physical and functional units of heredity,[13] while the related word genetics was first used by William Bateson in 1905.[14] He derived the word from de Vries' "pangen". In the early 1900s, Mendel's work received renewed attention from scientists. In 1910, Thomas Hunt Morgan showed that genes reside on specific chromosomes. He later showed that genes occupy specific locations on the chromosome. With this knowledge, Morgan and his students began the first chromosomal map of the fruit fly Drosophila. In 1928, Frederick Griffith showed that genes could be transferred. In what is now known as Griffith's experiment, injections into a mouse of a deadly strain of bacteria that had been heat-killed transferred genetic information to a safe strain of the same bacteria, killing the mouse.

A series of subsequent discoveries led to the realization decades later that chromosomes within cells are the carriers of genetic material, and that they are made of DNA (deoxyribonucleic acid), a polymeric molecule found in all cells on which the 'discrete units' of Mendelian inheritance are encoded. In 1941, George Wells Beadle and Edward Lawrie Tatum showed that mutations in genes caused errors in specific steps in metabolic pathways. This showed that specific genes code for specific proteins, leading to the "one gene, one enzyme" hypothesis.[14] Oswald Avery, Colin Munro MacLeod, and Maclyn McCarty showed in 1944 that DNA holds the gene's information.[15] In 1953, James D. Watson and Francis Crick demonstrated the molecular structure of DNA. Together, these discoveries established the central dogma of molecular biology, which states that proteins are translated from RNA which is transcribed from DNA. This dogma has since been shown to have exceptions, such as reverse transcription in retroviruses.

In 1972, Walter Fiers and his team at the Laboratory of Molecular Biology of the University of Ghent (Ghent, Belgium) were the first to determine the sequence of a gene: the gene for Bacteriophage MS2 coat protein.[16] Richard J. Roberts and Phillip Sharp discovered in 1977 that genes can be split into segments. This led to the idea that one gene can make several proteins. Recently (as of 2003–2006), biological results let the notion of gene appear more slippery. In particular, genes do not seem to sit side by side on DNA like discrete beads. Instead, regions of the DNA producing distinct proteins may overlap, so that the idea emerges that "genes are one long continuum".[1] It was first hypothesized in 1986 by Walter Gilbert that neither DNA nor protein would be required in such a primitive system as that of a very early stage of the earth if RNA could perform as simply a catalyst and genetic information storage processor.

The modern study of genetics at the level of DNA is known as molecular genetics and the synthesis of molecular genetics with traditional Darwinian evolution is known as the modern evolutionary synthesis.

Mendelian inheritance and classical genetics

Crossing between two pea plants heterozygous for purple (B, dominant) and white (b, recessive) blossoms

According to the theory of Mendelian inheritance, variations in phenotype—the observable physical and behavioral characteristics of an organism—are due in part to variations in genotype, or the organism's particular set of genes, each of which specifies a particular trait. Different forms of a gene, which may give rise to different phenotypes, are known as alleles. Organisms such as the pea plants Mendel worked on, along with many plants and animals, have two alleles for each trait, one inherited from each parent. Alleles may be dominant or recessive; dominant alleles give rise to their corresponding phenotypes when paired with any other allele for the same trait, whereas recessive alleles give rise to their corresponding phenotype only when paired with another copy of the same allele. For example, if the allele specifying tall stems in pea plants is dominant over the allele specifying short stems, then pea plants that inherit one tall allele from one parent and one short allele from the other parent will also have tall stems. Mendel's work demonstrated that alleles assort independently in the production of gametes, or germ cells, ensuring variation in the next generation.

Mutation

DNA replication is for the most part extremely accurate, with an error rate per site of around 10−6 to 10−10 in eukaryotes.[9] (Although in prokaryotes and viruses, the rate is much higher.) Rare, spontaneous alterations in the base sequence of a particular gene arise from a number of sources, such as errors in DNA replication and the aftermath of DNA damage. These errors are called mutations.
The cell contains many DNA repair mechanisms for preventing mutations and maintaining the integrity of the genome; however, in some cases—such as breaks in both DNA strands of a chromosome—repairing the physical damage to the molecule is a higher priority than producing an exact copy. Due to the degeneracy of the genetic code, some mutations in protein-coding genes are silent, or produce no change in the amino acid sequence of the protein for which they code; for example, the codons UCU and UCC both code for serine, so the U→C mutation has no effect on the protein. Mutations that do have phenotypic effects are most often neutral or deleterious to the organism. Variants may confer benefits to the organism's fitness; it is commonly thought that mutations may produce beneficial variants. The most common mutations include point mutations in which a single codon is replaced, frame shift mutation where a single nucleotide base is inserted or deleted from the DNA strand so that all bases are shifted over, silent mutations where a single nucleotide base is replaced but without causing a change for the amino acid being coded for, and nonsense mutations, where a change in a single nucleotide base causes a codon to be turned into a stop codon hence terminating transcription at this point.

Mutations propagated to the next generation lead to variations within a species' population. Variants of a single gene are known as alleles, and differences in alleles may give rise to differences in traits. Although it is rare for the variants in a single gene to have clearly distinguishable phenotypic effects, certain well-defined traits are in fact controlled by single genetic loci. A gene's most common allele is called the wild type allele, and rare alleles are called mutants. However, this does not imply that the wild-type allele is the ancestor from which the mutants are descended. For the most part, these mutations are recessive and are phased out quickly. However, on occasion these mutations appear as dominant to other alleles, becoming predominant and increasing in the rate they are seen in a population.

Genome

Chromosomal organization

The total complement of genes in an organism or cell is known as its genome. In prokaryotes, the vast majority of genes are located on a single chromosome of circular DNA, while eukaryotes usually possess multiple individual linear DNA helices packed into dense DNA-protein complexes called chromosomes. Genes that appear together on one chromosome of one species may appear on separate chromosomes in another species. Many species carry more than one copy of their genome within each of their somatic cells. Cells or organisms with only one copy of each chromosome are called haploid; those with two copies are called diploid; and those with more than two copies are called polyploid. The copies of genes on the chromosomes are not necessarily identical. In sexually reproducing organisms, one copy is normally inherited from each parent.

Number of genes

The protein-encoding component of the human genome, categorized by function of each gene product, given both as number of genes and as percentage of all genes.[17]

Early estimates of the number of human genes that used expressed sequence tag data put it at 50 000–100 000.[18] Following the sequencing of the human genome and other genomes, it has been found that rather few genes (~20 000 in human, mouse and fly, ~13 000 in roundworm, >46,000 in rice[19]) encode all the proteins in an organism.[20] These protein-coding sequences make up 1–2% of the human genome.[21] A large part of the genome is transcribed however, to introns, retrotransposons and seemingly a large array of noncoding RNAs.[20][21] Total number of proteins (the Earth's proteome) is estimated to be 5 million sequences.[22]

Genetic and genomic nomenclature

Gene nomenclature has been established by the HUGO Gene Nomenclature Committee (HGNC) for each known human gene in the form of an approved gene name and symbol (short-form abbreviation). All approved symbols are stored in the HGNC Database. Each symbol is unique and each gene is only given one approved gene symbol. This also facilitates electronic data retrieval from publications. In preference each symbol maintains parallel construction in different members of a gene family and can be used in other species, especially the mouse.

Essential genes

Essential genes are those genes of an organism that are thought to be critical for its survival. Surprisingly few genes have been shown to be absolutely essential for the survival of bacteria, e.g. only about 10% of the ~4,200 genes of Escherichia coli.

Evolutionary concept of a gene

George C. Williams first explicitly advocated the gene-centric view of evolution in his 1966 book Adaptation and Natural Selection. He proposed an evolutionary concept of gene to be used when we are talking about natural selection favoring some genes. The definition is: "that which segregates and recombines with appreciable frequency." According to this definition, even an asexual genome could be considered a gene, insofar that it have an appreciable permanency through many generations.

The difference is: the molecular gene transcribes as a unit, and the evolutionary gene inherits as a unit.

Richard Dawkins' books The Selfish Gene (1976) and The Extended Phenotype (1982) defended the idea that the gene is the only replicator in living systems. This means that only genes transmit their structure largely intact and are potentially immortal in the form of copies. So, genes should be the unit of selection. In River Out of Eden, Dawkins further refined the idea of gene-centric selection by describing life as a river of compatible genes flowing through geological time. Scoop up a bucket of genes from the river of genes, and we have an organism serving as temporary bodies or survival machines. A river of genes may fork into two branches representing two non-interbreeding species as a result of geographical separation.

Gene targeting and implications

Gene targeting is commonly referred to techniques for altering or disrupting mouse genes and provides the mouse models for studying the roles of individual genes in embryonic development, human disorders, aging and diseases. The mouse models, where one or more of its genes are deactivated or made inoperable, are called knockout mice. Since the first reports in which homologous recombination among homologous chromosomes in embryonic stem cells was used to generate gene-targeted mice,[23] gene targeting has proven to be a powerful means of precisely manipulating the mammalian genome, producing at least ten thousand mutant mouse strains and it is now possible to introduce mutations that can be activated at specific time points, or in specific cells or organs, both during development and in the adult animal.[24][25]
Gene targeting strategies have been expanded to all kinds of modifications, including point mutations, isoform deletions, mutant allele correction, large pieces of chromosomal DNA insertion and deletion, tissue specific disruption combined with spatial and temporal regulation and so on. It is predicted that the ability to generate mouse models with predictable phenotypes will have a major impact on studies of all phases of development, immunology, neurobiology, oncology, physiology, metabolism, and human diseases. Gene targeting is also in theory applicable to species from which totipotent embryonic stem cells can be established, and therefore may offer a potential to the improvement of domestic animals and plants.[25][26]

Changing concept

The concept of the gene has changed considerably (see history section). From the original definition of a "unit of inheritance", the term evolved to mean a DNA-based unit that can exert its effects on the organism through RNA or protein products. It was also previously believed that one gene makes one protein; this concept was overthrown by the discovery of alternative splicing and trans-splicing.[14]

The definition of a gene is still changing. The first cases of RNA-based inheritance have been discovered in mammals.[27] Evidence is also accumulating that the control regions of a gene do not necessarily have to be close to the coding sequence on the linear molecule or even on the same chromosome. Spilianakis and colleagues discovered that the promoter region of the interferon-gamma gene on chromosome 10 and the regulatory regions of the T(H)2 cytokine locus on chromosome 11 come into close proximity in the nucleus possibly to be jointly regulated.[28] Even the coding sequence of a gene itself doesn't have to be all on the same chromosome: Marande and Burger showed that, in the mitochondria of the protist Diplonema papillatum, "genes are systematically fragmented into small pieces that are encoded on separate chromosomes, transcribed individually, and then concatenated into contiguous messenger RNA molecules".[29]

The concept that genes are clearly delimited is also being eroded. There is evidence for fused proteins stemming from two adjacent genes that can produce two separate protein products. While it is not clear whether these fusion proteins are functional, the phenomenon is more frequent than previously thought.[30] Even more ground-breaking than the discovery of fused genes is the observation that some proteins can be composed of exons from far away regions and even different chromosomes.[2][31] This new data has led to an updated, and probably tentative, definition of a gene as "a union of genomic sequences encoding a coherent set of potentially overlapping functional products".[14] This new definition categorizes genes by functional products, whether they be proteins or RNA, rather than specific DNA loci; all regulatory elements of DNA are therefore classified as gene-associated regions.[14]

Low Countries

Low Countries

From Wikipedia, the free encyclopedia


The Low Countries as seen from space.

The Low Countries (Dutch: de Lage Landen, French: les Pays-Bas) make up a coastal region in north western Europe, consisting especially of Belgium and the Netherlands, and the low-lying delta of the Rhine, Meuse, Scheldt, and Ems rivers where much of the land is at or below sea level.[1][2]

This wide area of Northern Europe roughly stretches from French Gravelines and Dunkirk at its southwestern point, to the area of Dutch Delfzijl and German Eastern Frisia at its northeastern point, and to Luxembourg and French Thionville in the southeast.

Most of the Low Countries are coastal regions bounded by the North Sea or the English Channel. The countries without access to the sea have linked themselves politically and economically to those with access to form one union of port and hinterland. A poetic description also calls the region the Low Countries by the Sea.

The Low Countries were the scene of the early northern towns, newly built rather than developed from ancient centres, that marked the reawakening of Europe in the 12th century. In that period, they rivaled northern Italy for the most densely populated region of Europe. Most of the cities were governed by guilds and councils along with a figurehead ruler; interaction with their ruler was regulated by a strict set of rules describing what the latter could and could not expect from them. All of the regions mainly depended on trade, manufacturing and the encouragement of the free flow of goods and craftsmen.

Germanic languages such as Dutch and Luxembourgish were the predominant languages, although Romance languages also played an important role. Secondary languages included French (Luxembourg, Brabant around Nivelles), Romance-speaking Belgium (cf. the Bishopric of Liège), the Romance Flanders (i.e. Cambrai, Lille, Tournai), and Namur (Walloon).

Terminology


The Low Countries from 1556 to 1648.

Southern part of the Low Countries with bishopry towns and abbeys ca. 7th century. Abbeys were the onset to larger villages and even some towns.

Historically, the term Low Countries arose at the Court of the Dukes of Burgundy, who used the term les pays de par deça (~ the lands over here) for the Low Countries as opposed to les pays de par delà (~ the lands over there) for the Duchy of Burgundy and the Free County of Burgundy, which were part of their realm but geographically disconnected from the Low Countries.[3][4] Governor Mary of Hungary used both the expressions les pays de par deça and Pays d'Embas (~ lands down here), which evolved to Pays-Bas or Low Countries. Today the term is typically fitted to modern political boundaries and used in the same way as the term Benelux, which also includes Luxembourg.
The name of the modern country the Netherlands has the same meaning and origin as the term "low countries" due to "nether" meaning "lower". The same name of these countries can be found in other European languages, for example German Niederlande, French, les Pays-Bas, and so on, which all literally mean "the Low Countries". In the Dutch language itself (known in Dutch as "Nederlands", meaning "Netherlandish") no plural is used for the name of the modern country. So Nederland (singular) is used for the modern nation and de Nederlanden (plural) for the 16th century domains of Charles V. (However, in official use the name of the Dutch kingdom is still Kingdom of the Netherlands (Koninkrijk der Nederlanden), a name deriving from the 19th century origins of the kingdom which originally included present-day Belgium.)

In Dutch, and to a lesser extent in English, the Low Countries colloquially means the Netherlands and Belgium, sometimes the Netherlands and Flanders—the Dutch-speaking north of Belgium. (This version does not include Luxembourg.) For example, a 'Derby der Lage Landen' (Derby of the Low Countries), is a sports event between Belgium and the Netherlands.

"Belgium" was renamed only in 1830, after splitting from the Kingdom of the Netherlands, in order to distinguish it from its northern neighbour. It had previously also commonly been referred to as one part of the geographic "Netherlands", being the part which remained in the hands of the Habsburg heirs of the Burgundian Dukes until the French Revolution. Politically, before the Napoleonic wars, it was referred to as the "Southern", "Spanish" or later "Austrian" Netherlands. It is still referred to as part of the "low countries".

History

History of the Low Countries
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Frisii

Belgae




Cana-
nefates
[5]
Chamavi, Tubanti[6] Vexilloid of the Roman Empire.svg Gallia Belgica (55BC-5th c.)


Salian Franks
Batavii[7]


unpopulated
(4th-5th c.)
Saxons Salian Franks[8]
(4th-5th c.)


Frisian Kingdom
(6th c.–734)

Frankish Kingdom (481-843) - Carolingian Empire (800-843)
Austrasia (511-687)




Middle Francia (843–855) West
Francia

(843–)

Kingdom of Lotharingia[9] (855– 959)
Duchy of Lower Lorraine[10] (959–)

Frisia


Arms of Flanders.svg

Friesland (kleine wapen).svg
Frisian
Free-
dom
[11]
(11–16th
century)
Counts of Holland Arms.svg
County of
Holland
[12]
(880–1432)
Coat of arms of Utrecht city.gif
Bishopric of
Utrecht
[13]
(695–1456)
Royal Arms of Belgium.svg
Duchy of
Brabant
[14]
(1183–1430)
Guelders-Jülich Arms.svg
Duchy of
Guelders
[15]
(1046–1543)
County of
Flanders
[16]
(862–1384)
Hainaut Modern Arms.svg
County of
Hainaut

(1071–1432)
Arms of Namur.svg
County of
Namur

(981–1421)
Armoiries Principauté de Liège.svg
P.-Bish.
of Liège

[17]
(980–1794)
Arms of Luxembourg.svg
Duchy of
Luxem-
bourg

(1059–1443)
Flag - Low Countries - XVth Century.png
Burgundian Netherlands (1384–1482)





Flag of the Low Countries.svg
Habsburg Netherlands (1482–1795)
(Seventeen Provinces after 1543)[18]



Statenvlag.svg
Dutch Republic
(Seven United Netherlands)
(1581–1795)
Flag of the Low Countries.svg
Spanish Netherlands
(1556–1714)

Austrian Low Countries Flag.svg
Austrian Netherlands
(1714–1795)


Flag of the Brabantine Revolution.svg
United States of Belgium
(1790)
LuikVlag.svg
R. Liège
(1789–'91)



Flag of the Batavian Republic.svg
Batavian Republic (1795–1806)
Kingdom of Holland (1806–1810)
Flag of France.svg
part of French First Republic (1795–1804)
part of First French Empire (1804–1815)
Flag of the Netherlands.svg
Princip. of the Netherlands (1813–1815)
United Kingdom of the Netherlands (1815–1830)


Kingdom of the Netherlands (1839–)
Flag of Belgium.svg
Kingdom of Belgium (1830–)
Flag of Luxembourg.svg
Gr D. L.
(1839–)


Gr D. of
Luxem-
bourg

(1890–)
The region politically had its origins in Carolingian empire; more precisely, most of it was within the Duchy of Lower Lotharingia.[19][20] After the disintegration of Lower Lotharingia, the Low Countries were brought under the rule of various lordships until they came to be in the hands of the Valois Dukes of Burgundy. Hence, a large part of the low countries came to be referred to as the Burgundian Netherlands also called the Seventeen Provinces up to 1581.
Even after the political secession of the autonomous Dutch Republic (or "United Provinces") in the north, the term "low countries" continued to be used to refer collectively to the region. The region was temporarily united politically between 1815 and 1839, as the United Kingdom of the Netherlands, before this split into the three modern countries of the Netherlands, Belgium and Luxembourg.

Early history

The Low Countries were part of the Roman provinces of Gallia Belgica, Germania Inferior and Germania Superior. They were inhabited by Belgic and Germanic tribes. In the 4th and 5th century, Frankish tribes had entered this Roman region and came to run it increasingly independently. They came to be ruled by the Merovingian dynasty, under which dynasty the southern part (below the Rhine) was re-Christianised.

Frankish empire

By the end of the 8th century, the Low Countries formed a core part of a much expanded Francia and the Merovingians were replaced by the Carolingian dynasty. In 800 the Pope crowned and appointed Charlemagne Emperor of the re-established Roman Empire.

After the death of Charlemagne, Francia was divided in three parts among his three grandsons. The middle slice, Middle Francia, was ruled by Lothair I, and thereby also came to be referred to as "Lotharingia" or "Lorraine". Apart from the original coastal County of Flanders, which was within West Francia, the rest of the Low Countries were within the lowland part of this, "Lower Lorraine".

After the death of Lothair, the Low Countries were coveted by the rulers of both West Francia and East Francia. Each tried to swallow the region and to merge it with their spheres of influence. Thus, the Low Countries consisted of fiefs whose sovereignty resided with either the Kingdom of France or the Holy Roman Empire. While the further history the Low Countries can be seen as the object of a continual struggle between these two powers, the title of Duke of Lothier was coveted in the low countries for centuries.

Duchy of Burgundy

Gradually, separate fiefs came to be ruled by a single family through royal intermarriage. This process culminated in the rule of the House of Valois, who were the rulers of the Duchy of Burgundy. In 1477 the Burgundian holdings in the area, the Burgundian Netherlands passed through an heiress—Mary of Burgundy—to the Habsburgs.

A documentary about the art in the region at this time was produced by the BBC, named The High Art of the Low Countries.[21]

Seventeen Provinces

In the following century the "Low Countries" corresponded roughly to the Seventeen Provinces covered by the Pragmatic Sanction of 1549 of Holy Roman Emperor Charles V, which freed the provinces from their archaic feudal obligations.

After the northern Seven United Provinces of the seventeen declared their independence from Habsburg Spain in 1581, the ten provinces of the Southern Netherlands remained occupied by the Army of Flanders under Spanish service and are therefore sometimes called the Spanish Netherlands. In 1713, under the Treaty of Utrecht following the War of the Spanish Succession, what was left of the Spanish Netherlands was ceded to Austria and thus became known as the Austrian Netherlands.
The United Kingdom of the Netherlands (1815–1830) temporarily united the Low Countries again.

After the Second World War

After the Second World War, Benelux was the name used for the trading region of the sovereign states of the Netherlands, Belgium and Luxembourg.

Literature

One of the Low Countries' earliest literary figures is the blind poet Bernlef, from c. 800, who sang both Christian pslams and pagan verses. Bernlef is representative of the coexistence of Christianity and Germanic polytheism in this time period.[22]:1–2

The earliest examples of written literature include the Wachtendonck Psalms, a collections of twenty five psalms that originated in the Moselle-Frankish region around the middle of the 9th century.[22]:3

Magnet school

From Wikipedia, the free encyclopedia https://en.wikipedia.org/wiki/Magnet_sc...