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A regulatory sequence is a segment of a nucleic acid molecule which is capable of increasing or decreasing the expression of specific genes within an organism. Regulation of gene expression is an essential feature of all living organisms and viruses.
Transcription factors are proteins that bind to specific DNA sequences in order to regulate the expression of a given gene. There are approximately 1,400 transcription factors in the human genome and they constitute about 6% of all human protein coding genes. [ 21 ]
Regulation of gene expression, or gene regulation, [1] includes a wide range of mechanisms that are used by cells to increase or decrease the production of specific gene products (protein or RNA). Sophisticated programs of gene expression are widely observed in biology, for example to trigger developmental pathways, respond to environmental ...
Deacetylation performed by HDAC molecules has the opposite effect. By deacetylating the histone tails, the DNA becomes more tightly wrapped around the histone cores, making it harder for transcription factors to bind to the DNA. This leads to decreased levels of gene expression and is known as gene silencing. [5] [6] [7]
In biochemistry, in the biological context of organisms' regulation of gene expression and production of gene products, downregulation is the process by which a cell decreases the production and quantities of its cellular components, such as RNA and proteins, in response to an external stimulus.
In general gene expression is regulated through changes [44] in the number and type of interactions between molecules [45] that collectively influence transcription of DNA [46] and translation of RNA. [47] Some simple examples of where gene expression is important are: Control of insulin expression so it gives a signal for blood glucose regulation.
In StEP, brief cycles of primer annealing to a template and extension by polymerase are employed to generate full-length sequences. [31] [32] The main advantages of StEP are the simplicity of the method and the lack of fragment purification. [7] [13] The disadvantages of StEP include that it is time consuming and requires sequence homology. [7 ...
The positive charge on a histone is always neutralized upon acetylation, creating euchromatin which increases transcription and expression of the target gene. [16] Lysine residues 9, 14, 18, and 23 of core histone H3 and residues 5, 8, 12, and 16 of H4 are all targeted for acetylation.