Methods for the detection of SNPs on a large scale have already b

Methods for the detection of SNPs on a large scale have already been developed by several companies44,46 and arc high on the agenda of most, companies involved in molecular biological research and development. The industrial aim is to develop high-throughput, accurate, sensitive, and cost-effective genetic diagnoses, which in turn could lead to accurate, sensitive, and cost-effective medication. Inhibitors,research,lifescience,medical DNA arrays and chip technology Most, of the hope is placed on DNA arrays and chip technology, which have been developed over the last 5 years. High-density DNA arrays allow complex mixtures of RNA and DNA to be

interrogated in a parallel and quantitative fashion. While the making of arrays with more than several hundred elements was until recently a significant

technical achievement, arrays with more than 250 000 Inhibitors,research,lifescience,medical different oligonucleotide probes or 10 000 different cDNAs (transcribed DNAs) per square centimeter can now be produced in significant, numbers.61,62 DNA chips are BIBR 1532 ic50 simply glass surfaces bearing arrays of DNA fragments at discrete addresses, at which the fragments are available for hybridization. There are many variations on the chip theme, but the general approach is as Inhibitors,research,lifescience,medical follows: – To immobilize multiple DNA samples on a solid support, which are then interrogated (hybridized) with a pool of oligonucleotide probes (a selected singlestranded string Inhibitors,research,lifescience,medical of nucleotides) that are specific for particular mutations or DNA variants (allele-specific oligonucleotides, ASOs). – To immobilize oligonucleotides on a solid support, which are then

interrogated by individual DNA samples. Either way, the sequence of the oligonucleotides that hybridize to the DNA samples is determined, thus revealing the nature of the mutation or variant, present in the DNA sample. DNA chips are commonly used either to monitor Inhibitors,research,lifescience,medical the expression of arrayed genes in mRNA samples from living cells or tissues, or to detect DNA sequence polymorphisms or mutations in genomic DNA. DNA chip technologies are distinguished by the sizes of the arrayed DNA fragments, the methods of arraying, the chemistries and linkers for attaching DNA to the chip, and Terminal deoxynucleotidyl transferase the hybridization and detection methods. The production of a DNA chip for the analysis of DNA variants or SNPs is shown in Figure 2. Figure 2. The development of an oligonucleotide array-based chip for single nucleotide polymorphism (SNP) analysis. P, polymorphism. One of the most prevalent uses of DNA arrays is to measure levels of gene expression (messenger RNA abundance) for tens of thousands of genes simultaneously. Such cDNA arrays consist, of either thousands of inserts of cDNA clones (transcribed DNA) by robotic deposition onto a glass surface, representing up to 10 000 genes on an area of 3.6 cm, or cDNA representing up to 30 000 human genes, that are synthesized on a chip.

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