Genetic engineering: deliberate modification of an organisms genetic information by directly changing the nucleic acid sequence. Recombinant dna technology: dna with a new sequence formed by joining fragments. Restriction enzymes: bind to dna at specific sequences called recognition site, cleave double stranded dna at this site or a defined distance from it. Agrose gel electrophoresis seperates the negatively charged dna molecules by size. Dna fragments are then denatured and transferred onto a nylon membrane. Membrane is bathed in radioactive probe comprised of a labled complementary single stranded nucleic acid. Rapid synthesis of many copies of a specific. Dna fragment from a complete mix of dna. Amplify environmental genes without culturing the microbes. Cloning vectors: plasmids, phages and viruses, cosmids, artificial chromosomes. Vectors engineered phage genomes previously genetically modified including restriction sites insertion of foreign dna; recombinant phage genone is packed into the capsid and used to infect host.
