MCB 2050 Study Guide - Midterm Guide: Selectable Marker, Ecori, Complementary Dna

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Ecori: escherichia coli strain ry13 restriction enzyme number i recognize palindromic and create either staggered (cohesive, sticky) or blunt ends. Smal- produces blunt ends (cccggg ----> ccc ggg ) G3"/3" cctag5" + 5"gatcc3"/3"g5") complementary single stranded ends produced by restriction enzyme cleavage can be joined (ligated) together using dna ligase to create recombinant dna molecule. Construction of recombinant dna molecule: cut plasmid and dna you want to clone with restriction enzyme, anneal and ligate complementary dna fragments. Mcs located upstream of the reporter gene can be used to clone in and assess the strength of potential gene regulatory sequence. Cloning vectors pbluescript classic blue white selection for identifying bacteria containing recombinant plasmids. Bluescript plasmid expresses e. coli lacz gene (encodes b-galactosidase which converts colourless substrate into blue product) Mcs allows insertion of potential gene regulatory sequences luciferase protein converts luciferin to light.

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