01:694:215 Lecture Notes - Lecture 9: Nonsense Mutation, Ecori, Reading Frame

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Developed rapidly, many genomes are completely sequenced. One needs a known or fixed starting point on one end of the dna to be sequenced. Dna fragments are then generated that are random in length but end with a defined type of base. The random populations of dna fragments are then separated using high-resolution bels or chromatography. This gel system can separate fragments that differ in as little as one base in length. Ddt has h group instead of oh group so nothing else can attach to it terminates the chain. In the synthesized strand, the first time you get the base is when synthesis stops because it has a h group instead of oh group. Add equal amounts of ddc and dc depends on whichever one is synthesized. Use two primers a and b on either side there will be overlap. Remove everything before the start codon (atg) and the bad wavelengths (sequence becomes poor quality)

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