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Question
How can a genomic library be prepared?
Long Answer
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Solution
- Isolation of Genomic DNA: The first step is to isolate pure chromosomal DNA from the organism whose genome is to be studied.
- Fragmentation of DNA: The genomic DNA is cut into smaller fragments using specific restriction enzymes that produce fragments with sticky ends.
- Insertion into Vectors: These DNA fragments are then inserted into suitable cloning vectors that have been cut with the same restriction enzyme to ensure compatibility of ends.
- Ligation: DNA ligase is used to join the DNA fragments with the vector DNA, forming recombinant DNA molecules.
- Transformation: The recombinant DNA molecules are introduced into competent host cells (usually bacteria) by transformation.
- Selection and Screening: Transformed cells are grown on selective media to identify those that contain recombinant DNA.
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