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प्रश्न
Give an account of the Blue-White Method of selection of recombinants.
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उत्तर
Recombinant DNA (rDNA) technology is the technique of manipulating the genome of a cell or the organism so as to change the phenotype desirably.
Following are the basic steps involved in the process:
- Isolating genomic DNA of a ‘donor’. The cell or organism from which the required gene is taken is called ‘donor’.
- Fragmenting this DNA using “molecular scissors” (Enzymes): Different enzymes used are restriction endonucleases, DNA ligase, reverse transcriptase, DNA polymerase, alkaline phosphatases, etc. The restriction endonucleases are used to cut DNA at specific points. They are called biological/molecular/chemical scissors/knives/scalpels.
- Screening the fragments for a ‘desired gene’.
- Inserting the fragments with the desired gene into a ‘cloning vector’ – vectors are the DNA molecules used to transfer genetic material into another cell. (a plasmid, cosmid or phage DNA), so as to develop a recombinant DNA or chimeric DNA.
- Introducing the recombinant vector into a competent host cell.
- Culturing these cells to obtain multiple copies or clones of the desired fragment of DNA.
- Using these copies to “Transform” suitable host cells so as to express the desired gene.
- Selection of transformants by the blue-white method of selection of recombinants.

It is a screening technique that allows for rapid and convenient detection of recombinant bacteria in vector-based molecular cloning experiments. Recombinant DNA is inserted into a competent host cell viable for transformation, which is then grown in the presence of X-gal. The cell transformed with vectors containing recombinant DNA will produce white colonies; cells transformed with non-recombinant plasmids (i.e., only the vector) grow into blue colonies. This method of screening is usually performed using a suitable bacterial strain, but other organisms such as yeast may also be used.
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