TEKNOLOGI PLASMID (KLONING GEN/DNA REKOMBINAN)

Sri Mulyani Biology

30 Oct 202011:35

Summary

TLDRThis video explains plasmid technology, focusing on its role in genetic engineering. It covers the use of plasmids as vectors to carry foreign DNA into bacteria, a key aspect of recombinant DNA technology. Key components like restriction enzymes, ligase, and marker genes are discussed, along with the step-by-step process of DNA cutting, ligating, transforming, and selecting successful recombinant bacteria. The video also explains how bacterial colonies are used to differentiate between recombinant and non-recombinant plasmids, highlighting the importance of selective markers such as antibiotic resistance and lactose metabolism.

Takeaways

😀 Plasmids are circular, double-stranded DNA molecules used in recombinant DNA technology as vectors to carry foreign genes.
😀 A plasmid, foreign DNA (target gene), bacteria (host cell), restriction enzymes, and ligase are essential components of plasmid technology.
😀 Restriction enzymes cut both the plasmid and the foreign DNA at specific sites to allow insertion of the gene of interest.
😀 Ligase enzyme is used to join the foreign DNA to the plasmid, creating recombinant DNA.
😀 Plasmids replicate independently of the bacterial chromosome, allowing for the production of large amounts of the target gene product.
😀 A plasmid must have a marker gene, like ampicillin resistance, to help identify and select bacteria containing recombinant plasmids.
😀 The LacZ gene, which metabolizes lactose, is often used as a second marker to identify successful plasmid incorporation.
😀 Plasmid vectors need a restriction site where foreign DNA can be inserted, which is critical for recombinant DNA technology.
😀 After recombinant plasmid formation, bacterial transformation is performed, inserting the plasmid into bacterial cells.
😀 Bacterial cells are then selected using a medium containing ampicillin and lactose; only the bacteria with the recombinant plasmid survive.
😀 Blue colonies indicate plasmids without foreign DNA (active LacZ gene), while white colonies indicate recombinant plasmids (inactivated LacZ gene).

Q & A

What is plasmid technology?
-Plasmid technology, also known as recombinant DNA technology, involves using bacterial plasmids as vectors to manipulate the genes of living organisms.
What are the essential components needed in plasmid technology?
-The essential components include plasmids, foreign DNA (target gene), bacteria (host cells), restriction enzymes (endonucleases), and ligase enzymes.
What role does a plasmid play in recombinant DNA technology?
-A plasmid serves as a vector or vehicle to carry foreign DNA or the target gene into bacterial cells for replication and gene expression.
What are restriction enzymes used for in plasmid technology?
-Restriction enzymes are used to cut DNA molecules, including both the plasmid and the foreign DNA, at specific sequences, making it possible to insert the foreign DNA into the plasmid.
What function does ligase perform in recombinant DNA technology?
-Ligase enzymes are used to join the foreign DNA with the plasmid, effectively 'gluing' the DNA fragments together to form a recombinant DNA molecule.
How is a plasmid structured in recombinant DNA technology?
-A plasmid is a circular, double-stranded DNA molecule that exists separately from the bacterial chromosomal DNA and is capable of self-replication.
What is the purpose of having a marker gene in a plasmid?
-A marker gene, such as one conferring antibiotic resistance, allows scientists to identify and select bacterial cells that have successfully incorporated the recombinant plasmid.
How does a restriction site help in plasmid technology?
-A restriction site is a specific DNA sequence where restriction enzymes cut. It enables the insertion of foreign DNA into the plasmid at a known location.
Why is it important to use the same restriction enzyme for both the plasmid and foreign DNA?
-Using the same restriction enzyme ensures that both the plasmid and the foreign DNA are cut at compatible sites, making it easier to insert the foreign DNA into the plasmid.
What is the difference between blue and white bacterial colonies in plasmid screening?
-Blue colonies indicate the presence of a non-recombinant plasmid, which can metabolize lactose, while white colonies indicate the presence of a recombinant plasmid, where the foreign gene has inactivated the ability to metabolize lactose.