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Production of Recombiant DNA products - notes and outlines

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  • Course
  • AU858 (MCRO07004)
  • Institution
  • ATU

Provides an outline for the basis of producing a recombinant product. Including applications and methods of transformation. These notes also include notes on the different bioreactors and how they work within the biopharmaceutical industry. - I can am also able to answer further questions should ...

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Document information

  • May 23, 2024
  • 3
  • 2023/2024
  • Class notes
  • Mary heneghan
  • Microbial biotechnology

Subjects

  • recombiant dna
  • production of dna
  • microbial biotechnology
  • polymerase chain reaction

Written for

  • ATU
  • AU858 (MCRO07004)
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Available practice questions

Quick Revision of Production of Recombinant Product Flashcards

Flashcards 12 Flashcards
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Flashcards 12 Flashcards
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Some examples from this set of practice questions

1.

What is the definition of \'Recombinant DNA Technology\'

Answer: Combining DNA of different species to create a new genetic combinations

2.

What are the primary operations of downstream purification?

Answer: cell recovery and clarification

3.

what are secondary processing steps in downstream purification?

Answer: separates the desired protein from the culture medium eliminates impurities from product

4.

what are the function of restriction enzymes and an example

Answer: They cut DNA are specific nucleotide sequences examples : HIND III , BAMH I, ECOK

5.

What are the factors affecting the choice of expression system

Answer: glycosylation yields regulatory approval

6.

What is the purpose of the Master Cell Bank (MCB)

Answer: Ensures consistent starting material for production over the years

Content preview

2.Production of a recombinant product
Monday, February 26, 2024 1:05 PM



Recombinant DNA Technology
Definitions: Recombinant DNA Technology involves combining DNA from different
species to create new genetic combinations.

Applications:
• producing DNA,
• proteins,
• biochemical pathway products
• chemical structures for science
• medicine,
• Agriculture
• industry.

Isolating Gene of Interest WHATS NEEDED TO CLONE GOI:
• Source DNA containing the gene of interest can be isolated from bacteria, yeast, • GOI
fungi, plant cells, or animal cells. • Restriction enzymes
• Vector to receive
• Genomic DNA extraction involves cell culture growth, cell lysis, removal of • Mechanism to "glue" GOI into vector
contaminants, and DNA concentration.

• Polymerase Chain Reaction (PCR) is used to separate the gene of interest from
chromosomal DNA by amplifying a specific DNA sequence.

• PCR involves denaturation, annealing, and extension steps to replicate DNA in a
test tube.
Production of Recombinant Product
Cloning process:
1. cloning the Gene of Interest (GOI) into a vector using restriction enzymes and a
mechanism to insert the GOI.

2. Restriction enzymes cut DNA at specific nucleotide sequences, creating sticky or
blunt ends for ligation.

3. Vectors, like plasmids, are circular DNA molecules used to transport foreign genes
into host cells for replication and expression.

4. Plasmids must have an origin of replication, selectable markers, and restriction
enzyme sites to be useful for recombination technology.

Characteristics of Vectors :
• must be circular, large enough to hold the gene of interest, and contain an Origin of
DNA replication (ORI).

• Multi-cloning sites (MCS) provide multiple restriction enzyme sites for gene
insertion.

• Marker genes and control sequences like transcription promoters help identify cells
with the vector and ensure gene expression.

• Copy number, the quantity of plasmids per bacterial cell, is crucial for successful
cloning, ranging from 1 to hundreds per cell.

Plasmid Copy Number and Cloning Vectors

DNA Ligase:
• repairs DNA breaks by joining nucleotides in a DNA strand.
• complements restriction enzymes by linking DNA fragments covalently.
• Enzyme acts as a 'spot welder' forming covalent bonds between DNA strands.

Cloning Technique with DNA Ligase
• Enzymes with staggered cuts create complementary ends for ligation.
• Sticky ends must be complementary for successful ligation

Bacterial Transformation and Recombinant Product Production

Bacterial Transformation:
• Vectors need to be incorporated into bacterial cells for replication or expression.
• Transformed cells are selected using antibiotic resistance genes.

Transformation Methods:
1. electroporation
2.CaCl2 (calcium chloride)/Heatshock

Recombinant Product Production:
• Verification steps include plasmid isolation, restriction digestion, PCR, and
sequencing.
• Expression systems like bacteria, fungi, yeast, or mammalian cells are used.
• Intracellular and extracellular product expression methods differ in purification
ease.
Cell Line Development
Cell Line Construction
expressing proteins in :

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