✅21 - Recombinant DNA Techniques Flashcards
What is recombinant DNA?
When DNA from two different organisms is combined and grown in microorganisms to form specific proteins
What are transgenic organisms?
Ones the have been genetically modified
What stages does making a protein using gene transfer and cloning involve?
Isolation Insertion Transformation Identification Growth/cloning
What is isolation?
The DNA fragments are isolated that have the gene for the desired protein
What is insertion?
The DNA fragment is inserted into a vector
What is transformation?
The transfer of DNA into suitable host cells
What is identification?
The host cells are identified that have successfully taken up the gene using gene markers
What is growth/cloning?
The population of host cells is cloned
What are the methods of producing DNA fragments?
Conversion of mRNA to cDNA using reverse transcriptase
Using restriction endonucleases to cut fragments containing the desired gene from DNA
Creating the gene in a gene machine, usually based on a known protein source.
How can reverse transcriptase be used to produce DNA fragments?
A cell that readily produces a protein is selected
These cells have large quantities of relevant mRNA which is more easily extracted
Reverse transcriptase is then used to make DNA from the RNA, known as cDNA (Complementary).
To make the other strand of DNA, DNA polymerase is used to build up the complementary strand
What are restriction endonucleases?
Enzymes that cut up viral DNA
What are blunt ends?
When restriction endonucleases cut DNA between two opposite base pairs, leaving two straight edges
What are sticky ends?
When restriction endonucleases cut DNA in a staggered way, leaving an uneven cut
What is a palindrome sequence?
When the sequences are opposite to each other in sticky ends
How are genes prepared for a ‘gene machine’?
The desired sequence of nucleotide bases of a gene is determined from the desired protein and the amino acid sequence determined. From this, the mRNA codons are looked up and complementary DNA triplets worked out. The desired sequence of nucleotides are then fed into a computer.
What are sequences check for before being fed into the computer of the gene machine?
Biosafety and biosecurity to ensure it meets international standards as well as ethical requirements
What are oligonucleotides?
A series of small, overlapping single strands of nucleotides which can be assembled into the desired gene.
What does the gene machine do with the oligonucleotides produced?
They are joined together to make a gene which doesn’t have introns or non-coding DNA. The gene is then replicated using PCR
How are genes from the gene machine inserted into bacterial plasmids?
Using sticky ends
What does the bacterial plasmid act as in the gene machine?
The vector
What is in vivo cloning?
Transferring fragments to a host cell using a vector
What is in vitro cloning?
Using PCR
What is the role of DNA ligase?
To bind the phosphate-sugar backbones of two sections of DNA at sticky ends and bind them
What is a promoter?
The binding site for RNA polymerase and transcription factors for transcription of a gene to occur
What is a terminator?
A region of DNA that releases RNA polymerase and ends transcription
What is a vector used for?
Transporting the DNA into the host cell