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DNA Technology - Biochemistry

What is gene cloning

Where a gene is located and then is inserted into a vector to produce recombinant DNA, where then the DNA is then cloned and amplified to get a large amount of a gene type

What is a cloning vector

They are used during gene cloning in order to generate a large amount of DNA
They are derived from small circular DNA called Plasmids in bacteria and can replicate independently from the host cell

How does Gene cloning happen

S1= Isolate the desired gene from the DNA
S2= Insert the isolated DNA to the vector in order to produce recombinant DNA

S3= Transport the Vector into a host cell such as E.coli

S4= Then the recombinant DNA is inserted to host cell DNA and then udergo replication of the cell to many cells

What is an expressor vector

If you want to extract a specific protein from a gene type, where vector is imnserted to animal cell for desired protein to be produced, rather than the gene being extracted in larger quantity

Why is Gene cloning important

To generate large amounts of DNA
Generate large amount of a protein from a gene of interest with expressor vector

For Gene sequencing and expression

For the detection of disease causing mutations and dtermine chance of it happening

Develop new ways to treat disease and cure inherited diseases by gene therapy

How do you Isolate a gene

With the use of PCR:
Need to design 2 primers to anneal at either end of the gene

Need to then lyse the DNA and PCR it to get enough DNA to clone into vector

What is needed for PCR to take place

DNA polymerase in the form of TAQ polymerase due to optimum at 72 and stabel at 94 degress celcius
Pair of oligonucleotide primers

Free nucleotides and a desired DNA template

How does PCR work

S1= Denature the DNA to ssDNA by using heat to break hydrogen bonds at 94 degrees
S2= Lower temperature to 72 to then allow primer to bind vai hydrogen bonding to complimentary pairs

S3= The TAQ polymerase then add other nucleotides via complimentary base pairing to extend the primers

What are the limotation of PCR

Hard to amplify prodjucts longer than 10-15 Kbp

What is needed for the gene to be inserted to the vector

Plasmid Vector
Restriction enzymes to cut the DNA

Gel electrophoresis to seperate DNA fragments

DNA ligase to join fragements together

What are restriction enzymes that cut DNA

They recognise specific sequences of bases in the DNA and can bind to them
Then they cut the double stranded DNA by bydrolysing phosphodiester bonds

Why can't restriction enzymes cleave bacterial DNA

Due to contain ECO RI methylase that will methylate the GATTC sequence

What is DNA methylation

DNA is replicated by semi-Conservative replication
DNA methylase selectively methylates hemi-methylated DNA

What are the 2 types of restriction enzymes

Exonuclease- Remove nucleotides from the end of the DNA chain
Endonuclease- Remove nucleotides from the middle of the DNA chain

Types of restriction endonucleases

Type 1 - Cut DNA 1000BP from recognition site
Type 2 - Cut DNA at the recognition site

Type 3- Cut DNA 25 BP from the recognition site

What are blunt end and sticky ends

When they cut they make blunt ends that are harder to join together comopared to others that make sticky ends that are easier to join together as greater chance of complimentary base pair binding to take place of overlap happens

What is the recogniton site

Many restriction enzymes recognise the hexanucleotide site and other recognise 4,5 or 8 nucleotide sequences

What is Gel electrophesis

The analysis and seperation of DNA fragments made by the restriction endonuclease
The DNA loaded in wells and then move from negative to postive charge

Can see the seperated DNA in the gel under UV light

How does DNA ligase work to join DNA fragment together

Needed to produce recombinant DNA by joing 2 DNA strands together by catalysing the formation of phosphodiester bonds during a condensation reaction and ATP is needed
Can be done with sticky or blunt ended fragments but stick yhas greater chance of happening

How is Recombinant DNA made with ssame restriction endonuclease

Cut vector and gene with same enzyme, to leave the same bidning sequence at the end of the ligation
Can only happen if gene have same sequence at both end

Produce sticky ends for DNA ligase

How to make recombinant DNA with 2 restriction endonuclease

Cut Vector and gene with different enzymes, to leave differing sequences at end of the genes,
Need the vector to have both sequences in the restriction site and need to use 2 enzymes to create 2 stciky ends for DNA liagse

How to make recombinant DNA with no compatible enzymes

Use nucleases to create blund ends due to cut off njon compatible sticky end
Carry out blunt end ligation or use DNA Polymerase to fill in sticky ends rather than cut to make blunt ends

How to use linkers to make recombinant DNA

Can use linker where blunt end undergo ligation to create sticky ends bu adding linkers to them

How to use TA cloning to make recombinant DNA

Method to clone PCR products, by manipulate them to have sticky ends and then can manipilate the vector by adding small bases with terminal tranferase to make sticky ends on the vector

How to introduce the DNA to living cell

This is called transformation before the recombinant DNA can be multiplied
You need to prepare a suitable bacteria cell before can instert the plasmid

How to prepare a competent bacteria cell

Treat bacteria with calcium chloride so plasmid bind to cell exterior
Heat shock at 42 degrees to increas membrane permeability so then plasmid can enter the bacteria

Then grwo tranfored bacteria on agar plate to form colonies of it

Only 0.001 % of E.coli wil be tranformed due to most vectors die in ampicillin so grow on amipicillin playe then only the vector with the recombinant DNA will grow due to have resistance gene

How to distinguish the recombinant DNA and self ligated bacteria

Replica plating for PBR322 due to tetracycline is selectable marker in the vector
Selectable marker help to distinguish the recombinant and self ligated

Recombinant DNA make tetra inactive

What is Blue White selection

Lac z gene endode for enzyme B galactosidase that is selectable marker
Enzyme convert the lactose to galactose and glucose

If have recombinant DNA then lac z wont work so colony is white not blue so then remove all the white ones as recombinant vectors

What is restriction mapping

Transform the ligation mix into bacteria
The plate this on agar+ampicilin

Then grow the bacteria and extract the DNA and use restriction enzymes to distinguish by gel electrophoresis

What the expression factors to grow the host cell

To produce a protein from target gene need an expression vector to allow protein synthesis of wanted protein
Transcription catalysed by RNA polymerase and RNA pol bind to promoter sequenece of the gene

If need an animal protein then add bacteria promoter sequence with is LAC promoter

Why choose a bacteria host cell

Grow in liquid medium and divide rapidly
Dont glycosolayte protein so no further modification takes place

Why use animal cell as host cell

Need to grow attached to solid matrix
Allow post translational modification to allow protein to function

Slower division

Need to use animal cloning vector

How to make Bioreceptors

Use animals to produce certain benefical proteins
Gene inserted to animal and get proteins from:

Chickens via eggs and cows via milk

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