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(A-level) AQA Biology DNA Technology Topic Summary

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In-depth summary for content covered in the DNA Technology topic of A-level AQA Biology, including content on DNA replication via in-vivo and in-vitro methods, restriction endonucleases, PCR, DNA probes and more. This will still be applicable to other exam boards, but take caution when looking at key-words and the order of specific processes. NOTE: a colour code (and use of italics) is used for keywords and expressions in the document, in some documents this may be consistent throughout but for longer documents I have uploaded only the first pages may act as an example of this - giving you opportunity to work through and apply your own colour coding.

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Oliver Dyson


(21) Recombinant DNA technologies

Producing DNA fragments:

DNA and gene technologies have benefitted society in a wide range of ways

-> from medical to industrial applications

 Many diseases can be treated and detected using this – for example mass production of
insulin for diabetes treatment
 When DNA of two different organisms is combined, as is seen very often here (usually
insertion of eukaryotic into prokaryotic), this is called recombinant DNA
 The resulting organisms is known as a transgenic or genetically modified organism (GMO)

This is made possible by the genetic code being universal

-> which means there is no issue for incorporation / function (in most cases)

Making a protein using DNA technology:

This occurs in 5 main stages

-> which are:

1. Isolation of the DNA fragments that have the gene for the desired protein
2. Insertion of the DNA fragment into a vector
3. Transformation – transfer of DNA into suitable host cells
4. Identification – finding which host cells have taken up the gene using gene markers
5. Growth / cloning – increasing the population of the host cells

This can be done in a few different ways

-> finding and isolating gene is first:

 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 basing it off of a known protein
structure

Using reverse transcriptase:

This is an enzyme which is found in many retroviruses such as HIV

-> and is what is used to convert their RNA into DNA in a host cell

 A cell that readily produced the protein is selected (e.g. β-cells of islets of
Langerhans in the pancreas, for insulin production)
 These contain large amounts of the corresponding mRNA – easily extracted

 Reverse transcriptase is used to make DNA from RNA
 This DNA is called cDNA – because it is made up of nucleotides that are
complementary to the mRNA
 To make up the other strand of DNA – DNA polymerase is used to build up the
complementary nucleotides on the cDNA template, forming a double helix / strand Figure 1 – reproduced
from [1]

, Oliver Dyson


Using restriction endonucleases:

All organisms have defensive mechanisms against pathogens

-> bacteria are frequently infected by viruses

 A defence against this is by producing enzymes that can cut up the viral DNA
 These are called restriction endonucleases

There are many types of this enzyme

-> each one cutting different sequences of bases apart

 These sections / sequences are called recognition sequences
 Cuts can sometimes occur between two opposite base pairs
 This leaves two straight edges known as blunt ends

For example, one endonuclease cuts in the middle of the base recognition sequence GTTAC (as in
diagram)

 Others cut DNA in a staggered fashion – leaving an uneven cut in which each strand of the
DNA has exposed bases
 E.g. the endonuclease for AAGCTT

The unpaired bases formed from this are a palindrome

-> and the recognition sequence is known as a six bp palindromic sequence

 This is used to cut DNA, leaving ‘sticky ends’




Figure 2 – reproduced from [1]

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Publié le
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Nombre de pages
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Écrit en
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