Recombinant DNA Technology

Question 1

What is Recombinant DNA?

Answer 1

• Recombinant DNA molecules are DNA molecules formed by laboratory methods of genetic recombination to bring together genetic material from multiple sources, creating sequences that would not otherwise be found in the genome

Question 2

Where are we with recombinant DNA technology so far?

Answer 2

• Therapeutic proteins (eg. Human growth hormone and human insulin) have been recombinantly produced in bacteria (E. coli)
• The first two recombinant proteins authorised for use in the USA as a drug therapeutic
• Many more therapeutics will be produced in bacteria in the future

Question 3

Why is recombinant DNA important?

Answer 3

• Much of what we know about gene structure and function stems from molecular studies using recombinant DNA techniques
• The ability to clone, sequence and assess the function of genes is reliant on recombinant DNA techniques, and has aided in the construction and extended use of DNA and protein databases

Question 4

Imagine you want to study the gene that is linked to cancer, or some other disease, what questions would you ask in preparation of finding the gene?

Answer 4

• What is the DNA sequence of the gene?
• What is the mutation(s) in the gene that causes disease?
• What is the function of the protein product of the gene?
• How is that function changed in the mutated protein?
• In which cells is the gene expressed?
• What are the promoter sequences that control the expression of the gene?
• Is the expression of the gene altered in cancer (or disease)?

Question 5

The preservation of endangered species involves three major genetic solutions, what are they?

Answer 5

• Gene Banks
• Cloning and the Preservation of Endangered species
• Conservation Genetics

Question 6

What are Gene Banks?

Answer 6

• Gene banks are helping to preserve endangered species by storing the biological and genetic material of animals that are under threat of extinction

Question 7

What is the Frozen Ark Project?

Answer 7

• The Frozen Ark is an organisation that preserves endangered species
• The Frozen Ark Project strives towards a world where extinction rates are sustainable and not created by man. Where the beauty, splendour and practical solutions found in all species is noted and used by man for the good of mankind and for the good of all life on Earth.

Question 8

What is Cloning and the Preservation of Endangered species

Answer 8

• Animal cloning is now a possibility and many species have been cloned. For conservation efforts this could mean that a clone is created from stored genetic material and implanted into the surrogate mother of a closely related species.

Question 9

What is Conservation Genetics?

Answer 9

• Applies genetic methods to the conservation and restoration of biodiversity. Essentially the field combines several disciplines: molecular biology, ecology, population genetics, mathematical modelling, and evolutionary systems, with the aim of preserving biological diversity.

Question 10

What is environmental DNA?

Answer 10

• Environmental DNA or eDNA is DNA that is collected from a variety of environmental samples such as soil, seawater, snow or even air rather than directly sampled from an individual organism

Question 11

What are some examples of Environments where eDNA might be found and collected?

Answer 11

• Glaciers
• Permafrost/tundra
• Aquatic sediments
• Lakes and streams
• Terrestrial habitats
• Oceans
  The first three are ancient environments while the latter three are modern

Question 12

What types of environmental sampling is used to retrieve eDNA from the environment?

Answer 12

• Ice cores
• Soil/sediment core samples
• Freshwater/seawater samples

Question 13

What DNA extraction procedures are used for getting the eDNA out of the environmental samples?

Answer 13

• The DNA extraction is carried out using procedures specific for the individual type of sample

Question 14

What is PCR?

Answer 14

• Polymerase chain reaction (PCR) is a method widely used in molecular biology to make several copies of a specific DNA segment

Question 15

What is the overall process of collecting eDNA?

Answer 15

• Find the environment (glaciers, tundra, etc)
• Gather environmental samplings (Ice cores, soil samples, etc)
• DNA extraction
• PCR amplification of extracted DNA
• Bioinformatic data processing

Question 16

How is PCR amplification done?

Answer 16

• Using generic or species specific primers targeting biodiversity and subsequent sequencing of amplicons
• An amplicon is a piece of DNA or RNA that is the source and/or product of amplification or replication events

Question 17

What is Bioinformatic data processing

Answer 17

• Bioinformatics is a science field that is similar to but distinct from biological computation.
• Bioinformatics and computational biology involve the analysis of biological data, particularly DNA, RNA, and protein sequences.

Question 18

Study the diagram of how eDNA is collected

Answer 18

https://docs.google.com/document/d/1Nzo4FTzXCbwOZjpoc_J_4IF3gsOXPcoyC2BowELmx0U/edit?usp=sharing

Question 19

How are Gene Coding and Recombinant DNA accomplished?

Answer 19

• Gene cloning is the isolation and amplification of a given gene
• A recombinant DNA molecule is a DNA molecule made by joining two or more different DNA molecules
• Both are accomplished using:
• Molecular scissors: Restriction Endonucleases
• Molecular glue: DNA Ligase
• As well as molecular glue and molecular scissors, we have the molecular equivalents of DNA production lines

Question 20

What is Restriction Endonuclease?

Answer 20

• Naturally occurring enzyme present in many bacteria, also called restriction enzymes or RE

Question 21

What is the function of Restriction Endnucleases?

Answer 21

• Natural functions can be likened to a bacterial immune system. Basic function of these enzymes is to cut up DNA. Any foreign DNA that enters the bacteria is cut up by the bacteria’s restriction endonucleases
• The bacteria’s own DNA is protected from digestion by the restriction enzymes, usually by a specific methylation pattern. Any infecting, foreign DNA is not methylated appropriately and so is digested
• Some restriction enzymes cut DNA in a random fashion, but others cut DNA strands at specific base sequences

Question 22

What is Methylation?

Answer 22

• In the chemical sciences, methylation denotes the addition of a methyl group on a substrate, or the substitution of an atom by a methyl group

Question 23

How is DNA protected from RE digestion via Methylation?

Answer 23

• Some restriction enzymes cut DNA in a random fashion, but others like EcoRI cut DNA strands at specific base sequences
• For example, The DNA strand of EcoRI will have a Methylated recognition sequence where the CH3 or some other methyl group will bond to the DNA strand. This prevents any enzyme binding which in turn prevents random DNA cutting.

Question 24

Study the diagrams for The Protection of DNA from Restriction Enzyme Digestion by Methylation

Answer 24

https://docs.google.com/document/d/1Nzo4FTzXCbwOZjpoc_J_4IF3gsOXPcoyC2BowELmx0U/edit?usp=sharing

Question 25

How is Site specific RE used?

Answer 25

• Site specific restriction endonucleases are used in recombinant DNA technology
• RE recognise a specific DNA sequence, normally between four and eight base pairs long
• The first site-specific restriction endonuclease discovered was HincII (HindII)

Question 26

How are site specific RE named?

Answer 26

• The first three letters of the name of the enzyme indicates the bacteria from which it was purified, e.g. HincII = Haemophilus influenzae
• If the enzyme is produced only in a particular strain, then a letter designating that strain is added (here c for strain Rc, d for strain Rd)

Question 27

What does the restriction enzyme HincII (HindII) do?

Answer 27

• HincII (HindII) recognises the sequence “GTPyPuAC” and CAPuPyTG
• It cuts the double stranded DNA in the middle of the sequence and leaves two blunt DNA ends

Question 28

How are sticky ends and blunt ends created?

Answer 28

• Different restriction enzymes cut the DNA in different ways
• The “ends” refer to the ends of the DNA strands
• Depending on where and how the RE cuts, it will produce either sticky or blunt ends

Question 29

What are Sticky ends?

Answer 29

• Sticky ends on the other hand are generated by a staggered cut and they have unpaired bases or overhangs at the 3′ and 5′ regions. These overhangs are useful during the ligation as they ensure proper joining of the fragments

Question 30

What are Blunt ends?

Answer 30

• Blunt ends are formed by a straight cut and they do not contain any unpaired bases or overhangs at the 3′ or 5′ regions. Hence, it is difficult to ligate the fragments with blunt ends.

Question 31

Study the diagram of the cutting of DNA

Answer 31

• Google doc

Question 32

What sequences are Restriction Endonuclease Recognition Sites usually found on?

Answer 32

• They are often palindromic sequences (Nucleotide pair sequences that read the same forward or backward from a central axis ‘*’ )
• E.g. EcoRI: GAATTC or CTTAAG

Question 33

How long are the Restriction Endonuclease Recognition Sites usually?

Answer 33

• Usually either 6 bases long, but also 4 bases. A few restriction endonucleases recognise 8 base sequences (eg. NotI)
• Some restriction enzymes have the same recognition sequence, eg. SmaI and XmaI, but they make different cuts
• E.g. SmaI: CCCGGG, where the cut is downward and GGG­CCC, where the cut is uppward (opposite strands)
• E.g. XmaI: CCCGGG, where the cut is downward and GGGCC­C, where the cut is upward (opposite strands)

Question 34

What are Isoschizomers?

Answer 34

• Restriction enzymes that recognise the same sequence

Question 35

Study the table for the recognition sequences and cleavage sites of representative restriction Endonucleases

Answer 35

• Google doc

Question 36

What is a “Digest” in genetics

Answer 36

• When fragments of DNA are cut by RE

Question 37

What is the SV40 chromosome?

Answer 37

• Simian virus 40 (SV40) is a useful model system for numerous studies in the fields of eukaryotic gene transcription, DNA replication, and cell transformation.
• Thus, the viral genome contains promoters with complex arrays of regulatory elements as typically found in regulated cellular genes.

Question 38

What are restriction maps?

Answer 38

• Restriction maps reflect true physical distances

- Restriction maps can be combined with other molecular techniques to construct physical maps of entire genomes

Question 39

What are the steps for the Construction of Recombinant DNA Molecules In Vitro

Answer 39

• Step one = cut both of the DNA from 2 speices with an RE
• Step 2 = mix the cut (digested) DNA’s and incubate under annealing conditions
• Step 3 = Treat annealing DNA fragments with DNA Ligase

Question 40

What is plasmid DNA?

Answer 40

• A plasmid is a small DNA molecule within a cell that is physically separated from chromosomal DNA and can replicate independently.

Question 41

How is Ligase used to make recombinant DNA?

Answer 41

• Ligase can join two pieces of DNA by forming the missing phosphodiester bonds between each strand of DNA
• Sticky ends created by restriction endonucleases (eg. EcoRI) facilitate this process
• Ligation takes place between 5’ -P and 3’ -OH termini

Question 42

Study the diagrams for the Construction of Recombinant DNA Molecules In Vitro and DNA Ligase Function

Answer 42

• Google doc