Recombinant Technology

Question 1

What are ‘restriction enzymes’?

Answer 1

Enzymes which reliantly cut DNA into more manageable sizes, by cutting at precise recognition sequences (palindromic sequences)

Question 2

Where were most restriction enzymes discovered?

Answer 2

In bacteria

Question 3

What is an example of a restriction enzyme?

Answer 3

Xbal

Question 4

How long are the recognition sequences of restriction enzymes?

Answer 4

6 nucleotides lons

Question 5

How do restriction enzymes usually act?

Answer 5

As dimers

Question 6

What 2 ways can DIFFERENT restriction enzymes cut DNA?

Answer 6

1) Sticky-ends: cut through the DNA backbone asymmetrically, leaving overhangs
2) Blunt: Cut symmetrically, flush ends

Question 7

How can restriction fragments be separated from each other?

What is the process of this?

Answer 7

Gel electrophoresis:

1) Place sample in the well in the top of the agarose gel (in buffer solution
2) Apply a current across the gel
3) The negatively charged DNA is attracted to the positive anode
4) As the fragments move, they become separated by size (smaller travel faster as they can pass through smaller holes)
5) Stain the gel using florsecence (eithidium brominde)

6) End up with many bands on one lane
- Can run many samples on one gel

7) Cut the DNA out of the gel

Question 8

What gel is used in gel electrophoresis to separate restriction fragments?

Answer 8

Agarose gel

Question 9

Using gel electrophoresis, how can the length of fragments be worked out?

Answer 9

Run known sized fragments on the gel and compare with the bands of the unknown fragments

Question 10

What is ligase?

Answer 10

An enzyme which joins 2 DNA fragments together to form recombinant DNA, using ATP

Question 11

What is recombinant DNA?

Answer 11

DNA which doesn’t normally exist in the nature - formed by laboratory methods, which bring together DNA from multiple sources

Question 12

How does ligation work better?

Answer 12

If the fragments of DNA have the same overhang (cut by the same restriction enzyme) as they can hybridise with each other and form H bonds

Question 13

What is another way to explain ‘sticky ends’?

Answer 13

Cohesive termini

Question 14

What are plasmids?

Answer 14

Small, circular, extra-chromosomal DNA that occur naturally in bacteria

They have a single origin of replication

Question 15

How many copies of the plasmid is made in bacteria?

Answer 15

50

Question 16

What does cloning DNA involve?

Answer 16

Ligation of DNA fragments into a plasmid vector

Question 17

What do plasmid vectors usually carry?

Answer 17

Antibiotic resistance, which is shared between strains of bacteria

Question 18

How are plasmids used to grow a large amount of small DNA fragments?

Why is this needed?

Answer 18

1) Engineer in many enzyme cut sites (to form a multiple cloning site)
2) Digest the plasmid vector with the required restriction enzyme
3) Insert in the DNA of interest - create a recombinant plasmid
4) Insert the plasmid back into the bacteria - each cell will make about 50 copies of the plasmid
5) Single colony lifted off the plate to start a liquid culture
6) Plasmid purified from the bacteria and stored or analysed

Needed in order to make many copies of a DNA fragment - to be able to study

Question 19

What is a ‘multiple cloning site’?

Answer 19

DNA region within a plasmid which contains multiple UNIQUE restriction enzyme cut sites - to allow foreign DNA to be inserted

Question 20

How much DNA can plasmids hold?

What happens if too much is added?

Answer 20

<30 kilobases

If too much - bacteria get sick, as they don’t have enough energy to produce that much DNA

Question 21

What can be used to add in more DNA to clone it? (2 things)

How much DNA can they hold?

What is the problem with these?

Answer 21

1) Bacterial Artificial Chromosome (<300 kilobases)
2) Yeast Artificial Chromosome (<3 megabases)

Larger chromosomes are more fragile and harder to work with

Question 22

What is transformation?

Answer 22

Inserting the plasmid (containing the DNA of interest) into the bacteria

Question 23

How is bacteria transformed?

Answer 23

By creating temporary holes in the cell membrane of the bacteria and mixing it with the plasmid containing the DNA

Question 24

How are holes made in the bacterial membrane, in order for the plasmid to be incorporated into it?

Answer 24

Electroporation - electric charge makes holes

OR by

Chemical treatment

Question 25

How do you select for bacteria that have taken up the plasmid?

Answer 25

By treating the bacteria on antibiotic plates - as the plasmid contains the gene for antibiotic resistant gene

Bacteria without the plasmid will die

Question 26

What is cloning?

Answer 26

Making multiple, identical copies of a single DNA fragment (plasmid)

Question 27

Where do we get DNA to start with to use in the lab? (2 places)

Answer 27

1) Library of genomic clones

2) Library of cDNA clones from mRNA

Question 28

What does a genomic library contain?

Answer 28

Fragments of genomic DNA - ALL the genes in the genome

Question 29

How is a genomic library formed?

Answer 29

By digesting DNA from tissue (using restriction enzymes) and cloning fragments in plasmids

If this is done enough times - get the entire genome

Question 30

What are the advantages of a genomic library?

Answer 30

Contains all the REGULATORY sequence (introns)

So can study transcriptional regulation

Question 31

What does a cDNA library contain?

Answer 31

Genes which are expressed in different cells - represents all the mRNA of a given cell type

Question 32

What are the advantages of a cDNA library?

Answer 32

Can compare the genes expressed in normal tissue and diseased tissue

Can identify genes involved in disease

Question 33

How is a cDNA library formed?

Answer 33

1) Extract mRNA from a cell
2) Using reverse transcriptase make cDNA
3) Ligate cDNA into a plasmid vector and transform into bacteria
4) Grow the bacteria culture and purify out the DNA clone

Question 34

Where is reverse transcriptase found?

Answer 34

In retroviruses:
RNA into ssDNA
ssDNA into dsDNA

Question 35

What is cDNA?

Answer 35

DNA made from mRNA - doesn’t contain any introns/promoters/regulatory elements (only the exons)

Question 36

What is the ‘transcriptome’?

Answer 36

All of the mRNA in a cell (all of the genes expressed)

Different in different cells

Question 37

When making a cDNA or genomic library, what is it important to ensure?

Answer 37

That there is only:
One insert in each plasmid
One plasmid in each bacteria
One bacteria starting each colony

So that one bacteria is representing ONE mRNA

Question 38

What types of genes will be expressed by different colonies when making a cDNA library?

Answer 38

1) Housekeeping genes

2) Tissue specific genes

Question 39

Why when making cDNA libraries, do you end up with many colonies of housekeeping genes?

Answer 39

These genes are more common and are highly transcribed, so there is many copies of the mRNA in the cell

Question 40

What are ESTs?

How are they used?

Answer 40

Expressed Sequence Tags:

• Small pieces of DNA generated by sequencing randomly selected clones from a cDNA library
• Used to identify what DNA is present in the colony and particular genes of interest

Question 41

What is a genomic library useful for?

Answer 41

Sequencing genomes

Question 42

When making genomic libraries, what is it possible to get at the end?

Answer 42

An individual bacteria clone which represents the entire genome

Question 43

What is the process of dideoxy terminator sequencing?

Answer 43

1) Denature (heat to 100 degrees) the template (DNA which want to identify) to make it single stranded
2) Allow the DNA to cool with a primer
3) DNA synthesis reaction with DNA polymerase, dNTPs and a ddNTP of a certain base (A,G,T or C) - do this in 4 different tubes
4) Different strands will terminate at different positions
5) Run ALL the samples of the gel - forms separate the bands, depending upon the size of the fragment
6) Can see the full length of the DNA as the DNA fragment is COMPLIMENTARY to the ddNTP sequence

Question 44

Describe the primer, added in dideoxy terminator sequencing

Answer 44

Short, single stranded DNA that can be easily synthesised

Designed to anneal against the edge of the vector

Extended by DNA polymerase

Question 45

What are ddNTPs and how are they different to dNTPs?

Answer 45

dNTPs have -OH at the 3’ end - so that oxygen can join to the phosphate and the DNA can elongate

ddNTPs have -H at the 3’ end (no O to join to phosphate) - Cannot be elongated and the DNA polymerase falls off
- Termination of the DNA sequence

Question 46

What is the process of AUTOMATED dideoxy terminator sequencing?

Answer 46

1) Label each ddNTP with a different fluorescent dye
2) Termination will be labelled in a colour corresponding to the nucleotide which terminated it
3) As pass through the gel - camera takes pictures of each band and measures its intensity (one position over time, not the whole gel)
4) Produces a graph (trace) showing colour intensity over time

Question 47

What size DNA can automated dideoxy terminator sequencing analyse?

What can be used if the size of the DNA is above this?

Answer 47

<1000 (1kb)

If above 1kb, can use other methods:
1) Progressive sequencing

2) Shotgun sequencing

Question 48

What is the process of progressive sequencing?

Answer 48

1) From a GENOMIC library, sequence the ends of the clones, using primers from the vector
2) Synthesise primes on each end - reading in
3) Design a primer based upon the new sequence - another round of sequencing is performed
4) Keep doing this until the primers meet in the middle - eventually get sequence of the whole fragment

Question 49

What is the full process of determining the function o DNA in the genome?

Answer 49

1) Source DNA or mRNA
2) Insert into plasmids and clone
3) Extract a sample of interest (can do this be sequencing the end - ESTs
4) Make a library (genomic or cDNA)
5) Sequence the DNA (dideoxy or progressive/shotgun for larger pieces of DNA)

Question 50

Why in progressive sequencing must primers of the VECTOR be used?

Answer 50

The vector has a known sequence

Question 51

What is needed in order to sequence a genome?

Answer 51

Many BAC clones (bacterial artificial chromosome), which can be localised to particular regions of the genome - chosen for sequencing

Question 52

What are the advantages of shotgun sequencing?

Answer 52

Requires no thought - automated primer design

Question 53

What are the disadvantages of shotgun sequencing?

Answer 53

Need to sequence more than 6X the size of the genome to get large contigs
Always be gaps

Question 54

What is the process of shotgun sequencing?

Answer 54

1) Make genomic plasmid libary
2) Sequence just the ENDS of the inserts (using a primer of the vector)
3) Use the same primer for the ENTIRE library (matches the vector - same throughout library)
4) End up with many random sequences
5) Short random sequences are assembled by a computer into a contig (continuous sequence) -based on OVERLAP of the small sequences

Question 55

How are shotgun sequencing and progressive sequencing used?

Answer 55

In parallel