lectures 12-17

Question 1

what are the key features which distinguish prokaryotes from eukaryotes?

Answer 1

• condensed free DNA
• circular chromosome
• unique DNA
• contiguous genes
• no introns
• co-transcribed groups of genes
• coupled transcription and translation
• chromosome segregation as an active process (not regulated)
• directional gene transfer
• diploids unstable

Question 2

what are merozygotes/merodiploids?

Answer 2

a prokaryotic cell which is temporarily a diploid, when DNA is transferred in and there is temporarily 2 copies of a gene

Question 3

what is: transformation, transduction and conjugation?

Answer 3

transformation: movement of extracellular DNA into the cell
transduction: bacteriophage dependent genetic exchange
conjugation: plasmid dependent exchange involving transposons

Question 4

what are the technical advantages of using bacteria?

Answer 4

• easy to grow
• powerful selection systems (easy to measure change)
• grow rapidly
• clonal growth

Question 5

what is meant by clonal growth?

Answer 5

all cells in the colony are identical

Question 6

give the features of the E.coli chromosome

Answer 6

• single dsDNA molecule in a 430mm circle
• 4.639 x10^6 bp
• DNA is supercoiled

Question 7

describe the features of nucleoids

Answer 7

• non membrane bound
• found in growing cells in centre
• replication causes them to ‘explode’ in loops
• blockage of replication causes them to compact

Question 8

where does chromosome replication begin and terminate?

Answer 8

oriC and terC

Question 9

what is the difference between slow growth chromosome replication and fast growth?

Answer 9

slow growth: single replication fork

fast growth: multiple replication forks

Question 10

what are the properties of plasmids?

Answer 10

• replicate autonomously
• genes encode protein and RNA
• used for recombinant DNA technology

Question 11

what are the types of plasmids?

Answer 11

• F plasmids: involved in transmission of plasmids from one cell to another
• Resistance plasmids
• tumour induction plasmids
• symbiosis plasmids
• virulence plasmids: responsible for enterotoxin and haemolysin

Question 12

what is a replicon?

Answer 12

a self-regulating, freely-replicating element

Question 13

what are the key features of plasmid replication?

Answer 13

characteristic fixed copy number per cell
copy control genes located next to oriV
related plasmids cannot coexist in the cell

Question 14

outline phage infection and lysis

Answer 14

adsorption to cell -> injection of DNA -> DNA replication + gene expression -> assembly of new phage particles -> cell lysis and release

Question 15

what is the basis for transduction?

Answer 15

mistakes in phage packaging; DNA from host packaged into phage, upon injection into new host, this DNA becomes part of host genome

Question 16

describe the lysogenic lifecycle

Answer 16

adsorption -> injection -> DNA circularises by ligation of cohesive ss ends -> site-specific recombination between phage genome and cell chromosome -> phage genome incorporated into chromosome with phage genes switched off

Question 17

what does stimulation of prophage cause?

Answer 17

• accurate excision of phage genome
• aberrant excision causing phage genome to be excised with flanking chromosomal DNA, so that phage particle carries bacterial genes

Question 18

what are insertion sequences? what enzyme do they require?

Answer 18

discrete DNA segments with inverted repeats

transposase

Question 19

what is meant by the term ‘operon’?

Answer 19

when multiple genes are expressed at the same time via a single mRNA

Question 20

how does coupled transcription and translation occur in prokaryotes?

Answer 20

1) RNA polymerase binds, initiating the promoter. transcription occurs
2) ribosomes immediately attach as soon as the shine-delgarno sequence is recognised, translation occurs immediately

Question 21

explain how bacterial transformation occurs

Answer 21

1) transfer of DNA from donor to recipient produces a partial diploid
2) homologous DNA on transferred DNA pairs with homologous regions of recipient DNA
3) 2 reciprocal crossovers occur causing a region of recipient DNA to be replaced with donor DNA
4) linear reciprocal recombinant product is degraded

Question 22

explain how plasmid conjugation occurs

Answer 22

pili/fimbriae on the surface allow mating pairs to form. genes are transferred from oriT in ssDNA transfer in 1-2 minutes

Question 23

explain how artificial transformation works

Answer 23

• cells permeabilised for DNA uptake using CaCl2, spheroplasts or electroporation
• homology is not required, any gene can be inserted

Question 24

what are the steps for gene cloning?

Answer 24

cut DNA with enzyme -> insert into a vector -> transport into host

Question 25

what are palindromes?

Answer 25

recognition sequences for restriction endonucleases

Question 26

what is the role of modification enzymes?

Answer 26

protects own DNA from cleavage by methylation of bases in the restriction endonuclease sites

Question 27

describe the features of restriction endonucleases

Answer 27

• recognise and cut up specific DNA sequences
• have 2-fold rotational symmetry
• produce staggered cuts, leaving cohesive ssDNA ends

Question 28

how is the DNA rejoined after it is cut with a restriction endonuclease?

Answer 28

• 5’ sticky ends are left
• bases anneal and ligation occurs via ligase
• leaving recleavable sites

Question 29

what is the role of ligase (restriction endonuclease)?

Answer 29

facilitates the joining of 2 DNA strands by catalysing the formation of phosphodiester bonds

Question 30

what are the essential features of cloning vectors?

Answer 30

• must be able to replicate in the host cell, maintaining appropriate copy number
• must have an appropriate restriction enzyme site
• must have an appropriate method of introduction into the host cell
• must have a genetic selection marker
• must identify recombinants

Question 31

what is blue-white screening?

Answer 31

allows us to differentiate between recombinants and vectors alone using LacZ gene for B-Galactosidase

Question 32

How does blue-white screening identify recombinants?

Answer 32

• LacZ encodes B-galactosidase, which converts colourless X-Gal into a blue compound
• recombinant contains fragments which insertionally inactivate LacZ = colourless plate
• vectors still produce blue compound

Question 33

how is a genomic library made?

Answer 33

take total genomic DNA -> cut into random fragments -> cut vector with same enzyme to give sticky ends -> anneal + ligate

Question 34

what are the advantages and disadvantages of large inserts when building a genomic library?

Answer 34

• fewer clones required for the library to be representative

- plasmids have small vector capacity, other vectors must be used

Question 35

what are the advantages and disadvantages of small inserts when building a genomic library?

Answer 35

• plasmids can be used

- more clones required for it to be representative

Question 36

what type of organism is yeast artificial chromosome useful as a vector for building a genomic library? why?

Answer 36

eukaryotes; yeast is eukaryotic, plus vector capacity is high, 200-2000kb compared to 10kb for a regular plasmid. useful for creating a representative library in organisms with a large genome

Question 37

how is the number of clones for a representative genomic library calculated?

Answer 37

N= ln(1-P) / ln(1-f/n)

Question 38

why are more clones required than the minimum amount to cover all the bases in a chromosome?

Answer 38

plasmid insertion is not 100% effective

Question 39

what do PHYSICAL methods of identifying clone of interest rely on?

Answer 39

base sequence complimentarity; you must know the identity of the gene you are investigating

Question 40

what do BIOLOGICAL methods of identifying clone of interest rely on?

Answer 40

screen for phenotype by complementation

Question 41

explain hybridisation as a method of identifying clone of interest and state what factors influence it

Answer 41

complementary strands find each other e.g. a probe and the clone.
influenced by temperature, salt concentration and sequence

Question 42

what result of a colony blot is indicative of positive hybridisation?

Answer 42

black spots

Question 43

how is a ‘specialist library’ made?

Answer 43

mRNA -> spliced mRNA -> reverse transcriptase used to make a DNA copy of mRNAs -> remove mRNAs -> dsDNA made from DNA using a polymerase

Question 44

why are ‘enriched/specialist libraries’ not used for prokaryotes?

Answer 44

prokaryotes do not have introns; removing non-coding DNA offers no advantage

Question 45

how is immunoblotting used for specific bacterial genome libraries?

Answer 45

1) transfer colonies (clones) to nylon filter
2) lyse bacteria
3) bind proteins from lysed bacteria to nylon
4) add labelled antibody-sticks to desired protein
5) detect label

Question 46

outline sanger sequencing

Answer 46

1) shear bacterial chromosome so it forms many fragments of different sizes which overlap
2) fragments inserted into a vector- forming a library
3) add individual clones to individual wells
4) sequence each individual clone

Question 47

what is de novo assembly?

Answer 47

when overlapping fragments are are assembled like a jigsaw until the whole genome is complete

Question 48

aside from de novo, which other types of assembly are used?

Answer 48

assembly to a reference genome: when fragments are aligned against a known reference
sequence assembly: when a computer is used to assemble fragments

Question 49

outline WGS by Next Generation Sequencing

Answer 49

1) make a fragment library, no vector required. attach an adapter to fragments
2) adapter sticks to solid matrix
3) amplify individual genome fragments on the matrix
4) all fragments sequenced at the same time

Question 50

what is the goal of annotating the genome (WGS)?

Answer 50

determining the position of coding genes and other sequence motifs

Question 51

how does computational analysis result in annotation of the genome?

Answer 51

computer recognises start, stop and sense codons, alongside shine-delgarno sequences. compares them to other sequences on database to establish homology

Question 52

why do bacteria need tightly controlled gene expression?

Answer 52

economy- efficient RNA/protein synthesis
preventing clashes in physiological processes
developmental pathways
responding to environmental conditions

Question 53

at which points can gene expression be controlled in bacteria?

Answer 53

transcriptional: via transcription factors
post-transcriptional: via sRNA
post-translational: via enzymes

Question 54

which elements are responsible for control of gene expression?

Answer 54

regulatory genes: produce proteins which control transcription
transcription factors: act on promoters of regulated genes
effectors: inducers and co-repressors which control a regulon

Question 55

what is a regulon?

Answer 55

group of genes controlled by specific transcription factors

Question 56

why does diauxic growth occur when E.coli is grown in a substrate containing glucose and lactose?

Answer 56

lac genes are repressed by glucose, when glucose is used up, lactose catabolic enzymes are produced and lactose is metabolised

Question 57

which enzymes are required for lactose utilisation in E.coli?

Answer 57

permease: transports lac into cell, encoded by lacY
B-galactosidase: breaks down lac into glucose and galactose, encoded by lacZ
transacetylase: unknown function, encoded by la
cA

Question 58

what is the structure of the lac operon?

Answer 58

LacZ-LacY-LacA

Question 59

what is the role of lac| and LacO in controlling activation of the lac operon?

Answer 59

LacI: DNA binding protein (repressor)
LacO: DNA consensus sequence where a repressor binds, blocking RNA polymerase and thus, transcription `

Question 60

explain positive control of the lac operon

Answer 60

catabolite activating protein senses glucose levels and binds to the promoter to activate transcription in the presence of cAMP (low glucose)

Question 61

briefly outline how two component signal transduction systems can alter gene expression

Answer 61

1) signal sensed by histidine protein kinase
2) conformational change causes them to dimerise and phosphorylate a his
3) His passed to a conserved aspartate on a DNA binding protein
4) DNA binding proteins dont bind unless phos.

Question 62

how do positively-acting small RNAs result in post-transcriptional gene expression control?

Answer 62

stimulate translation by unmasking ribosome binding sites

stabilise mRNA

Question 63

how do negatively-acting small RNAs result in post-transcriptional gene expression control?

Answer 63

inhibit translation by occluding ribosome binding site or stimulating degradation of mRNA